WO1998017310A2 - Polyanionic polymers as adjuvants for mucosal immunization - Google Patents

Polyanionic polymers as adjuvants for mucosal immunization Download PDF

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Publication number
WO1998017310A2
WO1998017310A2 PCT/EP1997/005861 EP9705861W WO9817310A2 WO 1998017310 A2 WO1998017310 A2 WO 1998017310A2 EP 9705861 W EP9705861 W EP 9705861W WO 9817310 A2 WO9817310 A2 WO 9817310A2
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acid
adjuvant
specimens
repeating units
constitutional repeating
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WO1998017310A3 (en
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Luuk Hilgers
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Dimminaco AG
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Dimminaco AG
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Priority to EP97950021A priority Critical patent/EP0934077B1/en
Priority to BR9712436-2A priority patent/BR9712436A/pt
Priority to DE69737658T priority patent/DE69737658T2/de
Priority to JP51897598A priority patent/JP4344014B2/ja
Priority to US09/297,214 priority patent/US6610310B2/en
Priority to CA002269780A priority patent/CA2269780C/en
Priority to AU53133/98A priority patent/AU717349B2/en
Publication of WO1998017310A2 publication Critical patent/WO1998017310A2/en
Publication of WO1998017310A3 publication Critical patent/WO1998017310A3/en
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    • 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
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • A61P37/02Immunomodulators
    • 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
    • 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
    • A61K2039/55555Liposomes; Vesicles, e.g. nanoparticles; Spheres, e.g. nanospheres; Polymers

Definitions

  • This invention relates to novel vaccine compositions, processes for the preparation thereof and methods for the use thereof for the mucosal (nonparenteral) immunization of warm blooded animals.
  • systemic immunity which is provided through parenteral vaccination
  • mucosal (or local) immunity which is provided through nonparenteral vaccination.
  • vaccine development has focused on the induction of systemic immunity, including humoral (specific antibodies of IgM or IgG class) and cellular immune responses (activated T lymphocytes, activated macrophages, or others) through the use of parenteral vaccines.
  • parenteral vaccines are administered through, inter alia, intramuscular or subcutaneous routes.
  • parenteral vaccines and parenteral vaccination to provide systemic immunity has other disadvantages, such as the need to breach the integrity of the skin of the organism being immunized therewith, difficulty of administration (needing, for example, trained personnel to administer such vaccines), the high grade of purity needed for such vaccines, a lack of establishment of immunity at the site of natural infection, nonprevention of infection and less than complete protection of the organism against both clinical and nonclinical symptoms of the infection as well as against the infection itself.
  • parenteral vaccines can present problems where the effective immunization of immunocompromised hosts (i.e., young animals with maternal antibodies) is desired.
  • Mucosal (or local) immunity results from the local formation and secretion of antibodies of the IgA class. These antibodies form di ers which can be secreted into the lumen of respiratory, gastro-intestinal or genital organ.
  • Specific IgA antibodies in the lumen are capable of reducing infection by impairing or blocking penetration of the host tissue by the pathogen.
  • Mechanisms known to underly the inhibition of host tissue penetration include: the neutralization of viruses; the complexation with enzymes, toxins or other components produced by the pathogens (resulting in either neutralization of the activity of these components and/or blocking the adsorption of these components); the inhibition of adherence of the pathogens to mucosal surfaces; the suppression of antibody mediated inflammatory reactions at the mucosal surfaces; and synergism with innate antibacterial factors at the musocal surface.
  • Mucosal (nonparenteral) vaccines and mucosal vaccination have other additional advantages over parenteral vaccines and parenteral vaccination.
  • mucosal (nonparenteral) vaccines mucosal vaccination and the immunity provided thereby is preferable over the use of parenteral vaccines, parenteral vaccination and the immunity provided thereby.
  • mucosal immunity Depending on various factors, natural or artificial infection with live microorganisms can induce considerable levels of mucosal immunity. These factors include: the route of infection, the nature of the microorganism, the infectious dose involved and the immune status of the host. However, the administration of killed (non-replicating) antigens gives little or no mucosal immunity. To alleviate this problem, adjuvants are used to increase the immune responses to killed antigens.
