CA2537290A1 - Delivery of physiological agents with in-situ gels comprising anionic polysaccharides - Google Patents

Delivery of physiological agents with in-situ gels comprising anionic polysaccharides Download PDF

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CA2537290A1
CA2537290A1 CA002537290A CA2537290A CA2537290A1 CA 2537290 A1 CA2537290 A1 CA 2537290A1 CA 002537290 A CA002537290 A CA 002537290A CA 2537290 A CA2537290 A CA 2537290A CA 2537290 A1 CA2537290 A1 CA 2537290A1
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animal
gel
pectin
solid
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CA2537290C (en
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Yawei Ni
Kenneth M. Yates
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Carrington Laboratories Inc
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Yawei Ni
Kenneth M. Yates
Carrington Laboratories, Inc.
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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/20Pills, tablets, discs, rods
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/0012Galenical forms characterised by the site of application
    • A61K9/0019Injectable compositions; Intramuscular, intravenous, arterial, subcutaneous administration; Compositions to be administered through the skin in an invasive manner
    • A61K9/0024Solid, semi-solid or solidifying implants, which are implanted or injected in body tissue
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides
    • A61K38/16Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • A61K38/17Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
    • A61K38/18Growth factors; Growth regulators
    • A61K38/1825Fibroblast growth factor [FGF]
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K39/02Bacterial antigens
    • A61K39/05Actinobacteria, e.g. Actinomyces, Streptomyces, Nocardia, Bifidobacterium, Gardnerella, Corynebacterium; Propionibacterium
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K39/12Viral antigens
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K39/39Medicinal preparations containing antigens or antibodies characterised by the immunostimulating additives, e.g. chemical adjuvants
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K47/00Medicinal preparations characterised by the non-active ingredients used, e.g. carriers or inert additives; Targeting or modifying agents chemically bound to the active ingredient
    • A61K47/30Macromolecular organic or inorganic compounds, e.g. inorganic polyphosphates
    • A61K47/36Polysaccharides; Derivatives thereof, e.g. gums, starch, alginate, dextrin, hyaluronic acid, chitosan, inulin, agar or pectin
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/06Ointments; Bases therefor; Other semi-solid forms, e.g. creams, sticks, gels
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/48Preparations in capsules, e.g. of gelatin, of chocolate
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P17/00Drugs for dermatological disorders
    • A61P17/02Drugs for dermatological disorders for treating wounds, ulcers, burns, scars, keloids, or the like
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/12Antivirals
    • A61P31/14Antivirals for RNA viruses
    • A61P31/16Antivirals for RNA viruses for influenza or rhinoviruses
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • A61P37/02Immunomodulators
    • A61P37/04Immunostimulants
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/51Medicinal preparations containing antigens or antibodies comprising whole cells, viruses or DNA/RNA
    • A61K2039/525Virus
    • A61K2039/5252Virus inactivated (killed)
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/54Medicinal preparations containing antigens or antibodies characterised by the route of administration
    • A61K2039/541Mucosal route
    • A61K2039/543Mucosal route intranasal
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/555Medicinal preparations containing antigens or antibodies characterised by a specific combination antigen/adjuvant
    • A61K2039/55505Inorganic adjuvants
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/555Medicinal preparations containing antigens or antibodies characterised by a specific combination antigen/adjuvant
    • A61K2039/55511Organic adjuvants
    • A61K2039/55583Polysaccharides
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K2039/70Multivalent vaccine
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B82NANOTECHNOLOGY
    • B82YSPECIFIC USES OR APPLICATIONS OF NANOSTRUCTURES; MEASUREMENT OR ANALYSIS OF NANOSTRUCTURES; MANUFACTURE OR TREATMENT OF NANOSTRUCTURES
    • B82Y5/00Nanobiotechnology or nanomedicine, e.g. protein engineering or drug delivery
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2760/00MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA ssRNA viruses negative-sense
    • C12N2760/00011Details
    • C12N2760/16011Orthomyxoviridae
    • C12N2760/16111Influenzavirus A, i.e. influenza A virus
    • C12N2760/16134Use of virus or viral component as vaccine, e.g. live-attenuated or inactivated virus, VLP, viral protein

Abstract

In-situ gelling compositions for delivering pharmacologically active substances to the tissues, body fluids, and mucosal surfaces of animal patients in the form of liquids, solids and powders, comprising anionic polysaccharides and especially low methoxyl pectins as gelling agents, methods of preparation, and method of use of the in-situ gelling compositions for the delivery and sustained release of a physiologically active agent, and especially vaccine antigens, to the tissues and mucosal surfaces of an animal.

Description

DELIVERY OF PHYSIOLOGICAL AGENTS WITH IN SITU GELS
COMPRISING ANIONIC POLYSACCHARIDES
REFERENCE TO RELATED APPLICATIONS
This application is a continuation-in-part of, and claims priority to U.S.
Utility Application Serial Number 10/652,622, filed August 29, 2003, the entire disclosure of which parent application is hereby incorporated herein in its entirety by this reference.
BACKGROUND OF THE INVENTION
A variety of polymer-based drug delivery systems for achieving sustained or controlled drug release have been described (See Langer, Nature, 392 (supplement), 5-10, 1998 and references therein). The goal of many of those systems was typically one or more of prolonging drug release, improving drug bioavailability, and/or providing non-injectable drug delivery systems that improve patient compliance and comfort.
The polymers, either synthetic or natural, provide delivery of the various agents by various mechanisms, depending on the properties of the polymer.
The polymer-based systems have been variously formulated as, for example, a liquid, a suspension, an emulsion, a powder comprising microparticle and/or microspheres, a film, or a tablet. The compositions have been administered via various routes or methods, including injection, topical administration, or administration to a mucosal surface of the eye, vaginal, anus, stomach or intestines, oral and nasal cavities, or the lungs. The polymer-based systems have been used to deliver a variety of physiologically active agents, including therapeutics and prophylactic agents, including small molecule- or protein-based drugs, nucleic acids, polysaccharides, fatty acids and esters, cells and fragments thereof, viruses, and vaccines for prevention of infectious diseases.
In many prior art polymer-based systems for drug delivery, prior to administration to the patient, the drugs and/or other pharmacologically active substances are encapsulated in polymers or gels that may absorb water, but are substantially water insoluble. Gels are a solid or deformable jelly-like semi-solid comprising a porous three dimensional network of polymer molecules, containing within the pores of the polymer network a reversibly absorbed liquid (i.e. a discontinuous liquid phase). Gels can often contain andlor absorb large and/or predominant amounts of a liquid, which is often water or another aqueous fluid, including a biological fluid, but the network of gelled polymer molecules are nevertheless substantially insoluble in the bulk liquid or biological fluid.
The individual polymer molecules can be cross-linked to form the insoluble network in various ways depending on the nature of the polymer. The cross-links between the polymer molecules can result from covalent bonds, coordinate bonds, or ionic interaction, or even weaker intermolecular forces such as hydrogen bonding.
Various synthetic and natural polymers have also been used in drug delivery formulations employing polymers such as starches and modified celluloses, gellan, chitosan, hyaluronic acids, pectins, and the like. For example, U.S. Patent No. 4,613,500 disclosed various powdery pharmaceutical compositions for nasal administration comprising various water soluble and water insoluble polymers, including pectins, but the use of low methoxyl pectins that could form calcium cross-linked gels was not described or suggested. U.S. Patent Nos. 5,707,644 and 5,804,212 recently disclosed the use of a long list of polymers, including pectins, in formulating bioadhesive microspheres of a diameter of less than 10 microns for the delivery of pharmaceuticals, peptides, and antigenic vaccines to nasal surfaces, and suggested that the compositions could be formulated with polymeric materials that could gel in-situ, but did not teach or suggest the use of low methoxyl pectins for in-situ gellation.
"In-situ" gelation has been described in some prior art pharmaceutical drug delivery systems and compositions, and involves gel formation at the site of application after the composition or formulation has been administered to the patient by application to a mucosal surface, tissue, wound, parental cavity, etc. "In-situ" gelling compositions form a bioadhesive gel only after contact with the tissues or body fluids. The polymer molecules of the in-situ gelling composition itself are typically not cross-linked at all, or not sufficiently cross-linked prior to application to the biological site of application so as to be in the form of water insoluble gel prior to application to the biological site, but upon or shortly after application to the biological site, polymer cross-linking typically occurs so as to result in the formation of a cross-linked polymer gel network that comprises water and/or the biological fluids within its porous network structure. The in-situ gel, once formed, is substantially and/or effectively insoluble in water or the biological fluids, at least under normal physicological conditions . Absorption of water and/or bodily fluids normally occurs concurrently with the process of in-situ gellation, but the formation of the insoluble polymer network upon administration to the site, rather than the mere absorption of water or fluids, is the primary phenomenon that defines ira-situ gellation.
Polymers capable of in-situ gelation have been previously described, including Poloxamer, Pluronics (Vadnere et al., Int. J. Pha~m., 22, 207-218, 1984), various copolymers such as PEO-PLLA and PEG-PLGA-PEG (Jeong et al., Nature 388, 860-862, 1997; Jeong et al., J. Cotatrolled Release 63, 155-163, 2000), cellulose acetophthalate latex (Gunny et al. J. Controlled Release 353-361, 1985), Gelrite (Rozier et al., Int. J. Pham. 57, 163-168, 1989), Carbopol, and Matrigel. The gel formation is induced by temperature change (Poloxamer, Pluronics, PEO-PLLA diblock copolymer, PEG-PLGA-PEG
triblock copolymer, and Matrigel), pH change (cellulose acetophalate latex and Carbopol), or reaction with mono- or di-valent cations (Gelrite and/or alginates). However, most of them require a high polymer concentration for in-situ gel formation (>20%) (Poloxamer, PEO-PLLA diblock copoly, PEG-PLGA-PEG triblock copolymer, cellulose and acetophalate latex). The thermally gelling polymers (Poloxamer, Pluronics, PEO-PLLA diblock copolymer, PEG-PLGA-PEG triblock copolymer, and Matrigel) also have the disadvantage of gelling before administration due to temperature change during packaging or storage.
Unfortunately some of these polymers are not biodegradable such as Poloxamer or require manipulation of the temperature before administration (PEO-PLLA diblock copolymer) or during formulation (Pluronics and Gelrite). An ophthalmic izz-situ gelling drug delivery formulation consisting of a mixture of Carbopol and Platonic was found to be more effective than formulations consisting of either one. However, Platonic is used at 14%
(Lin and Sung, .Iourrzal of Cofztrolled Release 69, 379-388, 2000). Such polymers are ' therefore not well suited for medical applications in humans and animals.
Furthermore, many of these polymers form only a hydrogel which is a viscous but still flowing solution (e.g., Poloxamer and Pluronics).
Irz-situ gelation compositions have been disclosed in U.S. Patent No.
5,958,443, which discloses liquid compositions comprising a drug, a film forming polymer and a gel forming ionic polysaccharide. These compositions employed two separately applied components, the first component being a solution of "extraneous" crosslinking divalent or multivalent canons, which is applied to the intended site of biological application. In a separate step (which may occur before, after or concurrently with the application of the first component solution) a second liquid component solution comprising the drug, film forming polymer and an ionic polysaccharide (such as an alginate) is separately applied to the intended site, with the result of a chemical cross-linking reaction between the ionic polysaccharide and the divalent or multivalent canons, at.the site of biological application to form a cross-linked and insoluble and bioadhesive izz-situ gel. The '443 patent describes pectins as one of many film forming polymers, rather than as a gel forming ionic polysaccharide.
Pectins are a biodegradable heteropolysaccharide isolated from plant cell walls having carboxylic acid side groups on the galacturonic acid residues within the polymer.
All vegetables and fruits that have been examined appear to contain pectins.
Pectins from sugar beets, sunflowers, potatoes, and grapefruits are just a few other well known examples. In virtually all natural pectins, more than 50% of the carboxylic acid groups of pectin are present in the form of methyl esters, and such pectins are termed "high methoxyl" (HM) pectins. Pectins wherein less than 50% of the carboxylic acid groups are methyl esterified (i. e. low methoxyl (LM) pectins) are uncommon in nature, and typically are prepared by synthetic processes from natural HM pectins. It is known in the art that LM pectins are capable of forming gels by coordination/crosslinking with divalent or multivalent metal ions such as calcium ions. The chemistry and biology of pectins have been extensively reviewed (Pilnik and Voragen, Advances in plant biochemistry and biotechnology l, 219-270, 1992; Voragen et al, Ita Food polysacchaYides and their applications. pp 2~7-339. Marcel Dekker, Inc. New York, 1995; Schols and Voragen, In Pr~og~ess in Biotechnology 14. Pectins and pectinases, J. Visser and A.G.J.Voragen (eds.).
pp. 3-20. Elsevier Science Publishers B.V. Amsterdam, 1996).
U.S. Patent 6,432,440 recently disclosed the use of LM pectins in liquid pharmaceutical formulations adapted to gel on contact with mucosal surfaces.
U.S. Patent 6,342,251 disclosed the use of a wide variety of polymers, including pectins in liquid and solid formulations fox nasal administration of drugs suitable for the treatment of erectile dysfunction. The entire descriptions of U.S. Patent Nos. 6,432,440, 6,342,251, 5,707,644, and 5,04,212 are hereby incorporated herein by this reference, in their entireties, for their teachings regarding the formulation of in-situ gelling pharmaceutical compositions, the pectins used to prepare such compositions, and the administration of the compositions to animals and humans.
Anderson et al. (T~accihe, 19, 840-843, 2001) described a nasal powder vaccine against rinderpest for administration to animals made by blending of lyophilized antigen with 4 mm nylon balls and mixing with talcum powder (calcium carbonate). Maa et al.
(U.S. Patent Publication No. 2002/0120228) describes gel-forming powder vaccine compositions comprising aluminum salt with an antigen absorbed therein, a saccharide, an amino acid, and a colloidal substance that can include a polysaccharide that is administered to the patients via transdermal delivery.
Powders containing small particles of less than 5 microns have also been used for pulmonary drug delivery to the deep lung. Lactose particles have been used as a coarse particle bulk carrier for physical blending with micronized particles of drugs for such pulmonary drug delivery applications (Malcomson and Embleton, Pharmacuetical Science and Technology Today, Vol 1 (9), 394-398, 1998). LiCalsi et al ( laccirae, Vol 19, 2629-2636, 2001) prepared a lyophilized live measles pulmonary powder vaccine. In above cited prior art, the drug or antigen is physically mixed with or dispersed on the surfaces of carrier particles and is not dispersed throughout the lactose matrix.
Recently Illum et al have reviewed state of the art of nasal delivery of drugs and vaccines in two articles, i. e., "Nasal Vaccines" in Advanced Drug Delivery Reviews, Vol. 51, pages 21-42, 2001, and in "Nasal Drug Delivery: New Developments and Strategies" published at www.dru~discover~~toda .com, in Vol. 7, No. 23, December 2002.
Both articles discuss the use of polymeric and/or high viscosity bioadhesive materials to formulate powders for the delivery of nasal vaccines and/or drugs, but neither article discloses or suggests that those nasal powder vaccine compositions should comprise moderate to large amounts of highly water soluble excipients and/or diluents.
The entire descriptions of the above-referenced patents and articles are hereby incorporated herein by this reference, in their entireties, for their teachings regarding the formulation of nasal powder drug delivery compositions, and the methods of administration of the compositions to animals and humans.
Biotechnology and associated methods for delivering drugs and related biopharmaceutical agents has been a subject of intense studies over recent years, but only limited progress has been made in the area of delivery of these agents, especially biopharmaceutical agents. Biopharmaceutical agents, such as peptides, proteins, nucleic acids, vaccines, antigens, and bioengineered cells, microorganisms, and viruses tend to be unstable, both in storage and after application. Injection of such agents into the tissues of an animal or human is sometimes successful, but is often economically and aesthetically undesirable, especially if frequent administrations are required. Many biopharmaceutical agents, especially the higher molecular weight and more polar agents such as proteins, nucleic acids, antigens, etc., have in the past only been poorly absorbed if administered orally or to mucosal membranes. Administration to nasal mucosal surfaces can be particularly challenging because of the rapid turnover and clearance of nasal mucosal fluids, which are believed to be cleared from the nasal cavity with a half life on the order of 15 minutes. ~nce successfully administered to the animal, many biopharmaceutical agents are rapidly degraded before they can effectively exert their desired function, and need protection from degradation andlor the benefits of time release formulations.
Therefore, many long felt but as yet unftilfilled needs exist in the area of administration of biopharmaceutical agents.
Thus, a great need exists for a simpler, improved, and/or more efficient ira-situ gelling compositions for drug andlor biopharmaceutical agent delivery.
SUMMARY OF THE INVENTION
The inventions disclosed herein relate to the delivery of physiologically active agents to the tissues or body fluids of animals, including humans. The inventions relate to methods of making and administering pharmaceutical compositions comprising polysaccharides, including pectins, that form an "ira-situ" gel comprising the physiologically active agents when contacted with the tissues or body fluids.
The compositions of the invention can be administered to the animal asld its tissues and body fluids in the form of liquids, or solids, or powders comprising microspheres or microparticles of selected size ranges.
The compositions of the invention can be formulated to improve the stability and/or storage life of sensitive biopharmaceuticals including peptides, proteins, antigens, vaccines, nucleic acids, viruses, whole cells or fragments thereof. The compositions can be administered by injection into body tissues, organs, or cavities, so as to contact body fluids such as blood or serum and gel therein, or the compositions can be administered to the various mucosal surfaces of the body, including those of the oralldigestive tract, or the nasal and lung cavities. The ira-situ gels, once formed can slow and/or modulate the release, or improve the bio-availability of the physiologically active agents.
In some embodiments, administration of biomolecules such as vaccines, antigens, peptides, andlor proteins via in-situ gels formed in the nasal cavity can be unexpectedly improved by such techniques of administration.
In some aspects of the invention, inclusion of or co-administration of solid or gel inducing agents and/or compositions comprising divalent or multivalent cations in the compositions can provide improved gel formations and provide a controlled drug release.
The features and benefits of the present invention can be illustrated by the following embodiments of the present invention.
In one aspect, the invention relates to a solid pharmaceutical composition for administering a physiologically active agent to an animal comprising:

a) one or more physiologically active agents in an amount effective to induce a physiological response in an animal; and b) one or more polysaccharides comprising subunits having anionic carboxylate or sulfate groups, and c) one or more solid polysaccharide gelling compositions comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal canon;
wherein the pharmaceutical composition is in a solid form that forms a gel when contacted with a tissue or body fluid of an animal.
In another aspect, the inventions relate to solid pharmaceutical compositions for achninistering a physiologically active agent to an animal comprising:
a) one or more physiologically active agents; and b) one or more pectic substances, wherein the pharmaceutical composition is a solid capable of forming a gel when contacted with a tissue or body fluid of an animal.
In a related aspect, the invention provides a composition for the sustained release of a physiologically active agent in an animal, wherein the composition is in a dry form comprising:
one or more physiologically active agents in an amount that exerts a physiological response in the body of an animal; and a pectic substance having a degree of methylation less than 30% and an average molecular weight of greater than 1 x 105 Daltons, in an amount effective to form a gel when the composition is contacted with a tissue or body fluid of the animal.