  • adjuvants for parenteral vaccines include the toxin of Vibrio cholera (Cholera toxin) or products thereof (Cholera toxin subunit B -- CTB), the heat-labile toxin of I coH or products thereof, bacterial toxins or products thereof which are conjugated to antigens, microparticles or microcapsules of different natural or synthetic polymers having antigens incorporated therein, liposomes antigen incorporated therein or liposomes mixed with antigen, lectins, i munostimulating complexes, muramyldipeptide and derivatives thereof, and cationic polymers (see, "Novelo cholera toxin) or products thereof (Cholera toxin subunit B -- CTB), the heat-labile toxin of I coH or products thereof, bacterial toxins or products thereof which are conjugated to antigens, microparticles or microcapsules of different natural or synthetic polymers having antigens incorporated therein, liposomes antigen incorporated
  • the present invention relates to mucosal adjuvants for incorporation into mucosal vaccines and to mucosal vaccines incorporating such adjuvants therein useful for the induction or enhancement of mucosal and/or systemic immune responses to antigens.
  • a mucosal adjuvant for vaccines comprising a water-soluble polyanionic polymer having anionic constitutional repeating units.
  • the mucosal adjuvants of the present invention are water-soluble polyanionic polymers having anionic constitutional repeating units which may be the same or different repeating units, or polyanionic polymers having anionic constitutional repeating units (same or different) and hydrophobic constitutional repeating units.
  • the polyanionic polymers may be linear (polymers having chemical units which are connected covalently to one or two other constitutional units), or branched (polymers having chemical units which are connected covalently to one or two other constitutional units and occasionally to three or more constitutional units) or reticular (polymers having chemical units which are connected covalently to one or two or three or more other constitutional units) in structure.
  • water soluble when referring to the polyanionic polymers of the present invention refers to polymers which are soluble in an aqueous phase at a concentration of at least 0.01 gram per liter.
  • polymer refers to compounds having at least three identical chemical constitutional repeating units, which said units are covalently connected with one another.
  • substitutional repeating unit refers to the minimal structural unit of a polymer.
  • homopolymer refers to polymers consisting of one type of constitutional repeating unit.
  • heteropolymer refers to polymers having two or more different constitutional repeating units.
  • polyanionic polymer refers to polymers which, when dissolved in an aqueous medium, are negatively charged due to the presence of anionic constitutional repeating units (e.g., units containing sulphate, sulphonate, carboxylate, phosphate and borate groups).
  • anionic constitutional repeating unit refers to constitutional repeating units of polymers which are negatively-charged in aqueous medium at physiological conditions.
  • hydrophobic constitutional repeating unit refers to constitutional repeating units of polymers which are characterised in that the corresponding monomer is less soluble in an aqueous phase than in an organic solvent [that is to say, the quantity, in weight (in grams), of the monomer that can be dissolved in a fixed volume, in ml, of an aqueous phase is less than the quantity, in weight (in grams), of the monomer that can be dissolved in the same fixed volume, in ml, of the organic solvent].
  • the anionic constitutional repeating units of the polyanionic polymer are preferably obtained from acrylic acid, methacrylic acid, maleic acid, fumaric acid, ethylsulphonic acid, vinylsulphuric acid, vinylsulphonic acid, styrenesulphonic acid (vinylbenzenesulphonic acid), vinylphenylsulphuric acid, 2-methacryloyloxyethane sulphonic acid, 3-methacryloyloxy- 2-hydroxypropanesulphonic acid, 3-methacryl amido-3-methylbutanoic acid, acrylamidomethylpropanesulfonic acid, vinylphosphoric acid, 4-vinylbenzoic acid, 3- vinyl oxypropane-1 -sulphonic acid, N-vinylsuccinimidic acid, and salts of the foregoing.
  • the anionic constitutional repeating units of the polyanionic polymer are obtained from acrylic acid, methacrylic acid, maleic acid, fumaric acid, ethylsulphonic acid, vinylsulphuric acid, vinylsulphonic acid, styrenesulphonic acid, and acrylamidomethylpropanesulfonic acid, and salts of the foregoing.
  • the anionic constitutional repeating units of the polyanionic polymer are obtained from acrylic acid, methacrylic acid, maleic acid and fumaric acid, vinylsulphonic acid, styrenesulphonic acid, and acrylamidomethylpropanesulfonic acid, and salts of the foregoing.
  • the mucosal adjuvants of the present invention include polyanionic homopolymers which are preferably obtained from polyacrylic acid, polymethacrylic acid, polymaleic acid, polyfumaric acid, polyethylsulphonic acid, polyvinylsulphuric acid, polyvinylsulphonic acid, polystyrenesulphonic acid (polyvinylbenzenesulphonic acid), polyvinylphenylsulphuric acid, poly 2-methacryloyloxyethanesulphonic acid, poly 3-methacryloyloxy-2-hydroxypropanesulphonic acid, poly 3-methacryl amido-3- methylbutanoic acid, polyacrylamidomethylpropanesulfonic acid, polyvinylphosphoric acid, poly 4-vinylbenzoic acid, poly 3-vinyl oxypropane-1 -sulphonic acid, poly N- vinylsuccinimidic acid, and salts of the foregoing. More preferably, the polyanionic homopolymers are obtained from
  • the mucosal adjuvants of the present invention further include polyanionic heteropolymers having two different (distinct) anionic groups, such as, but not limited to, a carboxylic group and a sulfate or sulfonic group, for example, acrylic acid and any of vinylsulphonic acid, styrenesulphonic acid and acrylamidomethylpropanesulfonic acid.
  • polyanionic heteropolymers having two different (distinct) anionic groups, such as, but not limited to, a carboxylic group and a sulfate or sulfonic group, for example, acrylic acid and any of vinylsulphonic acid, styrenesulphonic acid and acrylamidomethylpropanesulfonic acid.
  • the polyanionic polymer of the mucosal adjuvants of the present invention further has hydrophobic constitutional repeating units.
  • hydrophobic constitutional repeating units of the polyanionic polymer of the mucosal adjuvants of the present invention are obtained from alkylesters, cycloalkylesters, hydroxyalkylesters, ethers, glycols and aromatic groups and salts of the foregoing.
  • the alkylesters are selected from the group consisting of methyl-, ethyl-, propyl-, isopropyl, n-butyl-, isobutyl, sec.butyl-, t-butyl, n-hexyl-, n-octyl-, isooctyl-, 2-ethylhexyl-, n-decyl-, tetradecyl-, vinyl-, allyl- and oleylester.
  • the cycloalkylesters are selected from the group consisting of cyclohexyl-, 1-methylcyclohexyl-, 3- vinylcyclohexyl- and 3,3,5-trimethylcyclohexylester.
  • the hydroxyalkylesters are selected from the group consisting of 2-hydroxyethyl-, 2- hydroxypropyl-, 3-hydroxypropyl-, 3,4-dihydroxybutyl-, 2-hydroxypenyl- and 2- hydroxyhexylester.
  • the ethers are selected from the from the group consisting of methoxy methyl, ethoxyethyl, allyloxymethyl, 2-ethoxyethoxymethyl, benzyloxymethyl, cyclohexyloxymethyl, 1- ethoxyethyl, 2-ethoxyethyl, 2-butoxyethyl, methoxymethoxyethyl, methoxyethoxyethyl, 1-butoxy propyl, 1-ethoxybutyl, tetrahydrofurfuryl, furfuryl.
  • the glycols are selected from the group consisting of ethylene glycol, 1,2-propanediol, 1,3-propanediol, 1 ,3-butanediol, 1,4-butanediol, 2,5-dimethyl-l,6-hexanediol, 1,10-decanediol, diethyleneglycol and triethyleneglycol.
  • the aromatic groups are selected from the group consisting of benzyl, phenyl and nonylphenyl.
  • the hydrophobic constitutional repeating units of the polyanionic polymer are obtained from the group consisting of methyl-, ethyl, propyl, butyl-, pentyl-, hexyl-, heptyl-, octyl-, nonyl-, and decyl- esters of acrylic acid, methacrylic acid, maleic acid, fumaric acid, ethylsulphonic acid, vinylsulphuric acid and styrenesulphonic acid and salts of the foregoing.
  • the hydrophobic constitutional repeating units of the polyanionic polymer are obtained from the group consisting of butyl-, pentyl-, hexyl-, heptyl- and octyl- esters of acrylic acid, methacrylic acid, maleic acid and fumaric acid and salts of the foregoing.