The invention also relates to methods for making the compositions of the invention.
In one such aspect, the invention relates to a method for preparing a dry composition for the sustained release of a physiologically active agent in an animal, comprising dissolving a mixture of a pectic substance and a physiologically active agent in a carrier to give a solution or dispersion, wherein the amount of the pectic substance is effective to gel ifa situ in the animal; and removing volatile components in the earner to give the dry composition.
The invention also relates to methods for administering solid or liquid pharmaceutical compositions that will gel on contact with the tissues or body fluids of an animal In one aspect, the invention relates to a method comprising administering to a tissue or body fluid of an animal, in any order or combination, the following components, a. one or more physiologically active agents in an amount effective to induce a physiological response in an animal;
b. one or more polysaccharides comprising subunits having anionic carboxylate or sulfate groups, and c. one or more solid gel inducing compositions comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal cation;
to form a gel in contact with the tissue or body fluids of the animal.
In the embodiment described immediately above, the a, b, and c components can be administered in any order, and the a and b components may be in the form of either a solid or a liquid solution, and any combination or sub-combination of the a, b, and c components may be administered simultaneously or in mixtures.
The invention also relates to liquid compositions that are capable of gelling when contacted with the tissues of body fluids of an animal, and methods for applying the compositions to the tissues and body fluids. In one such aspect, the invention relates to a method for administering a physiologically active agent to an animal, comprising:

a) providing a liquid solution or dispersion comprising i) liquid Garner, ii) a pectic substance having a degree of methylation of less than 30%
and an average molecular weight of greater than 4.6 x 105 Daltons, in an amount effective to gel the liquid solution or dispersion when applied to the tissues or body fluids of the animal, and iii) one or more physiologically active agents; and b) applying the liquid solution or dispersion to the tissues or body fluids of the animal to form a gel comprising physiologically active agent in contact with the tissues or body fluids.
In another aspect, the invention relates to a vaccine composition for administration to the nasal mucosa of an animal comprising powder particles that comprise a nano-dispersion of a. one or more antigens in an amount effective to induce an immune response response in an animal, and b. one or more pectins or a monovalent cation salt thereof having a degree of methylation less than about 30% and an average molecular weight of greater than about 1 x 105 Daltons;
wherein the powder particles can pass through a sieve having an opening size of about 250 ~M in diameter.
In some other aspects, the invention relates to methods for administering vaccine composition to an animals or a humans, in either solid or liquid forms, comprising administering a vaccine composition to the mucosal surfaces of the animal or human. In one such aspect the invention relates to a method for-vaccinating an animal, comprising the steps of a. providing one or more powder compositions comprising powder particles that can pass through a sieve having an opening size of about 250 ~M in diameter, and that comprise i) a pectic substance having a degree of methylation less than about 30% and an average molecular weight of greater than 1 x 105 Daltons, in an amount effective to form a gel when the composition is contacted with the mucosal surfaces of an animal;
ii) one or more antigens selected from the group consisting of a peptide, a protein, a nucleic acid, a carbohydrate, a live cell or microorganism, a dead cell microorganism, or a portion thereof, or a virus or a portion thereof, in an amount that is capable of inducing an active immune response in the animal; and b. administering the powder to the nasal tissues and/or nasal fluids of the animal to form a gel in contact with the tissues or body fluids, and c. inducing an active immune response to one or more of the antigens in the animal.
The foregoing discussion has outlined some of the more pertinent features of the present invention. These should be construed to be merely illustrative of some of the more prominent features and applications of the invention. Accordingly, a fuller understanding of the invention may be had by referring to the following Detailed Description.
BRIEF DESCRIPTION OF THE DRAWINGS
For a more complete understanding of the preferred embodiment of the present invention, reference is made to the following detailed description taken in conjunction with the accompanying drawings, wherein like numerals refer to like elements, wherein:

Figure 1 is a bar graph representing the relationship of NaCl to the calcium gelation of Aloe pectin.
Figure 2 shows the Aloe pectin in-situ gelation at various Aloe pectin concentrations with normal animal serum.
Figure 3A shows the Aloe pectin in-situ gelation in the presence of a HEC
thickener With normal animal serum.
Figure 3B shows the Aloe pectin in-situ gelation in the presence of a sodium alginate thickener with normal animal serum.
Figure 4 shows the slow release effect obtained with Aloe pectin ira-situ gel using a small organic. compound (fast green).
Figure 5 shows a bar graph representing the relationship between bFGF
treatment and cell number in a defined area.
Figure 6. The release rate of fast green from liquid or dried formulations.
Figure 6a shows results for an LM pectin, and Figure 6b shows results for a LMW aloe pectin.
The diameter of the diffusion circle around the formulation placed in the normal calf serum was measured over time, as described in Example 17.
Figure 7. Controlled protein release from powder formulations comprising a high molecular aloe pectin, and suspended in simulated nasal fluid, as described in Example 20.
Figure ~. Specific serum IgG response against DT-CRM antigen following intranasal delivery to rats of a powder vaccine formulation, as described in Example 22.
Figure 9. Improved in-situ gelation of pectin formulations in contact with normal calf serum is achieved by addition of extraneous calcium, as described in Example 24.
Figure 10. Serial cross sections of the nasal cavity of a mouse 4 h after intranasal delivery of an HMW Aloe pectin solution (0.5%, w/v), showing formation of gel on the nasal mucosal surfaces, as described in Example 26.

Figure 11. Serum IgG and lung IgA immunological responses of mice to nasal administration of liquid vaccine compositions comprising aloe pectin and a protein antigen (DT-CRM) (a and b) or an inactivated influenza split subvirion antigen (A/New Caledonia/20/99, H1N1) (c and d), as described in Example 29.
DETAILED DESCRIPTION
The present invention can be understood more readily by reference to the following detailed description of various embodiments of the invention and the Examples included therein and to the Figures and their previous and following description.
Before the present compounds, compositions, and/or methods are disclosed arid described, it is to be understood that this invention is not limited to specific starting materials, pharmaceutical agents or specific synthetic methods unless otherwise specifically indicated, as such can, of course, vary. It is also to be understood that the terminology used herein is fox the purpose of describing particular embodiments only and is not intended to be limiting.
DEFINITIONS
In the specification and Formulae described herein the following terms are hereby defined.
"Optional" or "optionally" means that the subsequently described event or circumstance may or may not occur, and that the description includes instances where said event or circumstance occurs and instances where it does not. For example, the phrase "optional excipient" means that the excipient may or may not be included in the composition.
It must be noted that, as used in the specification and the appended claims, the singular forms "a," "an" and "the" include plural referents unless the context clearly dictates otherwise. Thus, for example, reference to "an aromatic compound"
includes mixtures of aromatic compounds.

Often, ranges are expressed herein as from "about" one particular value, and/or to "about" another particular value. When such a range is expressed, another embodiment includes from the one particular value and/or to the other particular value.
Similarly, when values are expressed as approximations, by use of the antecedent "about," it will be understood that the particular value forms another embodiment. It will be further understood that the endpoints of each of the ranges are significant both in relation to the other endpoint, and independently of the other endpoint.
By "pharmaceutically acceptable" is meant a material that is not biologically or otherwise undesirable, i.e., the material can be administered to an individual along with the relevant active compound without causing clinically unacceptable biological effects or interacting. in a deleterious manner with any of the other components of the pharmaceutical composition in which it is contained.
By the term "effective amount" of a compound as provided herein is meant a sufficient amount of the compound to provide the desired regulation of a desired function, such as gene expression, antigen induced immune reaction, protein function, or a disease condition. As will be pointed out below, the exact amount required will vary from subject to subject, depending on the species, age, and general condition of the subject, the severity of the disease that is being treated, the particular agent used, its mode of administration, and the like. Thus, it is not possible to specify an exact "effective amount."
However, an appropriate effective amount can be determined by one of ordinary skill in the art using only routine experimentation.
A "Gel" as the term is defined and used herein is an elastic solid or deformable semi-solid comprising a porous three dimensional network of organic polymer molecules containing within the network a reversibly absorbed liquid. In the context of the present invention, the reversibly absorbed liquid typically comprises the liquid water, although other liquid materials may also be present. In the context of the present invention, the network of polymer molecules typically comprise polysaccharides having repeat units comprising carboxylate or sulfate groups, including pectins. In many embodiments of the present invention, at least some of the carboxylate or sulfate groups of adjacent polysaccharide chains coordinate to divalent or multivalent cations such as calcium or aluminum, to form a cation crosslinked three dimensional network of polysaccharide molecules that is substantially insoluble in pure water. The existence and identity of such cation-crosslinked and water insoluble gels can typically be experimentally confirmed by first placing a sample of the gel in pure, neutral water for at several hours to confirm that they retain their semi-solid form and are substantially water insoluble, but that the addition of metal cation chelating agents such as the sodium salts of ethylenediaminetetraacetic acid (EDTA) induces the gel to quickly dissolve by removal of the divalent or multivalent metal ions.
Gellation, as the term is used herein, refers to the formation of a gel that involves the formation of a cross-linked polymer network and absorption of the liquid and/or other materials into the cross-linked polymer network, to form a solid or semi-solid that is substantially insoluble in the bulk liquid. Ih-Situ gels are formed from suitable precursor polymers and liquids that typically comprise water, and then become cross-linked on or after contact with a tissue or body fluid, or a simulated tissue or body fluid so as to form a solid or semi-solid comprising a cross-linked polymer network and water derived from the tissue or body fluid.
A "Polymer" is a macromolecule formed by the covalent boding together of more than 10 divalent or multivalent subunits that are typically called monomers.
The polymers of the present invention comprise both natural polymers such as proteins, nucleic acids, polysaccharides, and the like, which may contain a relatively large number of different types of monomers, or man-made polymers such as polyacrylates that often only contain one or a small number of different monomers.
A "Gel-inducing agent" is an agent capable of causing a polymer or a polymer solution to form a gel. Gel inducing agents often induce gel formation by inducing crosslinking between polymer chains, which in the context of the present invention include salts of divalent and multivalent cations, which can crosslink carboxylate or sulfate substituent groups on the same or differing polysaccharide molecules.
An "Ionic polymer" is a synthetic or natural polymer having monomers that have functional groups that is ionized or can be readily ionized (such as a carboxylic acid or the corresponding carboxylate group, or an organic sulfonic acid, and it corresponding organic sulfonate anionic group.
An "Ionotropic gel" is a gel formed by the crosslinking of a polymer with an ion.
"Dried pharmaceutical preparation", a dried pharmaceutical formulation has a moisture content less than 20% in the form of powder, pad, film, sponge, tablet, or capsule.
A "powder" is a solid, dry material that primarily comprises very small solid particles or spheres. The largest dimension'of the bulk of the particles or spheres of a powder are less than a millimeter. In the context of the above definition, "dry" means that there is very little, if any free flowing liquid or excess moisture (including water) on the surface of the powder particles or spheres that would tend to significantly inhibit the normally free-flowing physical characteristics of a powder. The powders of the current invention may in fact comprise absorbed water within their particles or polymer networks, but do not comprise significant amounts of flowable liquid water on their surfaces.
A "microsphere" is a small, approximately spherically shaped solid particle having a generally continuously curved and non-angular surface, the particle having effective diameters between about 0.1 and about 250 microns (,uM). Microspheres, as defined herein include microcapsules. A "microparticle" in contrast to a microsphere, has a flat, angular, rhombohedral, or irregular surface. Microparticles have a longest linear dimension of between about 0.1 and about 250 microns.
A "physiologically active agent" refers to an agent, compound, or composition that can induce a physiological response in the body of an animal. Physiologically active agents include nutrients, small molecule drugs and therapeutic agents, large molecule drugs and therapeutic agents, a pharmacologically active substance; a diagnostic agent; a therapeutic agent; a nucleic acid; a peptide; a polymer; a small protein; a large protein; and a live cell. A pharmacologically active substance includes a substance that illicits immune response, such as a vaccine that comprises one or more antigens. Examples of therapeutic agents include anti-bacterial substances, antimicrobial agents, antiparasitic agents, antibiotics, antihistamines, decongestants, antimetabolites, antiglaucoma agents, anti-cancer agents, antiviral agents, anti-fungal agents, anti-inflammatory agents, anti-diabetic agents, anesthetic agents, anti-depressant agents, analgesics, anti-coagulants, opthaltnic agents, angiogenic factors, immunosuppressants, and anti-allergic agents.
A "vaccine" comprises one or more antigens, typically in the form of a protein, a peptide; a carbohydrate, a lipid, or nucleic acid, a live or dead cell or microorganism in whole or part, a virus in whole or in part, etc., that is capable of inducing immune response in a treated mammal, often inducing the formation of anti-bodies (humoral responses) and/or cellular (T-cell) immune responses selective against the antigen or the microorganism or tissue from which it is derived, so as to treat or prevent diseases caused by microorganisms, viruses, and/or or cancer.
The term "pectic substance," as used in this invention, includes any material comprising a major proportion of one or more polysaccharide materials derived from a naturally occurring pectin. Pectic substances include low and high methoxyl pectins, de-esterified pectin, pectin calcium gel, Aloe pectin sodium gel, pectic acid, pectate, pectinic acid, pectinate, protopectin, and pectin-rich substances, such as Aloe vera inner gel cell wall fiber, individually, collectively, or in combination thereof. As discussed above, pectin is a group designation for those complex colloidal carbohydrate derivatives which occur in, or are prepared from, plants and contain a large proportion of anhydrogalacturonic acid monomeric units.
A "de-esterified" pectin is a pectin from which a plurality of methyl ester groups have been removed from the pectin polymer by an artificial process.
A "Pectic acid" is the group designation applied to pectic substances mostly composed of colloidal polygalacturonic acids and essentially free from methyl ester groups.
A totally de-esterified pectin is a pectic acid or polygalacturonic acid.
"Pectates" are either normal or acid salts of pectic acids. "Pectinic acids" are the colloidal polygalacturonic acids containing more than a negligible proportion of methyl ester groups.
"Pectinates" are either normal or acid salts of pectinic acids. "Protopectin" is applied to the water-insoluble parent pectin which occurs in plants and which upon restricted hydrolysis yields pectins, pectinic acids, and others. The water-insoluble pectin may be associated with the cellulose present in the plant, such as the Aloe vera inner gel or rind cell wall fiber.
A residue of a chemical species, as used in the specification and concluding claims, refers to a structural fragment, or a moiety that is the resulting product of the chemical species in a particular reaction scheme or subsequent formulation or chemical product, regardless of whether the structural fragment or moiety is actually obtained from the chemical species. Thus, an Gal A residue in a pectin refers to one or more of the galuronic acid monomeric repeat units in the pectin, regardless of whether galuronic acid itself is present in or was used to prepare the pectin.

In the subsequent description, reference is frequently made to units of "%
(w/v)".
By this expression the "% (w/v)" is defined to be the number of grams of substance in 100 ml of a liquid solution. In dilute aqueous solutions, the density of the liquid will be approximately 1 gram per milliliter, so that the "% (w/v)" would be approximately equal the number of grams of solid in 100 grams of liquid. In these "% (w/v)"units, a solution that was 1 % (w/v) would correspond to 1 gram per 100 mililiters, =1 gr/ 100 ml =10 mg/ml.
Abbreviations Used Herein Include:
CMC, carboxylinethyl cellulose; Da, dalton; DM, degree of methylation; Gal A, galacturonic acid; HEC, hydroxyethyl cellulose; HMS high methoxyl; HPMC, hydroxypropylinethylcellulose; kDa, kilodaltons; LM, low methoxyl; PBS, phosphate buffered saline; PEG-PLGA-PEG, polyethylene glycol-poly(lactic-co-glycolic acid)-polyethylene glycol; PEO-PLLA, polyethylene oxide) -poly(L-lactide); PEO-PPO-PEO, polyethylene oxide)-polypropylene oxide)-polyethylene oxide).
Pharmaceutical Compositions for In-Situ Gellation The pharmaceutical compositions of the present inventions are "in-situ"
gelling compositions, in either solid or liquid form, that comprise one or more anionic polysaccharides and one or more physiologically active agents, wherein upon or shortly after application to the tissues, body fluids, or mucosal surfaces of an animal, the anionic polysaccharides in the compositions typically form an in-situ gel by the formation of a porous three dimensional polymer network. Prior to their application to the tissues, body fluids, or mucosal surfaces of the animals, the pharmaceutical compositions of the present invention and most or all of their components are typically soluble in pure water prior to their application to the tissues and body fluids, but have the remarkable property that upon application to the tissues of body fluids carboxylate or sulfate groups of the anionic polysaccharides become sufficiently cross-linked by coordination to "endogenous" divalent calcium absorbed from the biological fluids so as to form a bioadhesive gel that is effectively insoluble in either water or bodily fluids at physiological conditions. The compositions of the present invention are accordingly distinguishable from prior art compositions that comprise previously cross-linked polymer compositions that do not become further cross-lined upon application.
In the context of the gel of the current inventions, the liquid in the pores of the polymer network often comprises water, saline, or biological fluids derived from the treated animal or patient that comprise water, and the drugs or pharmacologically active substances are also typically entrapped within the pores of cross-linked polymer network.
In the context of the current inventions, the gel networks are often formed by coordinateJionic bonding between anionic carboxylate or sulfate groups on adjacent polysaccharide molecules and cross-linking divalent or multivalent cations coordinating the carboxylate or sulfate groups.
Solid Comuositions In some embodiments, the invention relates to a solid pharmaceutical composition for the delivery of a physiologically active agent to an animal comprising:
a. one or more physiologically active agents.in an amount effective to induce a physiological response in an animal;
b. one or more polysaccharides comprising subunits having anionic carboxylate or sulfate groups, and c. one or mare solid, polysaccharide gel inducing compositions comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal cation;

wherein the pharmaceutical composition is in a solid form that forms a gel when contacted with a tissue or body fluid of an animal.
In another embodiment related to those described above, the invention relates to a composition for the administration of a physiologically active agent to an animal comprising:
a. one or more physiologically active agents in an amount effective to induce a physiological response in an animal; and b. one or more pectic substances having a degree of methylation less than about 30% and an average molecular weight of greater than about 1 x 105 Daltons, wherein the composition is a solid capable of forming a gel when contacted with a tissue or body fluid of an animal.
The above-described solid pharmaceutical compositions are a solid in any solid form, including a pad, a tablet, a capsule or a powder. In many embodiments the solid pharmaceutical composition is formulated in the form of a powder.
In yet another related embodiment, the invention relates to a vaccine composition for nasal administration to an animal comprising powder particles that comprise a nano-dispersion of:
a. one or more antigens in an amount effective to induce an immune response response in an animal, and b. one or more pectins or a monovalent cation salt thereof having a degree of methylation less than about 30% and an average molecular weight of greater than about 1 x 105 Daltons;
wherein the powder particles can pass through a sieve having an opening size of about 250 ~M in diameter.

The powders can be present as a plurality of microparticles andlor microspheres, as the terms are defined elsewhere herein. In practice, powders having desired ranges of particle size can be produced by any of many methods well known the art, including emulsion processes, encapsulation processes, spray drying processes, grinding or milling of solids, etc. In a final step of many processes, precursor solids or powders are passed through one or more sets of sieves. Such sieves have openings of defined and desirable sizes, for example, 250, 200, 150, 100, 80, 60, 50, 40, 30, 20, 11, 10, 9, 5, l, and 0.1 ~,M., so as to produce a variety of ranges of particle sizes for the powders, microparticles and/or microspheres. Desirable ranges of particle sizes can include the approximate ranges of particle sizes disclosed in Table 1 below. In one embodiments the opening of the sieves permit the powders, microparticles or microspheres to pass through so as to have size of about 250 ~M, or less. Optionally that powder can then be processed with another smaller sieve to remove the smallest particles, so as to produce a solid composition having particle sizes between, for example, about 11 ~M and about 250 ~,M.
There can also be beneficial effects to certain other constraints on particle size distributions. Accordingly, in some embodiments a specified percentage of the particles of a solid composition will fall inside the specified size range. For example, it could be desirable that about 80%, or about 85%, or about 90%, or about 95% of the particles fall within a specified particle size range. To cite one example, in some embodiments, the solid compositions of the invention comprise microspheres, and less than 90% of the microspheres have a diameter between 0.1 and 10 ~,M.
In some embodiments of the invention, the physiologically active agents are deposited on the surface of the particles that comprise the ionic polysaccharide and/or other solid ingredients, or a powder comprising the physiologically active agent is mixed with a powder comprising the ionic polysaccharides. Nevertheless, in many preferred embodiments of the invention, the physiologically active agents are preferably highly dispersed within a solid matrix that comprises a mixture of the anionic polysaccharides, thickerers, excipients, etc. Preferably in the solid matrix mixture the various components of the mixture are primarily dispersed in the form of a mixture of individual molecules and/or ions on the molecular level, though some larger ordered aggregates of like molecules (especially inorganic salts) may present. Such a semi-homogeneous solid matrix mixture rnay be termed a "nanodispersion" of the ingredients of the solid mixture. Even more preferably, the ingredients of the solid mixture and their constituent molecules are substantially homogeneously dispersed on the molecular level, to for a "solid solution" of the components of the solid mixture. Such "nanodispersions" and "solid solutions" provide superior stabilization of sensitive biological active agents, and typcically provide for improved dispersion, control of release reates, and/or bioavailabilty of the physiologically active agents.
Table 1. Selected Compositional Ranges for Components of the Gel-Forming Compositions of the Invention Dried formulations (% w/w) Liquid formulation Polysaccharides 0.0001 to 99 % 0.001 to 20 (% w/v) 0.001 to 50 % 0.01 to 10 0.005 to 20 % 0.05 to 8 0.01to10% O.lto4 Pharmaceutically Active Agent 0.0001 to 90 % 0.001 to 50 (% w/v) 0.001 to about 70% 0.01 to 25 0.01 to 50% 0.05 to 10 0.1 to 20% 0.1 to 8 Powder, Microsphere, or Microparticle Particle Size 0.1 wm to 300 ~m n/a 1 ~,m to 200 ~m n/a 10 ~m to 100 ~m n/a 12 ~,m to 60 wm n/a 15 ~,m to 50 ~m n/a Pharmaceutically Acceptable Thickeners 0.01 to 90% 0.01 to 10(% w/v) O.1to80% 0.1to8 1.0 to 70% 0.2 to 6 S.Oto50% 0.5to5 Dried formulations (% w/w) Liquid formulation Pharmaceutically Acceptable Excipients 0.1 to 90% 0.1 to 40(% w/v) l.0to50% 0.5to30 2.Oto30% l.Oto20 3.0 to 20% 2.0 to 10 Divalent or Multivalent Metal Canons 0.01 to 80% 0.00001 to 0.05(% w/v) 0.05 to 40% 0.0001 to 0.02 O.1to10% O.OOlto0.01 *Although shown pairwise in the table above, it is expressly contemplated herein that any of the endpoints recited for a particular category of components cited in the table may be combined with any of the other corresponding endpoints recited for that category of component, to form a new range for that category of components.
The one or more polysaccharides employed in the invention can be either neutral or anionic, because they comprise monosaccharide subunits having anionic carboxylate or sulfate groups. It is to be understood that the anionic earboxylate groups can be in the form of either a salt of carboxylic acid attached to the monomeric subunits, or the parent carboxylic acid itself, which is readily ionizable or ionized at physiological pH. Similarly, the anionic sulfate groups of the monosaccharide subunits include both a salt of a monosaccharide comprising a sulfonic acid group and a monomeric subunit comprising the acid form of the sulfate. A variety of polysaccharides comprise anionic carboxylate or sulfate groups, including carboxylated starches, pectic substances, an alginate, a carrageenan, or a gellan.
In many embodiments, the solid pharmaceutical compositions comprise one or more pectins, either in its acid form or in the form of a salt of the carboxylic acid. In many preferred embodiments, the anionic polysaccharides and/or pectins are present in the form of a salt of a monovalent cation, such cations including lithium, sodium, potassium, and/or ammonium (NH4+) cations, which tend to be readily water soluble at physiological pH.
Pectins have an a (1~4)-linked polygalacturonic acid (Gal A) polysaccharide polymer backbone intervened by rhamnose residues. The Gal A residues have carboxylic acid substituent groups attached to the sacchaxide ring, which may be in the form of the carboxylic acid, a salt thereof, or an ester thereof. The Gal A content of most pectins is about 70-75%, and the rhamnose content is typically <2%. The rhamnose residues are a (1-~2)-linked to Gal A residues in the backbone, and induce a T-shaped kink in the backbone chain, leading to more flexibility in the polysaccharide chains.
Neutral sugar side chains are attached to the rhamnose residues in the backbone, at the O-3 or O-4 position, and the rhamnose residues tend to be clustered together on the backbone. These rhamnose contain regions comprising the side chains is referred to as a "hairy region" of the pectin, while the long stretches of repeating and unbranched Gal A
residues are termed the "smooth region" of the pectin.
The,hydroxyl and/or carboxylic acid substituents on the saccharide rings are also often bonded to non- sugar components such as methyl and acetyl groups. The extent of rhamnose insertions and other modifications to the chain and its monomers vary depending on the plant source of the pectin. Methylation occurs at carboxyl groups of the Gal A
residues, so as to form carboxylic acid methyl esters. The degree of methylation or methyl-esterification ("DM") if a pectin is defined as the percentage of caxboxyl groups (Gal A
residues) esterified with methanol. Based on the DM, pectins are divided into two classes, low methoxyl ("LM") pectin with a DM of <50% and a high methoxyl ("HM") pectin with a DM of >50%. Most natural pectins and most commercial pectins, which are typically derived from citrus and apples, are HM pectins.
LM pectins are typically obtained from HM pectins through an artificial chemical or biochemical de-esterification process. Commercial LM pectins typically have a DM of 20-50 %. A completely de-esterified pectin is referred as "pectic acid" or "polygalacturonic acid". Pectic acid in the acid form is insoluble but is soluble in the salt form. The common salt form of pectic acid is either sodium or potassium.

Pectins are typically most stable at acidic pH levels between approximately 3 -4.
Below pH 3, removal of methoxyl and acetyl groups and neutral sugar side chains typically occurs. Under neutral and alkaline conditions, the methyl ester groups of the Gal A
residues axe known to be saponified to the carboxylic acid or carboxylate form, but the polygalacturonan backbone also breaks through (3-elimination-cleavage of glycosidic bonds on the non-reducing ends of methylated Gal A residues, with the result that the molecular weight of LM pectins is typically significantly less than the molecular weight its parent HM pectin. Once formed, pectic acids and LM pectins are relatively more resistant to loss of molecular weight at neutral and alkaline conditions since, there are only limited numbers of methyl ester groups, or none at all, so that a-elimination-cleavage of the polymer chains slows down.
Both HM and LM pectins form gels. However, these gels form via totally different mechanisms (Voragen et al, In Food polysaccharides and their applications. pp 287-339.
Marcel Dekker, Inc. New York, 1995). HM pectin forms a gel in the presence of high concentrations of certain co-solutes (for example sucrose) at low pH. HM
pectins are typically not reactive with calcium or other multivalent ions and therefore do not form a calcium gel as do the LM pectins (infra). However, certain HM pectins can be made calcium-reactive by a block wise de-esterification process, while still having a DM of >5O%. See, Christensen et al. U.S. Patent No. 6,083,540.
LM pectins, which have high percentages of un-esterified carboxylic acid and/or carboxylate groups, are known to form gels in the presence of sufficient concentrations of calcium cations. The calcium ions are believed to coordinate to anionic carboxylate groups of the Gal A polymer subunits, and thus, are known as "calcium-reactive." The calcium-LM pectin gel network is believed to be built up by formation of what is commonly referred to as "egg-box" junction zones in which Cap causes the coordination and cross-linking of complementary carboxylate groups along two complementary stretches of polygalacturonic acid polymer chains. Calcium-LM pectin gel formation is influenced by several factors, including the DM, ionic strength, pH, and molecular weight of the pectin (Gamier et al., Carbohydrate Research 240, 219-232, 1993; 256, 71-81, 1994).
Current commercial LM pectins typically have a molecular weight of 7-14 x 104 Da and a Gal A
content of ~75% (Voragen et al, In Food polysaccharides and their applications. pp 287-339. Marcel Dekker, Inc. New York, 1995). Typical pectins have a rhamnose content of <2%.
Pectins are typically utilized in the food industry and classified by the FDA
as "GRAS" (Generally Regarded As Safe). They have also long been used as colloidal and anti-diarrhea agents. Recently, pectins have been utilized in the areas of medical device and drug delivery (Thakur et al., Critical Reviews in Food Seience e~
Nutrition 37, 47-73, 1997). In the case of drug delivery, pectin has found its presence in many experimental formulations for oral drug delivery to the colon because pectin is readily degraded by bacteria present in this region of the intestines. The pectin is either used directly with no gelation involved, or a pectin calcium gel is pre-formed to encapsulate the drug agent before administration. Ashford et al., J. Controlled Release 26, 213-220, 1993; 30, 225-232; 1994; Munjeri et al., J. Controlled Release 46, 273-278, 1997;
Wakerly et al., J.
Pharmacy & Pharmacology 49, 622-625, 1997; International.Iournal of Pharmaceutics 153, 219-224, 1997; Miyazaki et al., International.Iournal ofPhartnaeeutics 204, 127-132, 2000.
In some embodiments the pectins have a degree of methylation (DM) of equal to or less than about 70%, 50%, 30%, 25%, 20%, 19%, 18%, 15%, 14%, 12, 10%, 9%, or 5%
Lower degrees of methylation typically, but not always lead to improved gellation properties, though many other factors are involved in determining the gellation properties of the pectins.
The molecular weight of a pectic substance or a pecin is an important factor in its gellation properties, higher molecular weights typically producing better gellation properties. The importance of molecular weight in the gellation of pectins is described in U.S. Patent No. 5.929,051, which is hereby incorporated herein by this reference, it its entirety, for its teaching of the characteristics of pectins and aloe pectins.
In many embodiments, the pectic substances or the pectins have an average molecular weight of greater than about 4.6 x 105 Daltons, or about 5.0 x 105 Daltons.
Alternatively, the pectic substances or pectins may have an average molecular weight of equal to or less than about 2 x 105 Daltons, 3 x 105 Daltons, 4 x 105 Daltons, 6 x 105 Daltons, 7 x 105 Daltons, ~ x 105 Daltons, or 9 x 105 Daltons. In some embodiments, the pectic ubstances or pectins have a molecular weight greater than 1 x 106 Daltons and a degree of methylation of less than 10%.
With some preferred pectins of the invention, such as the Aloe pectins available from DelSite Biotechnologies Tnc, and/or their water soluble monovalent cation salts, a firm resilient gel can with 0.5% (w/v) LM pectin and 30-60 mg/g Ca2+.
The solid compositions of the invention can comprise small amount of water, especially those comprising pectins, which tend to have residual water absorbed with the pectins. Therefore, the solid compositions of the invention may comprise about 20% water by weight, or about 15%, 12%, 10%, 9%, 8%, 7%, 6%, 5%, 3%, 2% 1%, or less. At any of the percentages of water described above the particles can typically be described as "dry,"
in the sense that no excess free flowing liquid or moisture is apparent on the surface of the particle so as to cause significant stickiness that would significantly impede the free flow of the solid in the form of a powder. Lower percentages of water by weight are preferred in some embodiments of the invention, so as to impxove the stability of the physiologically active agents during storage, or to improve the physical characteristics of the solid.
Active Agents The compositions of the invention (liquid or solid) can comprise one or more physiologically active agents, as that term is defined elsewhere herein. In some embodiments, the physiologically active agents can include a therapeutic agent, a diagnostic agent, a carbohydrate, a lipid, a peptide, a nucleic acid, a live cell, a dead cell in whole or part, a microorganism in whole or part, a virus in whole or part, a vaccine, an antigen, and a'protein. The compositions of the invention can comprise therapeutic agents such as small molecule drugs. In many embodiments the compositions of the invention can comprise a wide variety of larger biological agents including molecules, cells, viruses, antigens, etc.
In some preferred embodiments, the physiologically active agents are antigens for the preparation of vaccines, including peptides, proteins, live cells, dead cells in whole or in part, or viruses in whole or in paxt, inactivated microbes or viruses, live attenuated microbes or viruses, phages, subunit vaccine proteins, subunit vaccine peptides, subunit vaccine carbohydrates, replicons, viral vectors, plasmids, and other immunoactive genetic and recombinant materials, or mixtures thereof. In some embodiments, the one or more antigens axe independently selected from antigens for the prevention of influenza, diphtheria, tetanus, and pertusis, SARS, AmS, cholera, shigellosis, meningitis, plaque, hepatitis, dengue fever, yellow fever, encephalitis, malaria, herpes, measles, typhoid fever, tuberculosis, typhus, otitis media, anthrax or mixtures thereof.
In some embodiments, the one or more antigens are antigens for influenza, or mixtures thereof, such as for example one or more inactivated or attenuated influenza viruses (whole virion), or a subunit thereof (split virion, subvirion) , such as one or more viral membrane glycoprotein, such as a hemagglutinin (HA) or a neuraminidase (NA), or a viral internal protein such as a nucleocapsid protein, or mixtures thereof.
Currently, the split subvirion and subunit antigens are most widely used in the preparation of vaccines for influenza,. Typically influenza viruses exemplary of two or three viral strains that circulated in the intended population the previous year are grown in embryonic chicken eggs and harvested from allantoic fluids, or grown in certain animal cell lines such as MDCK (Madin-Darby canine kidney) cells, inactivated with chemical agents such as formaldehyde, and purified to yield purified whole viruses. Whole inactivated or attenuated viruses can be used to prepare a whole virion vaccine, or the purified viruses can be disrupted by chemicals to separate them into subcomponents such as the membrane proteins HA and NA, and their various known subtypes, then the protein antigens can be further purified. Antigens from one or more of the strains are then combined to produce the finall vaccine.
The influenza vaccine dose for many subvirion influenza vaccines is often formulated based on the HA content. Preferably, the one or more antigens for influenza are present in the compositions and/or administered to the patients in a quantity capable of inducing in the mammals or humans a hemagglutination inhibition (HAI] titer of >40. A
powder influenza vaccine composition for nasal administration might typically be formulated to contain about 5 to 50 micrograms of HA derived from each of three currently circulating viral strains per powder dose, for unit administration.
Vaccine antigens and other pharmacologically active agents based on proteins and other biological materials are often present in the compositions of the invention or administered via the methods of the invention at significantly lower concentrations than other man-made drugs or therapeutic agents, for example at the level of micrograms. The amount of vaccine antigen required in order to induce a medically acceptable level of immunity in the animal will of course vary with the species and weight of the animal, and the immune system characteristics of the particular type of mammal and/or individual.
Nevertheless, for exemplary purposes only, the one or more antigens may be present in the compositions in an amount from about 0.001 % to about 10% of the composition by weight, or from about 0.01% to about 1% by weight, or from about 0.05% to about 0.5%
by weight.
The biological agents employed in the invention tend to be significantly less stable, both in storage and during and after application, than other materials. The compositions of the present invention can be unexpectedly superior in terms of the stabilization and storage of such biological agents. In particular, when mixed with an appropriate gelling polysaccharide, especially pectins, and dried to form a solid, the polar character of the polysaccharide and other carriers and/or excipients in the solid compositions, and the iow water content of the solid composition can significantly prolong the shelf life a biological molecule that might otherwise be unstable in an aqueous solution stored at room temperature, or even under cold storage conditions. Moreover, once incorporated into an in-situ gel after application to tissues or body fluids, the large biological agents tend to be stabilized by the polysaccharide matrix, and tend to be released from the gel more slowly than smaller compounds, so as to achieve a high degree of bioavailability, but with a desirable slow release rate. These desirable characteristics of the compositions of the invention can be particularly important in the administration of vaccines and the associated antigens.
In another aspect, the invention relates to a method for delivering a physiologically active agent to an animal comprising administering to a tissue or body fluid of an animal, in any order or combination, the following components, a) one or more physiologically active agents in an amount effective to induce a physiological response in an animal;
b) one or more polysaccharides comprising subunits having anionic carboxylate or sulfate groups, and c) one or more solid gel inducing compositions comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal ration;
to form a gel in contact with the tissue or body fluids of the animal.
In this embodiment, and in other embodiments of the solid compositions of the .
invention, a solid gel inducing compositions comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal ration may be present as a chemically distinct solid phase, optionally in the presence of or in a mixture with the physiologically active agents andlor other solid excipients. The purpose of such solid gel inducing compositions is to provide an "exogenous" auxiliary solid source of gel-inducing divalent or multivalent rations to supplement those available in-situ from the tissues or body fluids at the site of application, so as to induce and/or improve the speed and/or efficiency of gel formation.
The divalent or multivalent ration of the solid gel-inducing composition is typically present in the form of.a pharmaceutically acceptable salt of the divalent or mufti-valent ration, which provides on contact with the body fluids an auxilliary source of the divalent or multivalent rations necessary for gellation of the anionic polymers, in order to rapidly and efficiently cross-link the anionic groups of adjacent polysaccharide chains so that the tendency to gel as desired is improved, or so that the concentration of anionic polysaccharide necessary to form a gel is decreased. Pharmaceutically acceptable calcium and aluminum salts are preferred salts for use as part of a solid gel inducing composition.

In some embodiments, the pharmaceutically acceptable salt of the divalent or multi-valent cation is readily soluble in water, saline, or body fluids such as serum or mucosal secretions. Upon contact with the body fluids, the soluble pharmaceutically acceptable salt of the divalent or multivalent cations dissolve quickly and liberate the cations into the aqueous medium, and rapidly diffuse into solution contact with the anionic polysaccharides such as the pectins, and coordinate to the anionic groups so as to cross-link the anionic polysaccharides. Examples of such readily soluble salts of divalent or multivalent cations include the calcium halides, especially calcium chloride.
In other embodiments, the pharmaceutically acceptable salt of the divalent or multi-valent cation is only poorly soluble in the aqueous environment of the biological fluids, or "practically insoluble" in the terminology of the Merck Index, in the body fluids.
Preferably such poorly soluble pharmaceutically acceptable salts of the divalent or multi-valent cation will not dissolve in water at ambient temperature and physiological pH to form a solution comprising any more than 5 x 10-3 moles per liter of the salt, or more preferably no more than 1 x 10-5 moles per liter of the poorly soluble salt.
Examples of poorly soluble pharmaceutically acceptable salts of the divalent or mufti-valent cation include calcium phosphate and aluminum hydroxide.
In the compositions of the invention that comprise such poorly soluble pharmaceutically acceptable salts of the divalent or multivalent cations, the anionic polysaccharides tend to diffuse to the surface of the solid particles of the poorly soluble salt, and react with the divalent or multivalent canons at the surface of the particle, so that a gel tends to form at the surface of the particles of the solid gel inducing composition. Thus the inclusion of a solid gel inducing composition tends to lead to the formation of gelled aggregates of the anionic polysaccharides comprising the physiologically active agent on the surfaces of the tissues or mucosal surfaces with a multitude of the particles of the solid gel inducing composition dispersed therein. Such gelled aggregates can provide superior bioadhesiveness as compared to compositions that do not comprise the solid gel inducing compositions, and can be more resistant to dissolution of the gel because of the presence of higher than normal concentrations of divalent or multivalent cations, which tend sto produce unexpectedly slow and superior delivery of the physiologically active agents that are encapsulated within those gels.
In the above-described methods, components a, b, and c can be administered in any order, combination, or physical form so long as component c is administered as a solid, and a gel is formed in contact with the tissues or body fluids of the liquid. In some embodiments of the method, components a, b, and c are administered as components of a powder composition, wherein the components can be in the form of a physical mixture of one or more solid phases. In some embodiments, solid component c is present as a distinct solid phase comprising powder particles, while in other embodiments solid component c may also be present in a mixture on the molecular level with the physiologically active agent.
In some embodiments, components a and b axe administered as separate or mixed powders, while component c is present a different and chemically distinct solid phase. For example, components a and b can be administered as a physical mixture of one or more powders comprising component a, and one or more powders comprising component b, which may be administered separately from or together with component c.
In some favorable embodiments, components a and b are administered as a solid composition prepared by dissolving one or more physiologically active agents and one or more polysaccharides in a liquid carrier, and then removing sufficient liquid carrier to form a solid mixed composition, wherein the agent and the polysaccharide are intimately intermixed on the molecular level. Component c can be administered before, concurrently with, or after the administration of the solid mixed composition, which is often administered in the form of a powder.
As described above, some embodiments of the invention relate to compositions and methods for administering vaccines andlor antigens to animals andlor humans.
Therefore, in some embodiments, the invention relates to method for administering a vaccine to the nasal mucosa of an animal, comprising administering to the mucosal surfaces of the animal:
a) one or more powders comprising microspheres or microparticles that separately or together comprise i) one or more polysaccharides comprising subunits having anionic carboxylate or sulfate groups, in an amount effective to form a gel when the composition is contacted with the mucosal surfaces of an animal;
ii) one or more antigens selected from the group consisting of a peptide, a protein, a nucleic acid, a live cell, a dead cell or a portion thereof, or a virus, in an amount that is capable of inducing an active immune response in the animal; and b) administering the powder to the nasal tissues and/or nasal fluids of the animal to form a gel in contact with the tissues or body fluids, and c) inducing an active immune response to one or more of the antigens in the animal.
Liquid Compositions In some other embodiments, components a and b are administered as a solution in a liquid Garner, while component c is administered as a separate solid.

In yet another embodiment, the invention relates to a method for sustained release of a physiologically active agent to an animal, comprising:
a) providing a liquid solution or dispersion comprising i) a liquid carrier, ii) a pectic substance having a degree of methylation of less than 30% and an average molecular weight of greater than 4.6 x 1 OS Daltons, in an amount effective to gel the liquid solution or dispersion when applied to the tissues or body fluids of the animal, and iii) one or more physiologically active agents; and b) applying the liquid solution or dispersion to the tissues or body fluids of the animal to form a gel comprising physiologically active agent in contact with the tissues.
1n some embodiments of the above methods of applying liquid compositions, the pectic substance can be an aloe pectin, whose beneficial characteristics have been described. In related embodiments of the above methods of applying liquid compositions, the physiologically active agent is a biological agent such as a peptide, a protein, an antigen, a vaccine, a live cell, a dead cell in whole or in part, or a virus in whole or in part.
In related embodiments, the tissue or body fluid can be a mucosal suxface, including a nasal mucosal surface.
In the above methods of applying liquid compositions, the compositions can be modified with certain agents so as to improve theix storage characteristics.
As further described in Example 25 and elsewhere herein, salts of monovalent cations such as sodium chloride and/or ammonium chloride, or buffering agents such as phosphate buffers can be added to the liquid composition to provide a solution of physiological pH, and ionic strength. Moreover, such solutions have some unexpectedly superior properties when employed for first storing and then applying the physiologically active agents. If NaCI or NH4C1 are added at appropriate concentrations to liquid solutions comprising the pectins and agents, the solution can reversibly form a gel when refrigerated for storage (at around 4 °C). The gel so formed can stabilize and protect sensitive biological active agents from precipitation and/or decay. When the composition is removed from storage for administration to the animal or human, the gel dissolves leaving a clear and precipitate free solution that is 'suitable for administration by injection, to mucosal surfaces, and the like.
Moreover, small amounts of salts of divalent cations can be added to the liquid solutions without gelling them, as is described in Example 24, with the benefit that when the modified solution is applied to a tissue or body fluid, ira-situ gelation is enhanced.
Additionally, the liquid solutions can comprise the other thickeners and/or excipients described elsewhere herein.
Nasal administration of vaccines is of particular interest, because of the many advantages of such administrations. Nasal administration typically avoids the discomfort and cost associated with injection, and also avoids the typically destructive effect of the acids and enzymes of the digestive tract on sensitive antigens. It is also known that the body maintains distinct systemic and mucosal immune systems, and that the mucosal immune system is very important in resisting the negative effects of many communicable diseases. In many cases, nasal administration of antigens can stimulate immune reactions in both the systemic and mucosal immune systems. Nevertheless, nasal administration of vaccines can be challenging, because the nasal mucosal surfaces are well known to rapidly renew themselves and clear foreign agents over very short time periods.
Therefore many prior art attempts at the nasal administration of vaccines have not achieved therapeutic success, due to rapid clearance of the vaccine components from the nasal mucosa, so that insufficient time and contact is maintained so as to effectively induce a desired level of 3~

immune response in the animal, especially in the case of high molecular weight and highly polar antigens such as proteins.
The current invention provides compositions and methods of administering those compositions that unexpectedly overcome the problems of the prior art, by providing compositions that form in-situ gels comprising the antigens that adhere to the nasal mucosal surfaces, and provide extended residence times for the antigen components of the vaccines. See Example 26, and Figure 10. As shown by Examples 22 and Figure ~, the result is an unexpectedly improved and superior induction of an active immune response in the animal.
In many embodiments, after administration of the vaccine and/or antigens to the nasal mucosa of the animal the immune response of the animal can increase by more than about 10%, as measured by the IgA levels in the lung washings of an animal as compared to the IgA levels obtained in a control experiment that administers a control composition that does not comprise the polysaccharide. Preferably, the immune response of the animal will increase by more than about 25%, 50%, 75%, 100%, 150%, or 200%, as measured by the IgA levels in the lung washings of an animal as compared to the IgA levels obtained in a control experiment that administers a control composition that does not comprise the polysaccharide.
It is realized that one unique advantage of the powder formulation with gel forming ionic polymers is the ability to blend the powder formulation with a dried gel-inducing agent to ensure a consistent gel formation after administration. Thus, a gel inducing agent made as a dried powder may be added to the powder formulation. Since the inducing agent is in a dry state, there will be no gel formation prior to delivery or hydration. After delivery, the gel-inducing agent is dissolved and thereby facilitates gelation of the formulation powder particles through interacting with the gelling ionic polymer.