  • Particulaly preferred polyanionic polymers according to the present invention are polyacrylic acid, butyl-polyacrylic acid, poly(acrylate-co-acrylamidomethylpropane sulfonic acid) copolymer (p(A-c-AMPS)), poly(acrylate-co-vinylsulfonate) copolymer (p(A-c-VS)), poly(acrylate-co-vinylbenzenesulfonate) copolymer (p(A-c-VBS)),
  • the molar ratio of hydrophobic constitutional repeating units and anionic constitutional repeating units of the polyanionic polymers of the present invention is between 0 hydrophobic constitutional repeating units per 1 anionic constitutional repeating unit and 0.6 hydrophobic constitutional repeating units per 1 anionic constitutional repeating unit.
  • the molar ratio of hydrophobic constitutional repeating units and anionic constitutional repeating units is between 0.02 and 0.60 hydrophobic constitutional repeating unit per 1 anionic constitutional repeating unit (which is from 2 to 60 hydrophobic constitutional repeating units per every 100 anionic constitutional repeating units).
  • the molar ratio of hydrophobic constitutional repeating units and anionic constitutional repeating units is between 0.05 and 0.30 hydrophobic constitutional repeating units per 1 anionic constitutional repeating unit (which is from 5 to 30 hydrophobic constitutional repeating units per every 100 anionic constitutional repeating units).
  • a mucosal (nonparenteral) vaccine having the mucosal adjuvant (including the polyanionic polymer thereof) of the present invention, wherein the vaccine is administered nonparenterally for the induction of either systemic or mucosal immunity against antigens.
  • the mucosal vaccine may further be comprised of an antigen or a drug molecule and/or a pharmaceutical ly-acceptable medium (carrier).
  • a pharmaceutical ly-acceptable medium carrier
  • disclosed herein is the use of the water-soluble polyanionic polymers of the present invention for the manufacture or production of mucosal adjuvants for the inducement or enhancement of mucosal or systemic immune responses.
  • the nonparenteral adjuvant comprised of a polyanionic polymer disclosed herein is administered nonparenterally for the enhancement of either systemic or mucosal immunity against antigens.
  • the antigen includes live or inactivated viruses, bacteria, fungi, parasites and other microorganisms as well as components or products derived from these microorganisms, products obtained by chemical synthesis capable of eliciting protective immunity, and products obtained by any other means capable of eliciting protective immunity.
  • Preferred antigens are thise capable of eliciting protective immunity to diseases which are infections of the respiratory tract.
  • diseases are Newcastle disease virus, infectious bronchitis virus, influenza virus, rhinovirus, parainfluenza virus, adenovirus, Actinobaccilus pleuropneumoniae, Pasteurella multocida, Streptococcus pneumonia, Streptococcus pyogenes, and infections of the gastro-intestinal tract with for example, rotavirus, parvovirus, caronavirus, E. coli, Salmonella, Shigella, Yersinia, Campylobactor, Clostridium, Vibrio and Giardia, Entamoeba, and Cryptosporidium.
  • polyanionic polymers which may be utilized as the adjuvants of the present invention may be obtained either by the isolation and purification of natural forms thereof or by the synthesis thereof.
  • the use of the adjuvants of the present invention in vaccines for mucosal vaccination offers various important advantages over those known mucosal adjuvants (and over parenteral vaccines) in that the adjuvants of the present invention are inexpensive, nonimmunogenic, water-soluble, chemically stable, easy to produce and easy to incorporate in the vaccines in which they are intended to be used. Furthermore, these adjuvants are more effective in inducing the desired mucosal immune responses than other adjuvants of which we are aware. Finally, various of the adjuvants described herein are already widely applied in food and pharmaceutical preparations, thereby increasing their acceptability.
  • the polyanionic polymers of the present invention are useful for the induction and or enhancement of mucosal immune responses to antigens when they are administered either in conjunction with the antigen or separately from the antigen via nonparenteral routes.
  • the mucosal vaccines having the adjuvants of the present invention are effective for the induction of mucosal immunity, and include both an antigen and an adjuvant, wherein the adjuvant is a water-soluble polyanionic polymer.
  • the adjuvants of the present invention are solids (for example, are in the form of a powder). If desired, they may be used as such, being applied directly to the surface where an immune response is desired. In such case, being water-soluble, they are solubilized by the mucosal surfaces natural liquids.
  • the mucosal adjuvants of the present invention may be incorporated into an aqueous solution by being dissolved or incorportade into a liquid medium.
  • the mucosal adjuvants of the present invention may further be incorporated into a vaccine having a liquid medium (such as a pharamaceutically-acceptable carrier).
  • a liquid medium such as a pharamaceutically-acceptable carrier.