For polymers like pectins, alginates, and polyphosphazene, the gel-inducing agent could be various 2+, 3+, and other multi-valent metal ions. Examples of these ions include calcium, zinc, magnesium, ferric, and aluminum. They may be prepared as a powder by themselves or in the presence of an excipient. The inducing agent powder particle density and size may be adjusted to allow it to be mixed with the active agent formulation powders in a consistent and homogenous manner.
Excinients and Adiuvants In addition, other groups of pharmaceutically acceptable excipients may be used, including binders, fillers or bulking agents, lubricants, flavoring agents, and taste masking agents. Binders are use to generate a free-glowing powders; fillers are used to increase the powder bulls; lubricants are used to increase the flow of a powder; taste-masking agents are used to reduce the unpleasant taste of a medicine.
One preferred class of pharmaceutically acceptable excipients are pharmaceutically acceptable mono- or di-saccharides, or mixtures thereof, or alkylated, hydroxyalkylated, or acylated derivatives thereof. Such mono- or di-saccharides are typically non-toxic andlor classified as "Generally Accepted As Safe", readily soluble in water or biological fluids, and inexpensive. Examples of such pharmaceutically acceptable mono- or di-saccharides include ribose, arabinose, xylose, fructose, glucose, rhamnose, glucosamine, galactosamine, gluconic acid, glucuronic acid, galactose, mannose, lactose, sucrose, maltose, xylitol, mannitol, and trehalose. A preferred subset of the pharmaceutically acceptable mono- or di-saccharides include fructose, glucose, galactose, mannose, lactose, sucrose, maltose, mannitol, and trehalose. Lactose, especially in the form of a monohydrate, is a preferred excipient.
The pharmaceutically acceptable mono- or di-sacchaxides may be present at any concentration, but in some embodiments are present in relatively high concentrations, i.e, from about 10.0 to about 99.9 % by weight of the compositions, or preferably from about 30 to about 99.5 % by weight, or from about 50 to about 99.5 % by weight, or from about 80 to about 99.5% by weight. When the mono- or di-saccharides are present in solid compositions at relatively high concentrations, the resulting particles powder particles may tend to partially dissolve or disintegrate partially upon contact with body fluids a mucosal surface before the composition gel. The mono- or di-saccharides tend to be quickly dissolved or absorbed, leaving a concentrated and viscous and bioadhesive gel residue of the active agents and/or the pectins or other anionic polysaccharides well dispersed across and adhered to the biological surface, such as a mucosal surface.
' The above-described uses of mono- or di-saccharides as excipients in the compositions of the invention can be particularly beneficial in the context of the formation of microparticle/microsphere powder formulations for nasal administration of vaccine antigens and other biological active agents that are administered in low concentrations.
The presence of the mono- or di-saccharides as excipients, diluents, andlor bulking agents can allow the particles to be prepared as relatively large particles in the 10-250 micron size range, which is known to be a size range that results of deposition of most of the particles on the nasal mucosa when the composition is administered by insufflation and similar techniques, yet in a short period of time the mono- or di-saccharides are dissolved and/or absorbed, leaving a concentrated, viscous and muco-adhesive in-situ gel residue comprising physicologically active agent well dispersed andlor adhered to the nasal mucosal surface.
The pharmaceutically acceptable mono- or di-saccharides are especially preferred excipients in solid formulations, wherein they can form readily water soluble diluents and/or stabilizers for the pharmacologically active agents, especially biopharmaceutical agents such as peptides, proteins, antigens, etc. that are typically somewhat unstable and are typically administered in low concentrations.
The compositions of the invention may also comprise one or more additional pharmaceutically acceptable adjuvants or absorption promoters, or mixtures thereof.
Adjuvants are additives in a formulation that improve or contribute to the effectiveness or activity of the primary pharmacologically active agent. In the context of vaccine compositions, adjuvants improve the immune response generated in the patient to the vaccine antigens. In some embodiments, the vaccine compositions of the invention comprise one or more vaccine adjuvants selected from the group consisting of lipopolysaccharide, E.Coli heat labile enterotoxin (LT), cholera toxin (CT), monophosphoryllipid A (MPL), saponin, cystosine phosphate guanosine (CpG), cytokines or their derivatives, aluminum salts, calcium phosphate, calcium carbonate, or mixtures thereof.
In the context of administration of pharmacologically active agents to mucosal ~ surfaces, and especially nasal mucosal surfaces, the inclusion of one or more absozption promoters can act on the mucosal surfaces, cell membranes, or inter-cell junctions to improve the absorption of the active agents. In the context of mucosal administration of the compositions of the invention, suitable absorption promoters can include surfactants, mucolytic agents, protein or nucleic acid degradative enzyme inhibitors, chelating agents (such as EGTA, EDTA), acyl glycerols, fatty acids and salts, tyloxapol, salicylates, bile salts and analogues and fusidates, or a mixture thereof.
Aloe Pectin Aloe pectins are isolated from Aloe vera plant as recently described in U.S.
Patent No. 5,929,051, the entire content of which is incorporated herein by reference. Aloe pectins are naturally a LM pectin and capable of calcium gelation. In addition, aloe pectins can possesses several unique chemical properties that are particularly related to gelation, including high molecular weight (>1 x 106 Da), a high Gal A content (> 75%, 80%, 85%, and in many cases >90%), and a low DM ( < 10 %). A DM below 10% makes Aloe pectin almost pectic acids, but with a significantly higher molecular weights than other commercially available low DM pectins and pectic acids, as illustrated in Example 27, Table 8. Aloe pectins also have a significantly higher percentage of carboxylate groups in the polymer as compared to other pectins, because of their high GalA content.
Aloe pectins also typically have a desirably high degree of branching in the polysaccharide backbone, and an unusually flexible polymer backbone, as a result of their high rhamnose contents, which can be > 3% or greater than 4%, as compared to about 2% in other pectins.
A pectin with such a low DM, a high molecular weight, and a high Gal A and rhamnose content had not been described previously to U.S. Patent No. 5,929,051. Aloe pectin, which has recently become commercially available in parities suitable for pharmaceutical applications, is an off white powder and completely soluble in water as the finished commercial product, whereas previously commercially available andlor experimental LM
pectins are yellow to tan powders that contain significant amount of insoluble materials, and thus are undesirable for pharmaceutical applications.
Aloe vera leaves consist of two parts, an outer green rind and a clear inner gel which is also referred to as pulp. Aloe pectin is extracted from the inner gel or outer rind cell wall fibers. Use of a chelating agent at a slight alkaline pH is found to be the most efficient extraction method. Aloe pectin is unique as compared to previously described pectins. It has a high rhamnose content of >4% in the purified pectin preparation which is at least 2 times higher than described in other pectins such as citrus, apple, sugar beet, and sunflower. Rhamnose is a key sugar in the pectin backbone whose content affects the flexibility of the molecule. Aloe pectin also possesses a rare sugar, 3-OMe-rhamnose which has not been described in any other pectins. Aloe pectin is naturally LM, having a DM generally <30% and can be as low as <10%. The Gal A content of Aloe pectin is >70% and can be as high as >90%. Aloe pectin is capable of gel formation in the presence of calcium. A monovalent cation, such as sodium, potassium and lithium accelerates the formation of gel.
Aloe pectin can be distinguished from other pectins by one or more of the following characteristics:
1. A high molecular weight (>1 x 106 Da) and a high intrinsic viscosity (> 550 ml/g);
2. A high rhamnose content (>4%);
3. A high galacturonic acid content (>90%);
4. Containing 3-OMe-rhamnose;
5. Being naturally LM with a DM as low as <10%;
6. Capable of calcium gel formation;
7. Capable of monovalent cation-based gel formation at low temperature (4 °C).
We found that by injecting into a body or by topically applying to wound surfaces as a route of administration, a non-gelled liquid pectin can form a gel in-situ at the site of administration. The in-situ gel is firm and non-flowing just like the calcium gel formed in vitro, which is distinct from the hydrogel, a viscous but still flowing solution. The ira-situ gelation of Aloe pectin was found to be particularly efficient such that the minimal Aloe pectin concentration needed for forming a firm solid ira-situ gel is as low as 2.5 mg/ml or 0.25 % (wlv) and can be even lower if a thickener is added.
Additionally, the capacity for monovalent cation gel formation can be advantageously applied to prepare compositions comprising sensitive biological molecules comprising sodium and/or ammonium chloride at physiological pH and ionic strength that will reversibly gel when refrigerated, so as to form a gel that can stabilize sensitive biological agents. The gels so formulated then redissolve when returned to room temperature to form clear, precipitate free liquid pharmaceutical composition, as described in Example 25. The redissolved solution can then be applied to tissues or body fluids by various methods of administration to form an in-situ gel.
The gel compositions can be made isotonic or iso-osmotic and adjusted to the pH of mammalian body fluids, such as lacrimal tears. The pH and osmotic pressure of such bodily fluids are 7.4 and 29 mOsmlkg, respectively. It is advantageous to deliver a pharmacologically active medicament to an area of the mammalian body requiring pharmacological treatment under desired pH and osmotic pressure conditions which, for instance, match those of bodily fluids. Optionally, the pharmaceutical compositions of the invention can be provided in a sterile condition.
Although not wanting to be bound by any theory, it is believed that the pectin in-situ gelation is primarily mediated by the calcium ions in the body fluids.
Blood has a calcium concentration of ~.5-10.3 mEq/dl. The calcium gelation of pectins is enhanced in the presence of NaCl which is also a normal component of the body fluids.
There are 134 mEq/L NaCI in the blood.
The ira-situ gel also forms in the presence of various agents, including small organic compounds, proteins, nucleic acid, live cells, and other polymers following subcutaneous injection, demonstrating the capability of the pectin for delivering a wide range of agents in an encapsulated or entrapped form. When a poorly soluble compound such as silvadene was incorporated, the ifa-situ gel still formed. Once delivered, the pectin in-situ gel clearly exerted a slow release effect. This was demonstrated under in vitro as well as in vivo conditions With a small organic model compound (fast green). In addition, when bFGF is delivered with the pectin ira-situ gel, a significantly increased cell proliferation surrounding the gel was observed.

Aloe pectin is more efficient than current commercial pectins including LM
pectins, and polygalacturonic acid, and amidated LM pectins for in situ gelation. A
well-formed in-situ gel was only obtained with commercial polygalacturonic acid or LM
pectin at a concentration 10 times higher than that for Aloe pectin. Current commercial LM
pectins and polygalacturonic acids have a lower Gal A content (~75%), a much lower molecular weight (7-14 x 104 Da), and a DM of 15-50%. There are other polymers that can form a calcium gel. One example is alginate. However, alginate was not previously believed capable of forming a well defined in-situ gel at concentrations tested.
Alginate is a polysaccharide block copolymer consisting of guluronic acid (G) and manuronic acid (M) (Moe et al., In Food polysaccharides and tlaeir applications. pp 287-339 .
Marcel Dekker, Inc. New York, 1995). These two residues in alginates exist as G-block, M-block, or alternating MG-block. Only the G-block is responsible for calcium gelation.
The total G
content varies widely dependent on the sources; the highest G content is ~70 %. In addition, the alginate calcium gelation is inhibited by the presence of NaCl, which exists in the physiological fluids.
Several other polymers have also been shown to be capable of in-situ gelation.
However, most of them require a high polymer concentration for ira-situ gel formation (>20%) (Poloxamer , PEO-PLLA diblock copoly, PEG-PLGA-PEG triblock copolymer, cellulose and acetophalate latex). Some of these polymers are not biodegradable, such as Poloxamer, or require manipulation of the temperature before administration (PEO-PLLA
diblock copolymer) or during formulation (Pluronics and Gelrite). The thermally gelling polymers (Poloxamer, Pluronics, PEO-PLLA diblock copolymer, PEG-PLGA-PEG
triblock copolymer, and Matrigel) also have the disadvantage of gelling before administration due to ambient temperature changes during packaging or storage.
Furthermore, many of these polymers form only a hydrogel, a viscous but still flowing solution (e.g., Poloxamer and Pluronics). In addition, some polymer formulations require two different polymers or the application of a second component for gelation to occur.
Pectin, especially the Aloe pectin, is advantageous over these polymers or compositions in that the polymer concentration required to achieve the i~c-situ gelation is very low (x0.25 %, wlv) and can be even lower if a thickener is added. The preparation does not require temperature or pH adjustment, or application of a second component for the irz-situ gelation to occur. The gel is transparent, and there is no dramatic increase in gel cloudiness beyond certain concentration ranges as with PEG-PLGA-PEG triblock copolymer and Pluronics.
The advancement of biotechnology is generating more and more protein-based therapeutics. Proteins are inherently unstable. Proper formulation and delivery are critical to their isz vivo functions (Langer, Nature 392, 5-10, 1998; Putney and Burke, Nature Biotechnology 16, 153-157, 1998). The pectin in-situ gel is particularly suited for protein delivery because of its mild gelling conditions. Many protein agents are also intended to be delivered locally in a sustained manner, e.g., growth factors for wound healing and angiogenic factors for therapeutic angiogenesis. This can also be achieved with pectin ifa-situ gel. When bFGF was delivered with the Aloe pectin in-situ 'gel, a significantly increased cell proliferation surrounding the gel was observed.
Based on the weight of the final composition or formulation, the physiologically active agent can vary from about 0.01 % to about over 90 %. The amount of the physiologically active agent used would depend on the type, form, and nature of the physiologically active agent.
The range of the pectic substance can vary from about 0.01 % to about 40 %, based on the total weight of the composition, preferably from about 0.1 % to about 20 %, and more preferably from about 0.25 % to about 2 %. The amount of the pectic substance used would depend on the type, form, and nature of the physiologically active agent. Optionally, a carrier or excipient may be used.
A carrier used for this invention includes any pharmaceutically acceptable carrier, such as water; saline; a buffered aqueous solution; emulsion, such as oil/water emulsion;
adjuvant; a wetting agent; tablet; and capsule. used on the weight of the final composition or formulation, the carrier can vary from about 0 % to about 90 %.
The amount of carrier present would depend on the physiologically active agent and the manner by which the formulation or composition is to be delivered.
Representative buffering agents include alkali or alkali earth carbonate, chloride, sulfate, phosphate, bicarbonate, citrate, borate, acetate, and succinate, and/or ammonium chloride. Representative preservatives include sodium bisulfate, sodium thiosulfate, ascorbate, benzalkonium chloride, chlorobutanol, thimerosal, phenylinercuric borate, paraben, benzylalcohol, and phenylethanol.
Thus, one embodiment of the current invention is to provide a composition for the sustained delivery of a physiologically active compound, and the composition contains a pectin and a physiologically active compound with or without a pharmaceutically acceptable thickener. Preferably, the composition changes from a liquid to a gel upon administration of the composition to the body of an animal, and thus the release of the physiologically active compound is sustained or controlled.
A biodegradable thickener such as polyvinylpyrrolidone ("PVP"), carboxymethylcellulose ("CMC"), hydroxyethylcellulose ("HPMC"), sodium alginate, collagen, gelatin, and hyaluronic acid may be added to the formulation.
Addition of such a thickener does not influence the gelling efficiency as described below, but provides an advantage of enhancing the density of the gel matrix and the ih-situ gel formation at lower pectin concentrations. In addition, polymers that are responsive to changes in pH, ionic strength, and temperature may also be used as long as they are synergistic with the pectin gelation. Furthermore, a blend of different pectins may be used with or without a thickener. Other thickeners include Carbopol, Gelrite, chitosan, and xyloglucan. Based on the weight of the final composition or formulation, the thickener can vary from about 0 to about 90 %. The amount of biodegradable thickener used would depend on the physiologically active agent and the manner of which the composition or formulation is used.
Still another embodiment of the current invention is to provide a composition consisting of a pectin with or without a pharmaceutically acceptable thickener for use as a medical device. ' Preferably, the pectic substance is calcium reactive, in that the carboxylate substituent groups of the galacturonic acid monomeric subunits of the pectin can react to coordinate calcium ions, and thereby form calcium crosslinked gels. The formation of such calcium reactive gels can be determined by various spectroscopic and/or wet chemical methods, including reaction of the crosslinked gels with calcium chelating agents, such as ethylenediamine-tetraacetic acid and its salts ("EDTA"), which can be used to remove the coordinated calcium from the gel and thereby cause dissolution of the gel.
More preferably, the pectic substance is a LM pectin or polygalacturonic acid.
Still more preferably, the pectic substance is Aloe pectin.
A pectin in-situ gelling compositions containing a therapeutic or diagnostic agents) may be administered or delivered to the animal by various means. For example, it may be applied topically to the eyes, mucosal surfaces, or wounds. It may also be delivered parenterally, such as subcutaneously, intramuscularly, or via intraperitoneal injection. It may also be injected into an organ, a joint cavity, or a tumor.

Pectin can be extracted from many different plant sources. Besides citrus and apples, for example, pectin has also been obtained from potatoes, grape fruits, sugar beets, and sunflower heads. Pectin may be modified. For example, an amidated pectin is produced by treatment with ammonia. It is conceivable that an Aloe-pectin-like pectin may be present in a different plant species or a pectin from a different plant source may be produced, re-processed, and/or modified in a way to enhance the in-situ gelling ability based on the principles disclosed herein. Furthermore, although an LM pectin with a DM <
50% is preferred for use in the present invention because of its calcium reactivity, certain HM pectins are also known to be calcium-sensitive and capable of forming calcium gel, and may therefore be used for in-situ gelling (Tibbits et al., Carbohydrate research 310, 101-107, 1998). In addition, a block wise de-esterified HM pectin that still has a DM of >50%, but is rendered calcium sensitive by the block wise de-esterification, may also be used. See, Christensen et al. U. S. No. 6,083,540.
Thus, it should be appreciated by those skilled in the art that the specific embodiments disclosed above may be readily utilized as a basis for modifying or designing other structures for carrying out the same purposes of the present invention.
It should also be realized by those skilled in the art that such equivalent constructions do not depart from the spirit and scope of the invention as set forth in the appended claims and/or examples.

In-situ Gelation of Aloe Pectins Extraction of Aloe pectin Aloe pectin was extracted from cell wall fibers prepared from either pulp or rind of Aloe vera leaves. The general methods of extracting pectins have been reported. See, Voragen et al, Ira Food polysaccharides and their applications. pp 287-339.
Marcel Dekker, Inc. New York, 1995. See also, U.S. Patent No. 5,929,051, the entire content of which is hereby specifically incorporated by reference. The extraction of Aloe pectin was achieved with a chelating agent such as EDTA or under other conditions including hot water, hot diluted acid (HCI, pH 1.5-3), and cold diluted base (NaOH and Na~C03; pH 10).
Following the initial extraction, the remaining fibers were removed by coarse and fine filtrations. The pectin was precipitated with ethanol. The pectin precipitates were further rinsed with ethanol solutions before being dried.
Aloe pectins obtained in this manner from either pulp or rind cell wall fibers were characterized with a molecular weight (>1 x 105 Da), a low DM (< 50%), and a Gal A
content (>80 %). Preferably, the molecular weight was >1 x 106 Da, the DM was <10%, and the Gal A content was >90%.
The molecular weight of the pectins was determined by HPLC-based size exclusion chromatography with pullulan as the standard. DM was determined by a selective reduction method (Maness et al., Analytical Biochefnistny 185, 346-352, 1990) and a HPLC-based method (Voragen et al., Food Hydrocolloids, 1, 65-70, 1986). Gal A
content was determined by m-hydroxyldiphenyl method (Blumenkrantz, N. and Asboe-Hansen, G.
Analytical Biochemistry 54, 484-489, 1973). The content of each of these three references is hereby incorporated by reference.
Iu-situ relation of Aloe Pectin Solutions Administered by Infection In Vivo Aloe pectin was first dissolved in sterile deionized water and then mixed with equal volume of 2 x physiological saline (0.3 M NaCl). Aloe pectin could not be readily dissolved in salt solution. However, once dissolved in water, the pectin can be mixed with the salt solution to achieve the physiological ionic strength. The pectin solution in physiological saline obtained in this manner remained clear. The pectin solutions were free-flowing at room temperature and had a pH of 5.0-6.0 depending on the polymer concentrations. No adjustment of temperature or pH was performed unless otherwise indicated. The preparation was injected subcutaneously into lower abdominal regions of Swiss Webster mice (0.05 or 0.1 ml per site) in accordance with the animal use protocols.
Mice were sacrificed at various times following injection and the gel formation was examined.
The swelling of the skin at the injection site did not disappear over time as in the case of the saline control. When the skin over the injection site was surgically incised, a piece of gel shaped like a ball or an oval was observed. The gel was clear, transparent, and firm. It could be readily separated from surrounding tissues. The gel was surgically excised along with skin, fixed in formalin, sectioned, stained with Ii&E, and examined under the microscope. The gel was only lightly stained but was clearly visible and surrounded by the dermal tissues. The same in-situ gelation was also observed in rats. The swelling at the injection site was not as evident in rats as in mice due to the thicker skin and hair coat. However, when skin at the injection site was surgically incised, the same in-situ gel was observed. With rats, one ml of Aloe pectin solution could be injected subcutaneously at the lower abdominal region and correspondingly much larger gel pieces were obtained.
The gel formation is pectin concentration-dependent. At a concentration of x 0.25% (w/v), a solid firm gel was obtained. No gel formation was observed at a 0.1%
(wlv). At concentrations between 0.1% and 0.25 %, a soft gel was obtained.
The in-situ gel also formed when the pH of the Aloe pectin solution was adjusted to ~7.2 with dilute sodium hydroxide.
The in-situ gelling ability is dependent on the molecular weight of Aloe pectin.
When an Aloe pectin with a much reduced molecular weight (~3 x 10~ Da) but the same DM and Gal A content was used, no in-situ gelation was observed when tested at 0.5%
(w/v).

The ifa-situ gel also formed following injection through intraperitoneal and intramuscular routes although the gel formed did not appear to have as uniform a shape as that formed following subcutaneous injection.

Iu-situ Gelation Following Topical Application To A Wound Surface Aloe pectin preparation (0.5 %, w/v) in physiological saline was directly applied to fresh full-thickness excisional skin wounds on mice or rats. A' 0.5 % (w/v) CMC
preparation. in physiological saline and a commercial hydrogel wound dressing were used as a control. The wounds were made with a biopsy punch in accordance with animal use protocols. After 4 hrs, rats were sacrificed and wounds surgically removed.
Wounds were fixed in formalin, sectioned, and stained with H&E. A layer of gel was clearly visually observable on the surface of wounds with the Aloe pectin preparation but not with CMC or the commercial hydrogel wound dressing.

Pectin hz Situ Gelation Mediated by Calcium Ions in Body Fluids, As Measured by A Gel Frontal Migration Assay Body fluids such as blood, lacrimal fluid, lung fluid and nasal secretions contain calcium ions (S.5-10.3 mEq/dl in blood, for example). Since Aloe pectin forms calcium gel, the role of calcium in the ifz-situ gelation of Aloe pectin was examined using an in vitro gelling assay with animal serum that simulates ira-situ gel formation. This in vitro assay is described as a gel frontal migration assay. Animal serum was placed at the bottom of a glass tube and the Aloe pectin solution was layered on top of the serum (the pectin solution may also be placed at the bottom of the tube dependent on the density of the test solution in relation to the pectin solution). Tissue culture grade normal calf serum was used. Two ml of serum was placed at the bottom of a glass tube (0.8 x 11 cm) and 1 ml pectin solution (0.5-0.75 %, w/v) was placed on top of it.
Gel formation was immediate at the contact line (interface of the solutions) and the gel phase or gel front gradually extended upward in the pectin solution over time. The gel formed in the upper pectin phase can be distinguished from the pectin solution by its increased turbidity when examined under a light source. Also, tilting the tube does not move the interface if a gel is formed. The thickness of the gel formed at the interface can be measured aver time (such measurements are referred to as "gel length"
hereinbelow).
FIowever, if the body fluid such as serum was first dialyzed against saline or EDTA
(a chelator for divalent cations) to remove free calcium from the solution, or EGTA (a specific chelator for calcium) was added to the serum to a final concentration of 10 mM, no gel formation was observed. This is evidence that indicates that the calcium ions present in body fluids is involved in pectin in-situ gelation.
The pectin gelation also occurred when tested in similar in-vivo experiments with heparinized whole mouse blood or plasma isolated therefrom.
E~LAMPLE 4 Pectin Ih-Situ Gelation with Other Body Fluids Besides serum or blood, there are many other types of calcium containing body fluids such as tear fluid, lung fluid, and nasal fluid. To determine if the pectin gelation also occurred in in-vitro experiments with other body fluids, the gel frontal migration assay described in Example 3 was used along with Aloe pectin (0.25% in saline).
The gel formation occurred with natural peritoneal fluid. In this case, the ascites from mice inj ected with hybridoma for monoclonal antibody production was used as peritoneal fluid.
Gel formation also occurred with simulated body fluids such as:

1. Tear fluid (0.68 g NaCl, 0.22 g NaHC03, 0.008 g CaC12.2H20, and 0.14 g ICI
per 100 ml. (See, Stjernschantz and Asitin, in Edman, P. (ed.), "Biopharmaceutics of Ocular Drug Delivery," CRC Press, Boca Raton, pp. 1-15, 1993. Alternatively, 0.268 g bovine serum albumin, 0.268 g lysozyme, 0.134 g globulin, 0.008 g CaC12.2H20, 0.650 g D-glucose, and 0.658 g NaCI per 100 ml. See, Cohen et al., Journal of Controlled Release 44, 201-208, 1997);
2. Lung fluid (0.01 g MgC12.6H20, 0.61 g NaCI, 0.03 g ICI, 0.027 g NaaHPO4.7H2O, 0.007 g Na2S04, 0.018 g CaC12.2H ZO, 0.095 g NaHC202.3H20, 0.26 g NaHCO3, and 0.01 g Na3H5C607.2H20 per 100 ml. See, Fisher and Briant, Radiation Protection Dosimetry, 53, 263-267, 1994); and 3. Nasal secretion (0.867 g NaCl, 0.44 g NaZHP04, 0.108 g NaH2PO4, 0.058 g CaC12.2H2O, 0.31 g KCl 0.636 g albumin per 100 ml. See, Lorin et al., Journal of Laboratory Clinical Medicine, 2, 275-267, 1994).

NaCI Enliances Pectin Calcium Gelation Body fluids such as blood and lacrimal fluids also contain sodium ions (135-mEq/L in blood). NaCI has been shown to enhance the calcium gelation of LM
pectins.
Pharmacological preparations for topical or parenteral use are commonly prepared in a buffered or non-buffered physiological saline (0.15 M NaCI) or isotonic solution. To determine if the enhancement of gelation induced by NaCI solutions also occurs with Aloe pectin, the gel frontal migration assay was used. Aloe pectin (0.5 %, w/v) solutions prepared in 0.15 M NaCI (2 ml) were placed at the bottom of the tube and a less dense 100 rnM CaCl2 solution (0.05 ml) was placed on top of the pectin solution. The gel formed, extending downward in the pectin solution over time. The migration of the gel front downward into the pectin solution was measured at intervals following the addition of CaCl2. The results showed that the gel front migrated faster in the presence of NaCl, i.e., the calcium gelation of Aloe pectin was enhanced by the presence of NaCI (See Figure 1).
The effect of NaCI was also calcium concentration dose-dependent; as the gel migration rate was faster in 0.15 M NaCI than in 0.05 M NaCI.
These observations are consistent with previous findings with other LM pectins (Gamier et al., Carbohydrate Research 240, 219-232, 1993; 256, 71-81, 1994).
Figure 1 is a bar graph representing the relationship of NaCl to the calcium gelation of Aloe pectin.

Pectin Ih Situ Gelation is Faster at Low Pectin Concentrations The gel frontal migration assay described above was used. Aloe pectin at various concentrations in saline (1 ml) was applied onto the normal calf serum (2 ml).
After 18 hrs at room temperature, the length of gels formed (i.e. gel thickness) was measured. The initial gelation at the contact phase is immediate regardless of the pectin concentration.
However, the rate at which the gel length grew over time differed at different pectin concentrations. It was found that the lower the pectin concentration, the faster the gelation;
as the length of the gel formed at 0.05% (w/v) was nearly 5 times longer than that at 0.5%
(w/v) (See Figure 2). The gel formed at low concentrations (<0.2%, w/v) was much softer and could be broken by strong agitation.
The same observation was also made when a calcium chloride solution was used to replace the serum. This indicates that the rate of pectin calcium gelation is higher at lower pectin concentrations.

Addition of Other Polymers or Thickeners Enhances the Pectin In-Situ Gel Formation The gel frontal migration assay described above was used. Polymers such as hydroxyethylcellulose (HEC, 0.45%, w/v) , carboxymethykellulose (CMC, 0.45%, w/v), or sodium alginate (0.45%, w/v) were mixed with Aloe pectin (0.05%, w/v).
Sodium alginate, although capable forming calcium gel with CaCl2 solutions under i~c vitro conditions, did not form an ih-situ gel with the serum. One ml of the polymer solutions were applied onto 2 ml normal calf serum in a gel frontal migration assay. The length of gels formed was measured 18 hrs later. The results showed that addition of other polymers did not influence the rate of the pectin in-situ gelation (See Figures 3A and 3B). The same result was also obtained when the polymer was mixed with Aloe pectin at a different ratio (0.4% vs 0.1 %).
In an in vivo mouse experiment similar to those described in Example 1, a mixture of Aloe pectin (0.375%, w/v) and CMC (0.375%, w/v) in saline formed an in-situ gel following subcutaneous injection to the mouse. In addition, the addition of a thickener .
(sodium alginate or HEC at 0.4% or 0.3%, w/v) resulted in a better formed in-situ gel at lower Aloe pectin concentrations (0.1% or 0.2%, w/v) in which the ita-situ gels were either soft or not formed with Aloe pectin alone (Example 1).

Comparison with Other Pectins and Alginates Several polysaccharides other than Aloe Pectin that are capable of calcium gelation were used in in-vivo gelation experiments. The other polysaccharides included an LM
pectin from citrus with a DM of 28% and a polygalacturonic acid prepared from apple pectin (DM=0), both of which were obtained from Sigma Chemical Co., and an amidated pectin with a DM of 28-34 % and a DA (degree of amidation) of 16-22 %. Before use, they were dissolved in de-ionized water, filtered, ethanol precipitated, and dried.
In-situ gelation experiments injecting mice with the solutions of the other pectins by subcutaneous route was performed as described in Example 1. Four injection sites on two mice were used for each sample. The results showed that following subcutaneous injection, no in-situ gel formation was clearly observed with any of the alternative polysaccharides at a concentration of 1.0 or 1.65 % (w/v), as only smear-like gel substances were observed. However, when tested at a higher concentration (3.0 or 3.3 %, wlv), well formed gels were obtained with both polygalacturonic acid and amidated LM
pectin.
Similarly, the low molecular weight of Aloe pectin described in Example 1 also gelled in situ at a high concentration (2.5 %, w/v).
An HM citrus pectin with a DM of 64 % was also tested. It was prepaxed in the same way as that for the LM pectins. No gel formation was observed for the HM
pectin at a concentration of 3 % (w/v). The injection site was wet and watery and no solid gel pieces were observed.
Alginates were also tested, including Keltone HVCR and the high G alginate Manugel DMB (G content, 60-70%) at a concentration of 0.5 %. Only a smear-like gel substance was observed when examined 4 hrs post subcutaneous injection, indicating that most of the materials had diffused away without gelling. The alginates also did not form a gel with the normal animal serum in the in vitr~ in-situ gelation assay as described above (Example 7). These results together showed that the LM pectin, polygalacturonic acid, amidated LM pectin, and alginate are much less efficient than Aloe pectin for in-situ gelation, under the same concentrations.

Delivery of Physiologically Active Agents by Pectin In-Situ Gel For the in-situ gelation to be used for drug delivery, the phenomena must occur in the presence of the drug or diagnostic agents. Thus, various compounds or agents were mixed with Aloe pectin in physiological saline with a final pectin concentration of 0.5%
(w/v). The experimental agents included a small molecule organic compound (fast green, N Ethyl-N (4-[(4- f ethyl[(3-sulfophenyl)methyl]amino)phenyl)-(4-hydroxy-2-sulfophenyl)methylene]-2,5-cyclohexadien-1-ylidene)-3-sulfobenzenemethanaminium hydroxide inner salt, disodium salt, 808 Da, 10 mg/ml), a small protein (bFGF, 17 kDa,10 p,g/ml), a medium-sized protein (bovine serum albumin, 66 kDa, 10 mg/ml), a large-size protein (type I bovine collagen, 2 mg/ml), a nucleic acid (Lamda DNA Hind III
fragments, 200 ,ug/ml), a carbohydrate polymer (CMC, 0.5%, w/v), and Raw 264.7 cells (a mouse macrophage line, 1 x 108/m1). The mixtures were inj ected subcutaneously into mice. ~ Gel formation was then examined 4 hrs after inj ection. The results showed that the ifa-situ gel ~ formation occurred in the presence of all the agents occurred similarly to the gels formed with the Aloe pectin alone controls.
Furthermore, by gel frontal migration assay, the in-situ gelation of a 0.5%
(w/v) Aloe pectin solution also occurred in the presence of 1) 0.1% (w/v) silvadene (silver sufadiazine), a poorly soluble anti-bacteria agent commonly used for wound treatment, 2) 0.5% (w/v) hydroxyethyl cellulose (HEC), and 3) 0.5% (w/v) sodium alginate (Keltone HVCR, Kelco). The presence of 0.5% (w/v) HEC or sodium alginate did not influence the efficiency of the in-situ gelation as described in Example 6.
Thus, the fact that the ira-situ gelation occurred with these many different agents clearly indicates that the pectin in-situ gel can be used for delivery of a wide range of drug agents.

Slow Release of a Small Organic Compound from Pectin Ih Situ Gels Under 1u Vitro Condition Therapeutic and diagnostic agents vary greatly in molecular weight, from ~ 100 Da to over 10,000 Da. Generally, the smaller the compound, the more difficult to achieve a slow release effect. Here the small organic compound fast green, a dye which is widely used in the food and pharmaceutical industry, was chosen as a test compound.
The dye was mixed with Aloe pectin (0.5%, w/v) in saline at a fast green concentration of 1 mg/ml.
A pectin-free 1 mg/ml dye solution in saline only was used as a control. One ml of the dye/pectin preparation or the control was placed into a dialysis tube (1 cm in diameter) with a 12 kDa cut-off. Dialysis tubes with samples were then placed into 25 ml normal calf serum in 30- ml glass tubes. One serum tube receiving the dye/Aloe pectin solution also received EDTA to a final concentration of 10 mM to prevent calcium gelation.
The serum tubes containing the samples were then shaken continuously at 100 rpm on a rotatory shaker. A small amount of serum (100 ~,1) was sampled at various time points.
The amount of dye released into the serum was determined by measuring the OD at 620 nm.
Serum samples with known amounts of fast green were used to establish the standard curve. The results showed that similar amounts of fast green were released from the control and dye/Aloe pectin with EDTA (without gel formation) and the amount of the dye released from the dye/Aloe pectin without EDTA (with gel formation) was significantly lower (p<0.05; student t-test) at the time points measured (See Figure 4).
This indicates that the presence of Aloe pectin and its gelation significantly slowed the release of the model small molecule pharmaceutical agent.

Slow Release of a Small Organic Compound from Pectin Iu Situ Gels following Subcutaneous Injection To determine if the above observed slow release could be obtained under ih vivo conditions, the fast green (1 mg/ml)/Aloe pectin (0.5%, w/v) in physiological saline or fast green in physiological saline alone was injected subcutaneously into mice. The injection sites (two per sample) were examined 4 hrs later. It was found that with the presence of pectin, ih-situ gels were formed which partially retained the dye although the color was not as strong as the original preparation prior to injection. In contrast, the injection sites of the control had no gel and no color, and thus no retained dye. Therefore, the pectin in-situ gel retained the dye and indeed slowed the release under the irc vivo condition.

Local Delivery of bFGF by Aloe Pectin Iu-Situ Gel For growth factors to exert local effect on tissues surrounding the administration site, they need to be delivered in a matrix to allow them to be released in a slow or sustained manner. A delivery in saline or buffer alone is not effective in this regard. In this example, a growth factor (bFGF) was used. bFGF (basic fibroblast growth factor or FGF-2) is a growth factor known to stimulate fibroblast proliferation and angiogenesis or blood vessel formation. It was mixed with Aloe pectin (0.5%, w/v) in physiological saline at a concentration of 1-10 ,ug/ml and then injected subcutaneously into the lower left or right side of abdominal region of mice. ~ne side received the control (pectin alone), and the other side received the bFGF-containing preparation. The in-situ gels from two mice were harvested along with skin at days 5-10 and subjected to fixation in formalin, sectioning, and H&E staining. Two identical areas, at either end of the gel, vertically between the gel surface and the skin muscle layer and horizontally 510 ~.m inward from the lateral end of the gel were selected, and the cells in these two selected areas from each gel were numerated using the NIH image software. The results showed that the cell number was more than 2 times higher in bFGF-treated than the control (Figure 5). An increase in blood vessel formation surrounding the gel was also observed at a high bFGF
concentration (10 ,ug/ml). This indicates that bFGF was released from the ifz-situ gel and exerted its function in the surrounding tissues.

Ih Situ Gelation of a Dried Pectin Composition A mixture of an Aloe pectin and CMC (0.75% by weight each) and 1.5% CMC
prepared in water were lyophilized in weighing trays, separately. The dried materials were cut out as round pads (about 1 cm in diameter and about 3 mm in thickness) and were immersed in a 10 ml of normal calf serum in a petri dish. The Aloe pectin/CMC
pad formed a clear gel which remained intact for four days until the experiments were terminated, whereas pads containing CMC alone were dissolved or disappeared in a few hours under the same conditions. Thus, these results show that pectin in a dried form can also form a gel after being immersed in a body fluid.

Use of Pectin Iu Situ Gel for Drug Delivery: Formulation Process The pectin in-situ gel can be used to provide a physiologically acceptable composition that contains a therapeutic or diagnostic agent and a low concentration of a gelling polymer (pectin) with a pH and osmotic pressure characteristic of the body fluids, and that has the capability to change from liquid to gel upon administration.
The process to prepare a liquid formulation includes the following steps.
1. Pectin is dissolved in sterile water.
2. A buffered or non-buffered saline is prepared.

3. The two solutions are mixed.
4. A physiologically active compound is added to the preparation at step 3.
The physiologically active agent may alternatively be added to either solution before mixing.
Besides water and buffered or non-buffered saline or aqueous solution, other pharmaceutically acceptable carriers may also be used, including emulsions such as an oil/water emulsion, adjuvant, various types of wetting agents, tablets, and capsules.
The pH of the formulation is adjusted with suitable buffering agents such as boric acid-sodium borate, sodium phosphate (monobasic)-sodium phosphate (dibasic), and Tris-HCl. Osmotic pressure of the formulation is adjusted to mimic that of body fluids with salts such as NaCI, KCL and MgCl2, and other osmotic adjusting agents such as sorbitol, sucrose, glycerin, and mannitol.
A pharmaceutically acceptable thickener may be added. The thickener can be polyvinylpyrrolidone ("PVP"), modified cellulose polymers such as carboxymethylcellulose ("CMC"), hydroxymethylcellulose ("HPMC"), hydroxyethylcellulose ("HEC"), alginate, gelatin, dextran, cyclodextrin, or hyaluronic acid.
The formulation may be stored at room temperature or refrigerated (4 °C). If the formulation contains 0.15 M NaCI, a (sodium) gel is formed when it is stored at 4 °C.
Prior to application, the gel is allowed to revert back to solution at room temperature. For drug or therapeutic agents that are particulate, prone to aggregate formation, or have a low water solubility such as silvadene (silver sulfadiazine), storage in a gel matrix may be advantageous because it may prevent aggregate or precipitate formation.
Alternatively, the formulation may be prepared in a dried form. A mixture of a pectin and a physiologically active agent in buffered or non-buffered water or saline are lyophilized. Alternatively, a pectin powder and a dry physiologically active agent are blended and compressed into a desired form. The dried form may be used as a pad, a tablet, a capsule, or a powder.
The relative amounts of the physiologically active agent and the pectic substance in the formulation or composition can vary widely dependent on the particular agent to be delivered. In a liquid formulation, the agent can range from about 0.01 % to about 50 (w/v) while the pectic substance can range from about 0.01 % to about 40 %
(w/v). In a dried or suspended formulation, either the agent or the pectic substance can range up to over 90 % (w/w).

Preparation of Pharmaceutical Powder Formulations Comprising Assorted Anionic Polysaccharides, and Their Gel-Forming Properties Powder formulations comprising model active agents, various anionic polysaccharides, thickeners, and an optional excipients, as detailed below in Table 2 were prepared. The ionic polymers used to prepare the formulation are listed below.
High Molecular Weight Aloe pectin, (HMW AP), DM < 10%, Mw > 1.0 x 106 Da Low Molecular Weight Aloe pectin (LMW AP) DM < 10%, Mw= 1.3 x 105 Da Polygalacturonic acid, (Poly Gal A) from Sigma, DM < 3%, Mw =1.7 x 105 Da Low Molecular Weight Pectin (LM Pectin) DM = 26%, Sigma, Mw= 2.0 x 105 Da Alginate, medium viscosity, Sigma Chemical Co.
Molecular weights were determined by Size Exclusion Chromatography using pullulan as a standard via the procedure described in example 10 of US Patent No 5929051.
SEC was performed using TSI~-Gel 65000 PWX column (Toso Haas). Samples were prepared at 0.3 mg/ml in water with 0.05% (w/v) sodium azide. 50 ,u1 of the sample was injected and eluted with 0.05% sodium azide at 1 ml/min. Refractive index was measured in line. Pullulans (4.04 x 105, 7.88 x 105, and 1.66x106 Da) were used as standards. The molecular weight was calculated against the linear regression line of the standards.
The now commercially available Aloe pectins are highly purified and micro-filtered and are made under cGMP (current Good Manufacturing Practice). The other polysaccharides listed in the table above all contained a considerable amount of insoluble material and produced cloudy solutions when dissolved in water. They were all micro-filtered to remove insoluble materials, precipitated with alcohol, and dried before use.
Bovine serum albumin (BSA) and lysozyme were initially used as pharmaceutically active agent. BSA is widely used for examining various pharmaceutical formulations as a model agent, especially those for protein delivery. Lysozyme is known to be antibacterial.
Povidone (polyvinylpyrrolidone, K29-32) was used as a thickener and lactose was used as a excipients, and both were obtained from Sigma Chemical Co.
Powders formulations were made by preparing a liquid mixture of all the ingredients listed in Table 2 and then lyophylizing the solution, to form a lyophilized solid.
The compositions of both the liquid precursor solutions and the final powders are shown in Table 2.

Sample Compositions liquid (%, w/v) and dried (%, w/w)*
#1 #2 #3 #4 #5 Polymer HMW AP LMW AP LM pectinPolyGal Alginate A

0.4 0.8 0.8 0.8 0.8 (0.03) (0.06) (0.06) (0.06) (0.06) Povidone 7.5 7.5 7.5 7.5 7.5 (57.69) (56.39) (56.39) (56.39) 56.39) Lactose 5 5 5 5 5 (38.46) (37.59) (37.59) (37.59) (37.59) Active agent 0.1 0.1 0.1 0.1 0.1 (BSA or lysozyme)(0.0077) (0.075) (0.075) (0.075) (0.075) *Numbers in parenthesis indicate the percent content of each ingredient in dried form on the moisture-free basis (w/w).

The lypholized solids were milled using an Eberbach blender with a micro-container. The resulting powder was sieved using a sterile 100 ~,m nylon membrane sieve to produce powders with a particle size < 100 ~.m and then sequentially with sterile nylon membranes of various pore sizes (40, 70, and 100 Vim; Cell strainer, Becton Dickinson Labware), yielding powders of various particle sizes (<40, 40-70, and 70-100 ~,m). The >
100 ~,m particles were also further sieved using a 200 ~,m sieve to produce 100 -200 ~m particles. The sieving was performed under vacuum using a glass filter holder and the powders were collected onto a 0.22 p,m membrane. The powders were stored at room temperature.
Control powders were also made with formulations having all components, except for the ionic polymers.
Two powder formulations made with HMW Aloe pectin according to Table 2, one sample with BSA and another control without BSA, were prepared, milled, and sieved to <
100 Vim. The moisture content of both these two samples was determined to be 2-(w/w) using a moisture analyzer at a drying temperature of 120 °C.

Gelation Properties of Powder Formulations.
To demonstrate gel formation properties of the powder formulations whose preparation is detailed in Example 15, powders (10 mg, < 100 ~,m) made with the various pectins and alginate were suspended in 2 ml saline solutions. The saline solutions of one sample set comprised 3 mM calcium chloride, and the other did not comprise calcium chloride. In the presence of calcium, the powder particles hydrated but remained in the form of particles, and the suspension remained cloudy. Under the microscope, the powder particles in calcium saline changed into clear and transparent gel particles or pieces. In contrast, in the absence of the calcium the particles quickly dissolved within ~ 10 min and the suspension changed into a clear solution (except for the powder made with the high molecular weight Aloe pectin, which is not readily soluble in typical NaCI
saline but also does not gel in the saline, see discussion below).
When the calcium chelating agent EDTA (10 mM) was added to the powders suspended in calcium saline describe above, the particles quickly dissolved within ~ 10 min.
Similar results were obtained when the powders made with pectins or alginate were suspended in normal calf serum. That is, powder particles remained in the form of solid particles after being suspended in calcium containing normal calf serum. But, upon addition of EDTA the particles mostly dissolved in ~ 10 minutes. Similar results were also obtained in simulated nasal fluid (0.867 g NaCI, 0.44 g NaaHP04, 0.108 g NaH2P04, 0.058 g CaCla.2H2O, 0.31 g KCl per 100 ml. See, Lorin et al., .Journal of Laboratory Clinical Medicine, 2, 275-267, 1994). These experiments are evidence that the powder particles suspended in the solutions containing free calcium ions formed a calcium crosslinked gel, but in the absence of calcium, or if the calcium was removed from the gel by the chelating agent, no gel was formed or was stable, and the polysaccharide particles dissolve.
As noted above, HMW Aloe pectin is soluble in water, but is not readily soluble or only partially soluble in NaCI saline or buffered saline. Powder particles comprising HMW Aloe pectin recovered from NaCI saline solutions by centrifugation (500 g for 5 min) and re-suspended in water quickly dissolved in a few minutes. This behavior contrasts with particle made from low molecular weight LM pectins, polygalacturonic acid, LMW Aloe pectin, or alginate, which are readily soluble in both water and NaCI
saline solutions.. Nevertheless, particles prepared from particles isolated from calcium-containing saline or normal calf serum solution rerrrained in the form of particles when placed i water, indicating the various polysaccharide powder particles had all gelled in the presence of calcium ions.

Comparison of Solid and Liquid Formulation For Gel Formation and Control of Drug Release.
Liquid formulations consisting of aqueous solutions of different anionic polysachharides and Fast Green dye (1 mg/ml) were prepared. Fast Green was used to simulate a small molecule therapeutic agent. The concentrations of anionic polysaccharide polymers employed were 0.5% for HMW Aloe pectin, 1% for alginate, and 2% for polygalacturonic acid, LMW Aloe pectin, and LM citrus pectin. To prepare the solid formulations, 20 microliters of the aqueous formulations were placed on a weighing tray as a drop, lyophilized, and then recovered as a dried disc.
The dried formulation discs, or 20 microliters of the liquid formulations, were placed in 3.5 mililiters of normal calf serum in 60 mm petri dishes, With or without the addition of 10 mM EDTA,. The diffusion of the Fast Green dye, which simulates the release of a drug agent, was observed by measuring over time the diameter of green dye diffusion circle around the initial insertion points of the fornmlations.
Tn normal calf serum without EDTA, the dried formulation discs remained in the form of a solid disc and gradually changed into clear and solid gel pieces.
After 24 hours, when all the dye diffused away, the gels from the dried formulation tuned clear and transparent. The gel formation of the dried formulation was further confirmed by soaking the gel discs in saline with 10 mM EDTA, wherein it quickly dissolved in ~ 30 min. In normal calf serum containing EDTA, the dried formulation discs also gradually dissolved, as either a disc or film.

In contrast, most of the liquid formulations gradually dissolved and/or diffused away, without formation of distinct gel pieces resembling the original drop, and formed only a thin layer of gel pieces as detected after gently shaking the petri dishes after 2 hours.
Therefore it appears that the powder formulations gelled more effectively than the liquids.
Nevertheless, when dropped into a 50 mM CaCla solution though a 25 G needle, the liquid formularions all held together and formed gel beads. Nevertheless, liquid formulations made with HMW Aloe Pectin held together and formed a small piece of gel with a size only slightly bigger than the original drop size in the serum. This underscores the high efficiency for gel formation shown by the high molecular weight aloe pectins.
Together, these observations indicate that the efficiency of ire-situ gel formation of a dried formulation can be superior to that of a liquid formulation.
The diameters of the diffusing Fast Green circle around the formulations immersed in normal calf serum with and without EDTA were measured over time with both dried and liquid formulations (see Figure 6). It appear that the gel formation in either solid or liquid samples without EDTA slows the dye or drug release consistent with the observation that gel formation is more efficient with the dried formulation. The same observation was observed with all formulations, except for the dried formulation with HMW Aloe pectin which exhibited a dye diffusion that was only slightly faster in sera with EDTA than the one without EDTA. This may be related to that the fact that HMW Aloe pectin is less soluble or insoluble in saline, which again, is another distinct feature of the HMW Aloe pectin.

Use of Powders Comprising Soluble Calcium Salts to Induce In-Situ Gelation of Polysaccharide/Agent Powder Formulations Two powder formulations comprising a protein active agent (BSA) and a polysaccharide selected from LMW Aloe pectin or alginate (as described in Table 2, samples 2 and 5) were sieved to produce powders having particle sizes under 100 ~,m. A
calcium-containing powder was made from a liquid formulation comprising 2.5%
(w/v) polyvinylpyrrolidone, 10% (w/v) lactose, and 1% (w/v) calcium chloride, drying the solution, and grinding the solid and sieving the powder to particle sizes of <40 ~,m, produce a gel inducing powder with a calcium chloride content of 7.4% after drying. The polysaccharide powders and gel inducing powders were mixed 4:1 by weight, resulting in a final calcium chloride content of the powder mixture of 1.48% (w/w).
The powder mixture was suspended in saline (5 mg in 1 ml). All three unmixed powders (i. e. pectin + protein, alginate + protein, and calcium-containing gel inducing powder dissolved when suspended individually in NaCl saline. Nevertheless, mixtures of the calcium gel inducing powder with powders comprising LMW Aloe pectin+
protein, or alginate + protein did not dissolve in NaCI saline. The same results were also obtained with lysozyme as the active agent. These results suggest that the calcium containing powder induced the polysaccharide/protein powders to gel when in contact with a saline solution model of a body fluid.

Use of Powders Comprising Poorly Soluble Multi-Valent Cation Salts to Induce In-Situ Gellation of Polysaccharide/Agent Powder Formulations.
Aluminum hydroxide (Al(OH)3) is poorly soluble in water, but has been approved as a pharmaceutical adjuvant for human use. An aluminum hydroxide suspension purchased from Sigma Chemical Co. was a whitish, cloudy, but homogenous particle suspension. An Aloe pectin solution (2 mg/ml in water) formed a gel when mixed with the insoluble aluminum hydroxide gel suspension, as indicated by the formation of visible large aggregates of aluminum hydroxide particles. The same observations were also observed with other pectins and alginate. The aggregates were large and easily visible when proper polymerlaluminum hydroxide ratio were reached. Similar results were also observed with calcium phosphate (Sigma Chemical Co.), although the aggregates formed were not as large as those with aluminum hydroxide. Both aluminum hydroxide and calcium phosphate are relatively insoluble materials (Merck Index, 13th ed.), but these poorly soluble salts apparently ionized at the surface when hydrated, allowing reaction with the Aloe pectin.
To further explore this observation, aluminum hydroxide and calcium phosphate powders were suspended in water or saline (10 mg/ml) and then mixed with HMW
Aloe pectin solution at various final concentrations (2.5 - 0.0012 mg/ml). The same gel formation indicated by large aggregate formation was observed. The same observation was also made with alginate, LM pectin, and polygalacturonic acid, indicating that it is possible to use poorly soluble metal divalent or multivalent cation salts as a gel-inducing agent.
As an example, a powder formulation made with Aloe pectin (HMW) as in example 15 was mixed with aluminum hydroxide powder at a 3:1 ratio. The mixtures (10 mg) were suspended in 2 ml saline. Large aggregates were immediately formed. Toluidine blue was added to the suspension to stain the ionic polymer powder particles. After 30 minutes or more, a small drop of the suspension was placed onto a glass slide and observed under a microscope. The aggregates consisted of both pink-stained formulation powder particle and the opaque grayish aluminum hydroxide particles, confirming the aggregate formation.

As a second example, a powder formulation made with LMW Aloe pectin was mixed with aluminum hydroxide powder at 3:1 ratio, and the powder mixture suspended in the saline. Although aggregates formed, there were few pink-stained formulation powder particles observed under the microscope and the aggregates appeared to consist primarily of the aluminum hydroxide particles. This indicates that the formulation powder particles dissolved and the insoluble salts did not cause gelation of the whole formulation particles.
However, when the polysaccharide formulation/ aluminum hydroxide powder mixture was suspended in saline comprising 3 mM calcium chloride, the polysaccharide formulation particles were again observed, aggregates also formed consisting, of the formulation particles and the aluminum hydroxide particles. The same aggregate formation was also observed when the mixture was suspended in normal calf serum.
The poorly soluble metal ion salts may not easily penetrate polysaccharide containing formulation particles, and therefore may not cause gellation of the whole particles, and may only cause the polymer cross-linking or gellation on the surface of the particles. Because they are only poorly soluble, or close to insoluble, the undissolved multi-valent cation-containing particles can act as a physical Garner for a gel, or as a long-lasting source of crosslinking divalent or multi-valent cations. Additionally, the formulation powder particles and the poorly soluble solid gel -inducing agents can cause the formation of gelled aggregate compositions. Dependent on the ratios and relative particle sizes of these two different powders in a mixture, the size and other characteristics of the aggregates formed can be varied and/or modulated. At a high or low ratio, the aggregate particles sizes can be very small, with one particle of one type surrounded by particles of another type, whereas at a ratio of ~1, the particles can interconnect as a network, forming a large network. Therefore, aggregate gel complexes formed under various conditions can be used to modulate the physical, solubility, and time release characteristics of in-situ gels formed at a site of administration, such as mucosal surfaces and/or the nasal cavity.

Sustained release of pharmaceutically active agent from powder formulations The effect of in-situ gelling powder formulation on the release of the active agent was evaluated using simulated nasal fluid (SNF) as a release media. The powder formulations were made as above with various amounts of povidone and lactose, but all had same protein (BSA) content (0.1% on dry weight basis) (See Table 3).
Control powders contained all components except for the ionic polymer (HMVd Aloe pectin).
Table 3 Formulation Composition liquid (%, w/v) and dried (%, w/w)*

Control Control HMW AP 0.4 0 0.4 0 (2.6) (0) (3.1) (0) Povidone 15 15 2.5 2.5 (97.3) (99.93) (19.3) (19.97) Lactose 0 0 10 10 (0) (0} (77.4) (79.9) BSA 0.015 0.015 0.0125 0.0125 (0.097) (0.099} - - X0.097) (0.099) * on the moisture-free basis Ten mg of powders were suspended in 0.25 ml SNF. After 30 min, the solution or supernatant was separated from the particles or pellet by centrifugation and the protein in the supernatant and pellet were analyzed by SDS gel electrophoresis and densitometry analysis. The percent release of the protein agent from each formulation was determined by the following formula - [protein in supernatantl(protein in supernatant +
protein in pellet)] x 100%. It was observed that proteins were almost all released from the control powders (>90% released), which were all completely dissolved. On the contrary, the protein release was significantly slowed from powders with Aloe pectin; only 55%

(formulation 1) or 6~% (formulation 2) was released with powders made with the ionic polymer (Figure 7). Similar results were also obtained with lysozyme as the active agent.
It was also found that protein release was faster from formulation 2 than formulation 1.
The formulation 2 had 2.5% PVP and 10% lactose, whereas formulation 1 contained 15%
PVP and no lactose (Table 3). This indicates that the release rate can be further adjusted by the amount and type of excipients used.

Physical Mixtures of Powders of Pharmacalogically Active Agents, Polysaccharides, Gel Inducing Compostions, and Other Excipients A powder formulation as in Table 2 is made in the absence of an active agent and sieved to an appropriate size. A powder of an active agent made with or without a pharmaceutically acceptable excipitent is then blended with the polymer powder. One or more solid gel inducing compositions as described elsewhere herein may also be optionally included. The mixture of powders is then delivered to an animal.

Intranasal Delivery of a Powder Vaccine Formulation Comprising An Antigen to an Animal.
A powder vaccine formulation comprising high molecular weight Aloe pectin and a diphtheria toxin mutant CIZ1VI (DT-CRM) antigen was prepared by dissolving the components listed in Table 4 in an aqueous solution, lyophilizing the solution to produce a powder, grinding the powder, then sieving the powder. Control formulations containing all the ingredients except for the antigen were similarly prepared.

Table 4 Antigen Control Components formulation formulation liquid (%, w/v) and liquid (%, w/v) and dried dried (%, w/w) (%, w/w) ~W ~ 0.4 0.4 (3.1) (3.1) Povidone 2.5 2.5 (19.4) (19.4) Lactose 10 10 (77.5) (77.5) DT-CRM 0.01 0 (0.077) (0) The vaccine formulations were made to deliver 7.75 ~,g antigen per 10 mg powder formulation. Rats weighing 200-250 grams were first anesthetized and 10 mg the powdesr were delivered into each nostril using a 200 ~,l pipette tip connected to a 5 ml syringe, using 3 ml of air through a rubber tube as previously described (Ryden and Edman, Int. J.
P72arna. 83 (1992), pp. 1-10; Schipper et al., Plaa~m. Res. 10 (1993), pp. 682-686).
Serum samples were collected from the rats one week after inoculation and specific serum IgG (immunoglobulin G) was assayed via ELISA (enzyme-linked imrnunosorbent assay). The end point for IgG titer was determined as the reciprocal of the highest dilution that has an absorbance value 50% greater than the background (absorbance of the antigen-coated wells without serum added).
The two rats that received the DT powder developed specific antibodies to the DT-CRM antigen with a mean IgG titer of 800 after only one week. The two control rats that received the control formulation having no DT-CRM antigen developed no such antibodies (Figure 8). This result indicates that nasally administering the powder vaccine formulation effectively induced a specific immune response in the rats.

Delivery of Powder Formulations to Animals Parenterally As described in Example 16, powder particles remain as particles or change into gel particles when suspended in calcium-containing saline. Thus, the powders may be injected as a particle suspension after being suspended in a calcium saline or calcium buffered saline. Alternatively, the formulation powders may be pre-mixed with calcium powders as described in example 17 wherein the powders are suspended in saline or buffered saline prior to injection into the tissues of an animal. The formulation powders described in Example 16 having a powder particle size < 100 ~,m were employed, although smaller powder particle sizes can be desirable for embodiments related to injection of suspended powders.
Each powder (80 mg) was suspended in 0.4 ml saline containing 3 mM CaCl2 and injected subcutaneously into mice (0.1 ml per injection site, two sites/mouse). At 4 hours post injection, the mice were sacrificed, the skin peeled open, and the injection sites were examined. A small nodule or swelling area representing the hydrated and gelled particles was observed at an injection site with powder formulations with an ionic polymer. In contrast, no such small nodule or swelling area was observed with the control powder made without an ionic polymer. Additionally, the injection sites were very moist, including those from the control, perhaps because of the presence of polyvinylpyrrolidone, which is a highly water-absorbing polymer.

Gelation of Liquid Formulations as Influenced By Exogenous Gel-Inducing Agents and Compositions A 0.6% (w/v) HMW Aloe pectin solution in water was mixed with calcium chloride dehydrate solutions at various concentrations, at an 1:1 ratio (1 ml to 1 ml) to achieve a final polymer concentration of 0.3%. (wlv) and a final calcium chloride dihydrate concentration from 0.0019 - 0.5% (w/v). See Table 5 below. The mixtures were immediately vortexed together, then the tubes were kept at room temperature and observed over time. A complete or partial gel formation clearly occurred upon mixing at a final calcium chloride concentration above 0.03125% (w/v) (2.125 mM) since the solution was completely or partially solidified and no longer free-flowing when tubes were tilted. At a concentration of 0.0156% CaCl2 the viscosity of the solution was increased and granular gel pieces were present. However, at a final concentration of <0.0078% (0.53 mM) or lower, there was no hint of gel formation and the mixture remained homogenous and remained so after more than 24 hrs.
Table 5 Concentrations (%, w/v, final)*
0.5 0.25 0.125 0.0625 0.0313 0.0156 0.0078 0.0039 0.0019 0 (:aL12.2Hz0 + + + + + ~ _ _ _ _ ZnClz + + + + + ~ _ _ _ _ * + indicates whole gel formation, ~ partial gel formation, and - no gel formation and solution remains clear and homogenous.
To demonstrate that incorporation of the divalent cation can increase the in-situ gelation, a gel frontal migration assay with normal calf serum was performed as described in Example 3. Thus, 1 ml 3 mg/ml pectin solutions containing 0%, 0.0039%, or 0.0078%
calcium chloride or zinc chloride was gently layered on to 3 ml normal calf serum in a 10 x 75 mm glass test tubes. Starting at the interphase, gel gradually formed in the pectin solution phase. The gel could be readily identified under a light source due to its slightly increased turbidity as compared to the solution. Thus, the length (thickness) of gel in the pectin solution phase at the interface was measured over time. The results showed that gel formation increased at both exogenous calcium chloride concentrations tested when compared to the control that has no added calcium chloride (Figure 9).

It should be noted that the results in Table 5 can be advantageously employed, in that small amounts of a divalent cation such as calcium or zinc (i.e. below about 0.0156 (w/v) can be added to pectin/agent solution without causing significant gellation, with the unexpected result that when the solution is administered to a tissue or body fluid comprising calcium ions, improved gellation will be induced.

Effect of various monovalent cations on the solution properties of LM pectins NaCI and NH4Cl were prepaxed in water at various concentrations. They were then mixed 1:1 v/v with solutions of LM pectin, HMW Aloe pectin, or a HM pectin.
The HM
pectin (DM=64%, Sigma chemical Co) was filtered to remove insoluble materials as described in Example 15. The solutions were then observed at room temperature for 1 hr.
They were then cooled at 4 °C for'2 hrs or longer and examined again.
The pectins with a degree of methylation below 50% exhibited a salt concentration-dependent precipitation of pectins at room temperature (see Tables 6 and 7).
HMW Aloe pectin was most prone to precipitate formation, followed by the LM pectin.
Using HMW
Aloe pectin, a pectin concentration-dependent effect was also observed, i.e., pectin at a lower concentration is less prone to precipitate formation. For example, precipitate formation slowly occurred in 0.15 NaCI with a 0.5% HMW Aloe pectin solution, but not with a 0.1 % pectin solution. In addition, there was an effect of molecular weight, since no precipitation was observed with 0.5% LMW Aloe pectin in 0.15 M NaCl. HM pectin solutions did not form precipitate or gel with either salt at any concentration or temperature tested.

Table 6 NaCI (1VI) 0 0.1 0.15 0.2 0.4 0.6 0.8 1.0 HMW AP 0.1 % - (-) - - (G) - (G) P P (P) P (P) P
(-) (P) (P) (MW=15x105) 0.5% - (-) - P (G/P) P (P) P (P) P (P) P
(G/P) P (P) (P) LM pectin (0.5%) - (-) - - (-) - (-) - P (P) P (P) P
(-) (-) (P) HM pectin (0.5%) - (-) - -. ' (-) - (-) - (-) - (-) -(-) - (-) ~-) "-", no change; "P", precipitate formation; "G", clear gel, "G/P", cloudy gel;
Letter or sign in parentheses indicates the observations after keeping samples at 4 °C
for 2 hr.
Cooling at 4 °C increases precipitate formation. Nevertheless, with 0.1% HMW
Aloe pectin, a clear gel was formed at 0.15 and 0.2 M NaCl. This gel was reversible, changing back to a solution when brought back to room temperature. This reversible gelation could be performed over several times by changing between 4 °C
and room temperature. Once changing back to the solution at room temperature, the preparation still gelled in-situ with the normal calf serum as described in Example 25.
These observations indicate that the precipitate or gel formation is related to low DM and HMW, i.e., the lower the DM and the higher the molecular weight, the more prone a pectin is to precipitation by a salt.
A marked difference was observed between NaCI and NH4Cl; the concentration of NH4Cl required for precipitate formation was much higher than that with NaCI.
A similar pectin concentration-dependent effect was also observed. See Table 7. With the 0.5%
HMW Aloe pectin, precipitate occurred at 0.6 M at room temperature and 0.4 M
at 4 °C.
The precipitates were whitish and could be fine or large granule-like depending on the salt concentration. The precipitates were the finest at the cut-off point or the salt concentration at which precipitates first appeared. This is in fact one efficient way to make pectin fine particles that can be used for drug delivery.

Table 7 NH4Cl (M) 0 0.1 0.15 0.2 0.4 0.6 0.8 1.0 HMW AP 0.1 % - (-) - (-) - (-) - (-) - (-) - (-) - (P) P ~') 0.5% - (-) - (-) - (-) - (-) - P (P) P (P) P (P) (G/P) LM pectin (0.5%) - (-) - (-) - (-) - (-) - (-) - (-) - (-) - (-) HM pectin (0.5%) -. ~-) - (-) - (-) - (-) - (-) - (-) - (-) - (-) "-", no change; "P", precipitate formation; "G", clear gel, "G/P", cloudy gel;
Letter or sign in parentheses indicates the observations after keeping samples at 4 °C
for 2 hr.
Beyond revealing the fundamental properties of different pectins, these observations indicate that for preparing a liquid formulation with HMW Aloe pectin at a physiological ionic strength or as an isotonic solution (as embodied by 0.9%
(w/v) - 0.154 M NaCl) an alternative to NaCI is needed if the formulation needs to be stored as a solution at 4 °C and a pectin concentration > 1 mg/ml will be used, as might be envisioned for a liquid ih-situ gelling formulation physiological ionic strength of an unstable active agent such as a protein, which would need to be stored in a refrigerator.
Precipitation of some or all of the pectin from such solution on cold storage would be highly undesirable.
One such alternative salt that can be used in such a formulation is NH4C1, particularly at its concentration for an isotonic solution (0.84% (w/v) or 0:157 M, which is also equivalent to 0.154 M NaCI in ionic strength). At this concentration, NH4Cl also improves ifz-situ gelation of such liquid pectin-based pharmaceutical compositions.

In-situ gelation of Aloe pectin in the nasal cavity An 0.5% Aloe pectin solution was prepared in 10 xnM NaH2P04/ Na2HPO4 buffer, 0.84% NH4C1, pH 7.4, with or without a protein (BSA). The liquid formulation was delivered intranasally by dropping directly onto the nares of mice following anesthesia by inhalation of metofane, 20 ~1/mouse evenly divided between the two nares. At 4 h post inoculation, mice were sacrificed and tissues were fixed in formalin. Serial cross sections were made of the nasal cavity starting anterior to the orbit of the eye.
The gel was detected by staining tissue sections with toluidine blue and H&E.
The toluidine blue revealed in-situ gel as a pinkishlpurplish substance, whereas the H&E
stained the gel pale pinkish (Figure 10). The gels were of various shapes and sizes, and could be found in various nasal cavity areas including those near the septum and middle and inferior concha.
To determine the effect of Aloe pectin concentration, Aloe pectin solutions at 0.25 or 0.5 % were delivered intranasally to 2 mice per concentration. Gel formation was examined microscopically 4 hours after delivery. The area of gels in each section was measured by using Image) software (National Institute of Health) and expressed as mma.
The gel areas on cross sections at the same position were used as an indirect measurement of the relative amounts of gel present in the nasal cavity. Thus, the results showed that more and larger gels were detected in the nasal cavity with 0.5 % than 0.25%, suggesting that the amount of gel formed in the nasal cavity is polymer concentration-dependent.

Comparison with other pectins for in-situ gelation in the nasal cavity Various commercial LM pectins were used along with HMW Aloe pectins (Table 8). The commercial pectins, i.e., Genu pectins and polygalacturonic acid from Sigma Chemical Co., were used as purchased. One sample obtained by reprocessing Genu pectin LM12G was also used. It was dissolved in water, microfiltered, recovered by alcohol precipitation, and designated Genu pectin LM12G (R) after being dried under vacuum. The molecular weight of Genu pectin splendid type 100 was similar to other low molecular weight pectins (Table 8). Two different HMW Aloe pectin samples designated as A and B were used.

All commercial pectin samples were prepared as a 2% (w/v) solution in water and were then diluted 1:1 with a 2 x saline solution (0.3 M NaCI). These commercial pectins produced a low pH when dissolved, i. e. 3 - 4. The pH of the solutions was adjusted to 6.5 with NaOH. The HMW Aloe pectins were prepared as above with a final concentration of 0.5 % (w/v) in 0.84% (w/v) NH4Cl. The pH of HMW Aloe pectin solution was 5.5 -6.0 and no pH adjustment was made. All samples were delivered intranasally to mice as above, 2 mice per sample. Gel formation was examined 4 hrs later as above.
TahlP R
Pectins DM MW ConcentrationGel areas ~A x 105) (%, w/v) (mm~') Genu ectin LM12G31% NA 1 0.0075 p Genu pectin LM12G31% < 2.0 1 0.0015 Genu pectin LM18G40% NA 1 none observed Genu pectin 15% 3.8 1 none observed splendid type Polygalacturonic<3% 1.7 1 0.0023 acid, Sigma Chemical co HMW AP (A) <10% >10 0.5 0.049 HMW AP (B) <10% >10 0.275 0.051 Two cross sections were made of the nasal cavity starting anterior to the orbit of the eye from each mouse. The gel area on the cross sections at the same position was used as an indirect measurement of the relative amounts of gel present in the nasal cavity. The total gel areas on all 4 sections from the two mice from each group was determined and divided by 4 to produce the average gel area per cross nasal section. The results showed that gels were detected with Genu pectin LM12G, Genu pectin LM12G (R), polygalacturonic acid, and HMW Aloe pectins, but no gel was detected with formulations employing the LM18G and Slendid Type 100 pectins, which are both pectins with low degrees of methylation and typical molecular weights. The areas of the gels detected with Genu LM12G and polygalacturonic acid were very limited or 6.5 to 33 fold smaller as compared to the gel areas measured for the formulation prepared from the HMW
Aloe pectins, which were used at a concentration at least 2-fold lower concentrations(see Table 8). These results also illustrate the unexpectedly superior gellation properties of HMW aloe pectins, as compared to prior art pectins.

Nasal residence time of the in-situ gel To determine the nasal residence time of in-situ gel, an HMW Aloe pectin solution (5 mg/ml) in 0.84% (w/v) NH4C1 was delivered intranasally and gel formation was examined at various'time points using two mice per time point. ' The relative amounts of gel present were determined by measuring the gel areas on nasal cavity tissue sections as above.
The results showed that gel was present in the nasal cavity through 24 h, but disappeared by 48 h-(Table 9). Based on gel areas measured in the cross section of the nasal cavity, 50% clearance occurred at 24 h. Thus, the gel stayed in the nasal cavity between 24 and 48 h.
Table 9 Hours Presence of gel Yes Yes Yes Yes* No * At 24 h post intranasal delivery, the amount of gel in the nasal cavity was reduced by >
50% as measured by gel areas in the cross section of the nasal cavity.

Increased immune response against DT-CRM and influenza antigens following intranasal delivery with liquid formulations to animals Anti~etzs, anianals and ifzoculation: Two antigens, DT-CluVI (diphtheria toxin mutant CRM) and inactivated subvirion split influenza virus antigen (A/New Caledonia/20/99, H1N1), were used. Groups of 7 female 6-8 week old Balb/c mice were inoculated intranasally 2 or 3 times, 10 days apart with formulations consisting of antigen (0.5 mg/ml), HMW Aloe pectin (5 mg/ml for DT-CRM and 2.75 mg/ml for influenza), or a combination of both by dropping them directly onto the nostrils of mice (20 ~,1/mouse).
The antigen dose was 10 ~,g/mouse. The antigen formulations were prepared in 0.84%
NHøCl and 10 mM phosphate buffer, pH 7.4 Sample collection and ELISA: Blood and lung wash samples were collected two weeks after the last inoculation. Specific serum IgG (immunoglobulin G) and lung IgA
(immunoglobulin A) were measured by indirect ELISA (Enzyme-linked immunosorbent assay). For influenza (Flu), recombinant HA (Hemoagglutinin) protein of A/New Caledonial20/99 (H1N1) obtained from Protein Science Co. was also used as an antigen for detecting HA-specific response. The end point for IgG titer was determined as the reciprocal of the highest dilution that has an absorbance value 50% greater than the background (absorbance of the antigen-coated wells without serum added). Each lung wash was assayed for antigen-specific and total IgA in two separate ELISA
protocols. The results were expressed as ng (specific)/~g (total). To determine the level of antigen-specific IgA, the plates were coated with antigen and also serially diluted purified mouse IgA standard (1.0 to 0.002 ~,g/ml). The level of antigen-specific IgA was calculated from the standard curve generated with the absorbance values of the purified IgA
standard.
Total IgA was determined by a sandwich ELISA with purified mouse IgA as a standard.
Mean IgG titers in serum and specific to total IgA ratios in lung wash along with their standaxd errors were determined for every group of mice. Means were compared using Student's t test. A serum sample having a titer > 10 or a lung wash sample having a specific/total IgA ratio 2 times higher than the control was considered a responder.

Results Strong serum IgG and lung IgA responses were only obtained when antigens were delivered with Aloe pectin. Minimal or no response was detected with antigen alone.
DT CRM: The serum IgG and lung IgA responses were significantly higher when antigen was combined with Aloe pectin than antigen given alone after either single or multiple inoculations. The peak response was detected at week 3 with Aloe pectin /DT-CRM after single inoculation. The response was also initiated faster with Aloe pectin /DT-CRM, detectable at week 2.
After three inoculations, mice in the Aloe pectin/DT-CRM group had serum IgG
and lung IgA titers that were significantly higher (50 or 100 times, respectively) than the DT-CRM alone group (Figures 11a and 11b). In addition, all 7 mice in the Aloe pectin/DT-CRM group responded with both serum IgG and lung IgA, whereas only 4 of 7 responded with serum IgG and 3 of 7 with lung IgA in the group given DT-CRM
alone.
No response was detected in the Aloe pectin alone group.
Ih ueuza: After two inoculations, mice receiving Aloe pectin /Flu antigen had significantly higher serum IgG (6 times) and lung IgA (60 times) titers than the group given the Flu antigen alone (Figures llc and 11d). For serum IgG, all 7 mice in both Aloe pectin /Flu antigen and Flu antigen alone groups responded. However, for lung IgA, 6 of 7 responded in the Aloe pectin /Flu antigen group and only 1/7 in the Flu antigen alone group. No response was detected in the Aloe pectin alone group.
The same results were also obtained when recombinant HA protein was used as the antigen in ELISA for measuring HA-specific IgG or IgA.

In-Situ Gelling Influenza Nasal Powder Vaccine Composition Comprising Lactose and Aloe Pectin A powder nasal influenza vaccine formulation was prepared by mixing lactose (Sigma Chemical Co or NF grade, Fisher Scientific), a very low methoxyl and high molecular weight Aloe pectin as obtained from DelSite Biotechnologies Inc of Irving Texas, and influenza antigen solutions. The antigen were split subvirion antigens; derived from A/New Caledonia/20/99 strain, HlNl, Lactose and Aloe pectin (AP)were dissolved in water, while the antigen was prepared in water or buffered saline (10 mM phosphate, pH 7.2; 150 mM NaCI or NH4Cl);
at the concentrations shown in Table 1, then mixed in the indicated volumes.
The liquid mixture was then lyophilized. For lyophilization, the liquid mixture was frozen at -80 C
for 1 hr and then dried under vaccum till < 100 micron Hg (Centrivap, Labconco).
Lyophilization produced a porous solid, which was milled in a microblender to produce a powder which was sized to 40-100 ~,m under vacuum using sterile 40 and 100 um nylon membranes (cell strainers, BD). Depending on the blender speed and blending times, the yield of the 40-100 um particles could vary, but could be >50% of the dried formulation. A
similar control formulation without the antigen was also prepared without including the antigen.
Table 9.
Solution Vol % w/v % w/w Components (ml) (liquid(calculated, mixture)post drying) Aloe Pectin 1 0.1 1 (1 gr/100m1) Lactose 5 10 98.7 (20 gr/100m1) Influenza Antigens1 0.029 0.289 0.29 gr/100m1 Water and buffered3 - -saline As shown in Table 9, the powder was calculated to comprise about 98.7 wt Lactose, 1 % by weight Aloe Pectin, and 0.289% by weight influenz antigen, and was formulated so as to deliver 28 ~,g antigen per 10 mg powder formulation. A
control formulation without the antigen was also prepared.
One group of three 200-gram Sprague-Dawley rats was inoculated intranasally with the antigen containing formulation and another group of three rats inoculated intranasally with the control formulation. The rats were first anesthetized and 10 mg of the powder was delivered into each nostril using a 200 ~l pipette tip connected to a 5 ml syringe, using 3 ml of air through a rubber tube as previously described (see Ryden and Edman, Int. J.
Pharm. 83 (1992), pp. 1-10; Schipper et al., Pharm. Res. 10 (1993), pp. 682-686). The rats were treated again 10 days later via the same procedure.
Blood samples were collected from the rats at 2, 4, and 6 weeks after the second inoculation. The lung wash sample was also collected at the end of the experiment (week 6). The lung wash was performed after the animals were euthanized through an insertion into trachea using 3 ml of phosphate buffed saline. Specific serum IgG
(immunoglobulin G) and lung IgA were assayed with indirect ELISA. The 96-well plates were coated with the influenza antigen and specific IgG from serum samples bound to the antigen were detected with anti-rat IgG-alkaline phosphatase conjugate. The end point for IgG titer was determined as the reciprocal of the highest serum dilution that has an absorbance value (410 nm) SO% greater than the background (absorbance of the antigen-coated wells without serum added).
Each lung wash was assayed for antigen-specific and total IgA in two separate ELISA protocols. The results were expressed as ng (specific)/~,g (total). To determine the level of antigen-specific IgA, the plates were coated with antigen and also serially diluted purified rat IgA standard (1.0 to 0.002 ~,g/ml). The level of antigen-specific IgA was calculated from the standard curve generated with the absorbance values of the purified IgA standard. Total IgA was determined by a sandwich ELISA with purified rat IgA as a standard.
Specific serum antibodies were also measured by hemagglutination inhibition assay (HAI) with chicken red blood cell (RBC). The endpoint of HAI titer was the highest serum dilution that produced a positive inhibition of agglutination of the RBCs. Mean IgG
and HAI titers in serum and specific to total IgA ratios in lung wash along were determined for every group of rats.
No antibody responses were detected in the control group. High serum antibody responses as shown by ELISA and HAI were observed in all three rats that received the influenza antigen powder formulation (See table 2). In humans, a hemagglutination inhibition (HAI) titer of >40 is generally considered the protective threshold. The observed HAI titers from the treated rats were all higher than 1:40 and proportional to IgG titers by ELISA. In addition, a significant level of specific lung IgA was also detected at the end of the experiment (i.e week 6).
Table 10. Average Antibody Titers Time Serum IgG Serum HAI Lung IgA
(wks (ELISA) n /w ) In-Situ Gelling Influenza Nasal Powder Vaccine Composition Comprising Lactose, Aloe Pectin, and Polyvinylpyrrolidone A powder nasal influenza vaccine formulation was prepared by mixing lactose (Sigma Chemical Co or NF grade, Fisher Scientific), Aloe pectin, polyvinylpyrrolidone (Povidone K29-32, USP; Sigma Chemical Co), and influenza antigen solutions (split subvirion; A/New Caledonia/1/99, H1N1) according to the menu in Table 11.
Lactose, Aloe pectin, and povidone were dissolved in water while the antigen was prepared in water or buffered saline (10 mM phosphate, pH 7.2; 150 mM NaCI or NH4C1). The liquid mixture was then lyophilized and made into powder as described above. A
control formulation without the antigen was also prepared without including the antigen.
The powder was calculated to comprise about 98.8 % by weight lactose, 0.5 % by weight Aloe Pectin, and 0.2% by weight antigen, and was formulated so as to deliver 20 ~g antigen per 10 mg powder formulation. A control formulation without antigen was also prepared.
Table 11 Com onents Vol % w/v % w/w ( ost dr (ml) in Aloe Pectin 0.5 0.05 0.5 (1 gr/100 ml) Lactose 5 10 98.8 (20 gr/100 ml) Povidone 0.017 0.05 0.5 (30 gr/100 ml) Influenza Antigen 2 0.02 0.2 (0.2 gr/100 ml) Water and buffered 2.483 - -saline Animal experiments and antibody measurement were conducted same as above, except for that lung wash samples were not measured. No antibody responses were detected in the control group. High serum antibody responses as shown by ELISA
and HAI
were observed in all three rats that received the influenza antigen powder formulation (See table 4).
Table 12. Average Antihndv Titerc Time Serum IgG (ELISA) Serum HAI
(wks Use of pH to control gelation or precipitate formation of powder formulations There axe many polymers that gel or form precipitate in response to a change in pH.
For example, chitosan glutamate is soluble at a pH up to 6.5. But beyond pH
6.5, it becomes insoluble, forming precipitates or gel-like substance which can be used for controlled drug delivery. Thus, a liquid drug formulation with chitosan is prepared at pH
6.5 or lower and made into a dry powder using a method described above.
Following delivery, these particles can be partially or completely dissolved due to its internal buffering capacity, although they may be hydrated by a bodily fluid or secretion having a pH of 7.0-7.4. In the case of intranasal delivery, however, the nasal fluids are acidic and can have a pH as low as 5.5 (England et al., Clinical Otolaryggology 24, 67-6~, 1999;
Ireson et al., Clinical Science 100, 327-333, 2001).
Thus, the formulation powder is then blended with an appropriate amount of buffer powder such as a phosphate buffer at pH 7.4. Upon delivery and hydration, the buffer agents will be quickly dissolved upon hydration, ensuring the local environment at pH 7.4 and thereby keeping the formulation particles insoluble or insoluble for a longer period of time.
Throughout this application, various publications and patents are referenced.
The disclosures of these publications and patents are hereby incorporated by reference into this application in their entirety, for all purposes, especially for their teachings regarding formulation of pharmaceutical compositions.
While the preferred compositions or formulations and methods have been disclosed, it will be apparent to those skilled in the art that numerous modifications and variations are possible in light of the above teaching. It should also be realized by those skilled in the art that such modifications and variations do not depart from the spirit and scope of the invention as set forth in the appended claims.

Claims (140)

1. A solid pharmaceutical composition for the delivery of a physiologically active agent to an animal comprising:
a. one or more physiologically active agents in an amount effective to induce a physiological response in an animal;
b. one or more polysaccharides comprising subunits having anionic carboxylate or sulfate groups, and c. one or more solid, polysaccharide gel inducing compositions comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal cation;
wherein the pharmaceutical composition is in a solid form that forms a gel when contacted with a tissue or body fluid of an animal.
2. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are selected from the group consisting of a pectic substance, alginate, carrageenan, and gellan.
3. The solid pharmaceutical composition of claim 1 in the form of a pad, a tablet, or a capsule.
4. The solid pharmaceutical composition of claim 1 in the form of a powder.
5. The solid pharmaceutical composition of claim 4 wherein the powder comprises a plurality of microparticles and/or microspheres having a particle size suitable to permit the microparticles or microspheres to pass through a sieve having an opening size of about 250 µM in diameter.
6. The solid pharmaceutical composition of claim 4 wherein the one or more polysaccharides comprise one or more pectins.
7. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are a pectin having a degree of methylation of less than 70%.
8. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are a pectin having a degree of methylation of less than 50%.
9. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are a pectin having a degree of methylation of less than 25%.
10. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are a pectin having a degree of methylation of less than 10%.
11. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are a pectin having an average molecular weight of greater than about 4.0 × 10 5 Daltons.
12. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are a pectin having an average molecular weight of greater than about 1.0 × 10 6 Daltons.
13. The solid pharmaceutical composition of claim 1 wherein the one or more polysaccharides are a pectin having an average molecular weight of greater than about 1.0 × 10 6 Daltons, and a degree of methylation of less than about 10%.
14. The solid pharmaceutical composition of claim 6 wherein the one or more pectins are an aloe pectin.
15. The solid pharmaceutical composition of claim 6 wherein the one or more pectins have a galacturonic acid content of greater than about 80% w/w.
16. The solid pharmaceutical composition of claim 6 wherein the one or more pectins have a rhamnose content of greater than 4% by mole.
17. The solid pharmaceutical composition of claim 1 wherein the tissue or body fluid is normal calf serum.
18. The solid pharmaceutical composition of claim 1 wherein the one or more physiologically active agents are selected from the group consisting of a therapeutic agent, a diagnostic agent, a carbohydrate, a lipid, a peptide, a nucleic acid, a live cell, a dead cell in whole or part, a microorganism in whole or part, a virus in whole or part, a vaccine, an antigen, and a protein.
19. The solid pharmaceutical composition of claim 1 wherein the one or more physiologically active agents comprise a peptide or a protein.
20. The solid pharmaceutical composition of claim 1 wherein the one or more physiologically active agents comprises a one or more antigens.
21. The solid pharmaceutical composition of claim 20 wherein the one or more antigens are independently selected from a peptide, a protein, a live cell in whole or in part, a dead cell in whole or in part, or viruses in whole or in part, inactivated microbes or viruses, live attenuated microbes or viruses, phages, subunit vaccine proteins, subunit vaccine peptides, subunit vaccine carbohydrates, replicons, viral vectors, plasmids.
22. The solid pharmaceutical composition of claim 20 wherein the one or more antigens are independently selected from antigens for influenza.
23. The solid pharmaceutical composition of claim 1 wherein the divalent or multivalent metal cation is calcium, magnesium, copper, manganese, nickel, cobalt, iron, zinc, or aluminum.
24. The solid pharmaceutical composition of claim 1 wherein the divalent or multivalent metal cation is calcium or aluminum.
25. The solid pharmaceutical composition of claim 1 wherein the pharmaceutically acceptable salt is soluble in water to the extent of at least about 1 ×
10 -5 moles per liter.
26. The solid pharmaceutical composition of claim 1 wherein the pharmaceutically acceptable salt will not dissolve in water to form a solution comprising at least 1 ×
-5 moles per liter.
27. The solid pharmaceutical composition of claim 1 wherein the one or more pharmaceutically acceptable salts comprise aluminum hydroxide or calcium phosphate.
28. The solid pharmaceutical composition of claim 1 wherein the polysaccharide gel inducing composition further comprises one or more pharmaceutically acceptable excipients.
29. The solid pharmaceutical composition of claim 28 wherein the one or more pharmaceutically acceptable excipients are selected from the group consisting of mono- or di-saccharides, binders, fillers or bulking agents, lubricants, flavors, and taste masking agents.
30. The solid pharmaceutical composition of claim 1 further comprising one or more pharmaceutically acceptable thickeners.
31. The solid pharmaceutical composition of claim 29 wherein the one or more pharmaceutically acceptable thickeners are selected from the group consisting of polyvinylpyrrolidone, carboxymethylcellulose, hydroxypropylmethylcellulose, collagen, gelatin, dextran, hyaluronic acid.
32. The solid pharmaceutical composition of claim 29 wherein the one or more pharmaceutically acceptable thickeners comprise polyvinylpyrrolidone.
33. The solid pharmaceutical composition of claim 1 wherein the one or more physiologically active agents, and the one or more polysaccharides are present as a solid mixture on the molecular level, and the one or more solid gel inducing compositions are distinct solid phases.
34. The solid composition of claim 33 wherein the mixture on the molecular level is produced by a process of dissolving the one or more physiologically active agents, and the one or more polysaccharides in a liquid carrier, then removing the liquid carrier to produce a solid mixture on the molecular level.
35. The solid pharmaceutical composition of claim 1 wherein the one or more physiologically active agents, the one or more polysaccharides, and the one or more solid gel inducing compositions are present as a physical mixture of separate solid components.
36. The solid pharmaceutical composition of claim 1 wherein the animal is a human.
37. The solid pharmaceutical composition of claim 1 further comprising from about 30.0 to about 99.5% of one or more pharmaceutically acceptable mono- or di-saccharides.
38. The solid pharmaceutical composition of claim 1 wherein the mono- or di-saccharide is selected from ribose, arabinose, xylose, fructose, glucose, rhamnose, glucosamine, galactosamine, gluconic acid, glucurionic acid, galactose, mannose, lactose, sucrose, maltose, xylitol, mannitol, and trehalose, or a mixture therof.
39. The solid pharmaceutical composition of claim 1 wherein the mono- or di-saccharide is lactose.
40. A method for the sustained release of a physiologically active agent to an animal comprising administering the solid pharmaceutical composition of claim 1 to a tissue or body fluid of an animal, to form a gel in contact with the tissue or body fluids of the animal.
41. A method for the sustained release of a physiologically active agent to an animal comprising administering a liquid suspension of the solid pharmaceutical composition of claim 1, or the components thereof, to a tissue or body fluid of an animal to form a gel in contact with the tissue or body fluids of the animal.
42. The method of claim 40 wherein the tissues or body.fluid of the animal are selected from the group consisting of mucosal surfaces, blood, serum, tear fluid, lung fluid, interstitial fluid, or nasal secretions.
43. The method of claim 40 wherein the animal is a human.
44. The method of claim 40 wherein the tissues or body fluids of the animal are nasal mucosal surfaces or nasal secretions.
45. The gel formed by the process of claim 40.
46. A method for the administration of a physiologically active agent to an animal comprising administering to a tissue or body fluid of an animal, in any order or combination, the following components, a. one or more physiologically active agents in an amount effective to induce a physiological response in an animal;
b. one or more polysaccharides comprising subunits having anionic carboxylate or sulfate groups, and one or more solid gel inducing compositions comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal ration;
to form a gel in contact with the tissue or body fluids of the animal.
47. The method of claim 46 wherein components a, b, and c are administered as components of a powder composition.
48. The method of claim 46 wherein components a and b are administered as separate or mixed powders.
49. The method of claim 46 wherein components a and b are administered as a mixture of one or more powders comprising component a and one or more powders comprising component b.
50. The method of claim 46 wherein components a and b are administered as components of a solid composition prepared by dissolving one or more physiologically active agents and one or more ionic polysaccharides in a liquid carrier, and then removing sufficient liquid carrier to form the solid mixed composition.
51. The method of claim 50 wherein the solid mixed composition is in the form of a powder.
52. The method of claim 46 wherein components a and b are administered as a solution in a liquid carrier.
53. The method of claim 46 wherein the one or more polysaccharides comprise a low methoxyl pectin.
54. The method of claim 46 wherein the one or more physiologically active agents comprise a peptide, a protein, or a vaccine.
55. The method of claim 46 wherein the tissue body fluid is a nasal mucosal surface or a nasal secretion.
56. The method of claim 46 wherein the animal is a human.
57. A composition for the controlled release of a physiologically active agent to an animal comprising:
a. one or more physiologically active agents in an amount effective to induce a physiological response in an animal; and b. one or more pectic substances having a degree of methylation less than about 30% and an average molecular weight of greater than about 1 × 10 5 Daltons, wherein the composition is a solid capable of forming a gel when contacted with a tissue or body fluid of an animal.
58. The composition of claim 57 wherein the composition is in the form of a pad, a tablet, a capsule, or a powder.
59. The composition of claim 57 wherein the pectic substance has a degree of methylation less than about 15%.
60. The composition of claim 57 wherein the pectic substance has an average molecular weight of greater than about 5.0 × 10 5 Daltons.
61. The composition of claim 57 wherein the pectic substance has a molecular weight greater than 1 × 10 6 Daltons and a degree of methylation of less than 10%.
62. The composition of claim 57 wherein the pectic substance has a galacturonic acid content of greater than about 90% w/w.
63. The composition of claim 57 wherein the pectic substance comprises 3-methoxy-rhamnose.
64. The composition of claim 57 wherein the pectic substance has a rhamnose content of greater than 4% by mole.
65. The composition of claim 57 wherein the pectic substance is an Aloe pectin.
66. The composition of claim 57 wherein the composition comprises about 20%
water by weight, or less.
67. The composition of claim 57 comprising microparticles and/or microspheres that have an particle size suitable to permit the microparticles or microspheres to pass through a sieve having an opening size of about 250 µM in diameter.
68. The composition of claim 57 wherein the composition is in the form of a powder.
69. The composition of claim 68 wherein the powder comprises at least about 80% by weight of microparticles and/or microspheres having particle sizes suitable to permit the microparticles and/or microspheres to pass through a sieve having an opening size of 100 µM in diameter but not pass through a sieve having an opening size of about 0.1 µM in diameter.
70. The composition of claim 68 consisting essentially of microparticles and/or microspheres, wherein the microparticles and/or microspheres having particle sizes that permits them to pass through a sieve having an opening size of about 50 µM in diameter but not pass through a sieve having an opening size of 10 µM in diameter.
71. The composition of claim 57 wherein the solid composition comprises microspheres, wherein less than 90% of the microspheres have a diameter between 0.1 and 10 µM.
72. The composition of claim 57 further comprising one or more pharmaceutically acceptable thickeners.
73. The composition of claim 72 wherein the one or more thickeners are selected from the group consisting of polyvinylpyrrolidone, carboxymethylcellulose, hydroxypropylmethylcellulose, collagen, gelatin, dextran, hyaluronic acid, or alginate.
74. The composition of claim 72 wherein the one or more thickeners comprise polyvinylpyrrolidone.
75. The composition of claim 72 wherein the thickener comprises from about 01.
to about 90% of the composition by weight.
76. The composition of claim 57 further comprising from about 30.0 to about 99.5% of one or more pharmaceutically acceptable mono- or di-saccharides.
77. The composition of claim 76 wherein the mono- or di-saccharide is selected from ribose, arabinose, xylose, fructose, glucose, rhamnose, glucosamine, galatosamine, gluconic acid, glucurionic acid, galactose, mannose, lactose, sucrose, maltose, xylitol, mannitol, and trehalose, or a mixture therof.
78. The composition of claim 76 wherein the mono- or di-saccharide is lactose.
79. The composition of claim 57 wherein the one or more physiologically active agents comprise one or more pharmacologically active substances selected from the group consisting of a therapeutic agent, a diagnostic agent, a carbohydrate, a lipid, a peptide, a nucleic acid, a live cell, a dead cell in whole or part, a microorganism in whole or part, a virus in whole or part, a vaccine, an antigen, and a protein.
80. The composition of claim 57 wherein the one or more physiologically active agents comprise a therapeutic agent in an amount effective to treat a disease or disease condition in an animal.
81. The composition of claim 57 wherein the one or more physiologically active agents comprise a peptide or a protein.
82. The composition of claim 57 wherein the one or more physiologically active agents comprises one or more antigens.
83. The composition of claim 82 wherein the one or more antigens are independently selected from a peptide, a protein, a live cell in whole or in part, a dead cell in whole or in part, or viruses in whole or in part, inactivated microbes or viruses, live attenuated microbes or viruses, phages, subunit vaccine proteins, subunit vaccine peptides, subunit vaccine carbohydrates, replicons, viral vectors, plasmids.
84. The composition of claim 82 wherein the one or more antigens are independently selected from antigens for influenza.
85. The composition of claim 82 wherein the one or more antigens induce an active immune response in the animal when the composition is administered to the nasal mucosa of the animal.
86. The composition of claim 82 wherein after administration of the composition to an animal the immune response of the animal increases by more than about a factor of about 10%, as measured by the IgA levels in the lung washings of an animal as compared to the IgA levels obtained in a control experiment that administers a control composition that does not comprise the pectic substance.
87. The composition of claim 57 wherein, based on the weight of the composition, the physiologically active agent comprises from about 0.01 % to about 90 % of the composition.
88. The composition of claim 57 wherein the pectic substance comprises from about 0.0001 % to about 99% by weight of the composition.
89. The composition of claim 57 wherein the pectic substance comprises from about 0.001% to about 50% by weight of the composition.
90. The composition of claim 57 wherein the pectic substance comprises from about 0.005% to about 20% by weight of the composition.
91. The composition of claim 57 wherein the pectic substance comprises from about 0.01 to about 10% by weight of the composition.
92. The composition of claim 57 further comprising a solid polysaccharide gel inducing agent.
93. The composition of claim 92 wherein the solid polysaccharide gel inducing agent comprises one or more pharmaceutically acceptable salts of a divalent or multivalent metal cation.
94. The composition of claim 93 wherein the divalent or multivalent metal ration is calcium, magnesium, copper, manganese, nickel, cobalt, iron, zinc, or aluminum.
95. The composition of claim 93 wherein the pharmaceutically acceptable salt can dissolve in water to form a solution comprising at least about 1 × 10 -5 moles per liter of the salt.
96. The composition of claim 93 wherein the pharmaceutically acceptable salt is a calcium salt.
97. The composition of claim 93 wherein the pharmaceutically acceptable salt is a calcium halide salt.
98. The composition of claim 93 wherein the pharmaceutically acceptable salt is sufficiently insoluble in water so as to not be capable of dissolving in water to form a solution comprising at least 1 × 10 -5 moles per liter of the salt.
99. The composition of claim 93 wherein the one or more pharmaceutically acceptable salts comprise aluminum hydroxide or calcium phosphate.
100. The composition of claim 93 wherein the one or more pharmaceutically acceptable salts comprise from about 0.1 % to about 80% (w/w) of the composition.
101. The composition of claim 93 wherein the one or more divalent or multivalent metal ration salts react with the pectic substance to crosslink the carboxylate groups of the pectic substance so as to form a gel comprising the metal ration.
102. The composition of claim 93 wherein the one or more divalent or multivalent metal ration salts induce the composition to form a gel when the composition is contacted with the tissue or body fluid of an animal.
103. The composition of claim 57 wherein the tissues or body fluids of the animal are selected from the group consisting of mucosal surfaces, blood, serum, tear fluid, lung fluid, interstitial fluid, or nasal secretions.
104. The composition of claim 57 wherein the tissues or body fluids of the animal are nasal secretions.
105. A method for the sustained release of a physiologically active agent to an animal comprising contacting the composition of claim 57 with a tissue or body fluid of the animal.
106. The method of claim 105 wherein the composition forms a gel comprising the physiologically active agent in contact with the tissues or body fluids on or after administration to the tissues or body fluids.
107. The method of claim 105 wherein the gel provides a sustained time release of the physiologically active agent to the tissues or body fluids.
108. The method of claim 105 wherein the tissues or body fluids of the animal are nasal mucosal surfaces and the one or more physiologically active agents are antigens for influenza
109. The gel formed by the process of claim 105.
110. A method for the sustained release of a physiologically active agent to an animal comprising administering a liquid suspension of the solid pharmaceutical composition of claim 57, or the components thereof, to a tissue or body fluid of an animal to form a gel in contact with the tissue or body fluids of the animal.
111. A method for the sustained release of a physiologically active agent to an animal comprising contacting the composition of claim 57 with an eye, a mucosal surface, or a wound of the animal.
112. A method for the sustained release of a physiologically active agent to an animal comprising contacting the composition of claim 57 with one or more bodily fluids of the animal selected from the group consisting of blood, serum, tear fluid, lung fluids, interstitial fluid, or nasal secretions.
113. A method for the sustained release of a physiologically active agent to an animal comprising administering the composition of claim 57 to the nasal mucosal surfaces and secretions of a human.
114. A method of making the composition of claim 57 comprising mixing in any sequence the physiologically active agent, the pectic substance, and one or more optional components and processing the mixture to form the solid composition.
115. The method of claim 114 wherein the one or more optional components comprise a thickener.
116. The method of claim 114 wherein the one or more optional components comprise a polyvinyl pyrrolidone.
117. The method of claim 114 wherein the physiologically active agent and the pectic substance are dissolved in a liquid carrier, then the volatile components of the liquid carrier are removed to form the solid composition.
118. The method of claim 114 wherein the physiologically active agent, the pectic substance, and any optional components are solids and are mixed and processed as solids.
119. The method of claim 114 wherein the optional component comprises a solid gel inducing agent comprising one or more pharmaceutically acceptable salts of a divalent or multivalent metal cation.
120. A method for-vaccinating an animal, comprising the steps of:

a. providing one or more powder compositions comprising powder particles that can pass through a sieve having an opening size of about 250 µM in diameter, and that comprise i) a pectic,substance having a degree of methylation less than about 30% and an average molecular weight of greater than 1 x 10 5 Daltons, in an amount effective to form a gel when the composition is contacted with the mucosal surfaces of an animal;
ii) one or more antigens selected from the group consisting of a peptide, a protein, a nucleic acid, a live cell, a dead cell or a portion thereof, or a virus, in an amount that is capable of inducing an active immune response in the animal; and b. administering the powder to the nasal tissues and/or nasal fluids of the animal to form a gel in contact with the tissues or body fluids, and c. inducing an active immune response to one or more of the antigens in the animal.
121. The method of claim 120 wherein the pectic substance is a sodium, potassium, or NH4+ salt of a pectin having an average molecular weight of greater than about 1.0 × 10 6 Daltons.
122. The solid pharmaceutical composition of claim 1 wherein the one or more anionic polysaccharides are a sodium, potassium, or NH4+ salt of a pectin having an average molecular weight of greater than about 1.0 × 10 6 Daltons.
123. A vaccine composition for nasal administration to an animal comprising powder particles that comprise a nano-dispersion of:
a. one or more antigens in an amount effective to induce an immune response response in an animal, and b. one or more pectins or a monovalent cation salt thereof having a degree of methylation less than about 30% and an average molecular weight of greater than about 1 × 10 5 Daltons;
wherein the powder particles can pass through a sieve having an opening size of about 250 µM in diameter.
124. The vaccine composition of claim 123 wherein the powder particles are a substantially homogeneous solid solution of the one or more antigens and the one or more pectins or a monovalent cation salt thereof.
125. The vaccine composition of claim 123 wherein the pectins are present as a water soluble monovalent cation salt that becomes cross-linked with calcium ions to form a gel when contacted with the nasal mucosa of an animal.
126. The vaccine composition of claim 123 wherein at least about 90% of the powder particles will not pass through a sieve having an opening size of about 11 µM in diameter.
127. The vaccine composition of claim 123 wherein at least about 90% of the powder particles are microspheres or microparticles having a particle size between about 12 µM and about 60 µM.
128. The vaccine composition of claim 123 wherein the one or more antigens are independently selected from the group consisting of a peptide, a protein, a nucleic acid, a live cell, a dead cell or a portion thereof, or a virus in whole or in part.
129. The vaccine composition of claim 123 wherein the one or more antigen comprise at least one antigen for influenza.
130. The vaccine composition of claim 123 wherein the one or more antigen comprise
131. The vaccine composition of claim 123 wherein the one or more pectins are independently selected from a sodium, potassium, or NH4+ salt of a pectin having an average molecular weight of greater than about 1.0 × 10 6 Daltons, and a degree of methylation of less than about 10%.
132. The vaccine composition of claim 123 wherein the pectic substance comprises from about 0.01 to about 10% by weight of the composition.
133. The composition of claim 123 further comprising one or more pharmaceutically acceptable thickeners.
134. The composition of claim 123 wherein the one or more thickeners are selected from the group consisting of polyvinylpyrrolidone, carboxymethylcellulose, hydroxypropylinethylcellulose, collagen, gelatin, dextran, hyaluronic acid, or alginate.
135. The vaccine composition of claim 123 wherein the one or more thickeners comprise polyvinylpyrrolidone.
136. The vaccine composition of claim 123 further comprising one or more pharmaceutically acceptable mono- or di-saccharides.
137. The vaccine composition of claim 136 wherein the one or more pharmaceutically acceptable mono- or di-saccharides are independently selected from the group consisting of ribose, arabinose, xylose, fructose, glucose, rhamnose, glucosamine, galactosamine, gluconic acid, glucuronic acid, galactose, mannose, lactose, sucrose, maltose, xylitol, mannitol, and trehalose.
138. The vaccine composition of claim 136 wherein the one or more pharmaceutically acceptable mono- or di-saccharides is lactose.
139. The vaccine composition of claim 136 wherein one or more pharmaceutically acceptable mono- or di-saccharides, is present in an amount from about 10.0 to about 99.9 % by weight.
140. The vaccine composition of claim 136 wherein the mono- or di-saccharides are present in an amount from about 50.0 to about 99.5 % by weight.
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