  • solubilized as, for example, a powder
  • a solution such as an aqueous solution
  • an antigen and/or a drug molecule
  • Another alternative method of achieving this may be by first dissolving the solid adjuvant in an aqueous phase which may then be either mixed with an aqueous solution of the antigen (and/or drug molecule) or which may then have a lyophilized antigen (and/or drug molecule) solubilized in the solution containing the adjuvant.
  • the vaccines of the present invention are formulated so as to have between 0.01 and 40 mg of the polyanionic polymer (mucosal adjuvant) per ml vaccine.
  • the vaccines of the present invention are formulated so as to have between 0.02 and 20 mg of the polyanionic polymer (mucosal adjuvant) per ml vaccine.
  • the vaccines of the present invention are formulated so as to have between 0.25 and 5 mg of the polyanionic polymer (mucosal adjuvant) per ml vaccine.
  • the vaccines of the present invention may be applied to mucosal surfaces of animals or humans by nonparenteral routes such as intranasal, oral, oro-nasal, intratracheal and intracloacal. Such application may be made by, for example, the use of liquid aerosols, drinking-water, food, etc.
  • parenteral immunization means the administration of a vaccine via the skin by use of a needle or another device using, inter alia, one of the following routes: intracutaneous, subcutaneous, intraperitoneal, intramuscular and/or intradermal.
  • nonparenteral immunization and “mucosal immunization” refer to the administration of a vaccine to a mucosal surface by, inter alia, one of the following routes: intranasal, oro-nasal, intratracheal, intragastric, intra-testinal, oral, rectal, intracloacal and/or intravaginal.
  • systemic immunity refers to antigen-specific host defense mediated by serum antibodies of IgM or IgG class or by activated T lymphocytes.
  • macosal immunity refers to antigen-specific host defense mediated by antibodies of IgA class present in the host or secreted into the lumen of different organs.
  • macosal vaccine refers to vaccines which are administered via a nonparenteral route to increase mucosal or systemic immune response to an antigen.
  • macosal adjuvant refers to adjuvants which are administered via a nonparenteral route to increase mucosal or systemic immune response to an antigen.
  • grafted polymer refers to polymers which are obtained by the addition of chemical groups with a significant effect on chemical, physicochemical or biological properties of the polymer.
  • copolymer refers to polymers which are obtained by the polymerisation of two or more distinct monomers in conjunction with one another with significant distinct chemical, physiochemical or biological properties as compared to polymers obtained from either monomer.
  • liquid medium refers to mediums of liquid including, but not limited to: aqueous solutions, physiological aqueous solutions, emulsions of the type oil-in-water and suspensions of insoluble salts in an aqueous solution
  • the preferred liquid mediums are aqueous solutions with physiological aqueous solutions being most preferred, although one of the advantages of the present invention is that the vaccine formulation inco ⁇ orating the mucosal adjuvants disclosed herein need not be physiologic.
  • Example 1
  • the reaction mixture was subsequently dialysed against 1 M NaCl and 0.15 M NaCl using a dialysis membrane with a cut-off of 10 kD (Spectra/por) and then dialysed for at least seven days against distilled water to obtain the polymer.
  • the product was then lyophilized to remove the water therefrom and stored as a dry powder at room temperature.
  • Respective one gram samples of polyacrylic acid-907 (PAA-907) (CARBOPOL-907 by BFGoodrich, Cleveland, Ohio, USA) were esterified according to the method described by Cohen (J. Polymer Sci. 14, 7-22, 1976) by being solubilized in respective 50 ml samples of pure alkanol (octanol, butanol and methanol, respective) and the solutions were heated to 135°C. Fifty ⁇ l of 18 M H2SO were added to each of the solutions and the mixtures were maintained at 135°C for 10 to 30 minutes. The reactions were then terminated by adding 50 ml of cold distilled water to each reaction mixture and by cooling the reaction mixtures to room temperature. The pH of each reaction mixture was then adjusted to 6 with a 1M NaOH solution and the solvents were removed therefrom by heating the mixtures to 80°C at low pressure (10" ⁇ bar).
  • the products obtained were then solubilized in distilled water, dialysed for at least seven days using a membrane with a cut-off of 10 kD (Spectra/por) against distilled water and lyophilized to remove the water therefrom.
  • the compounds obtained in this manner were (grafted polymers) octyl-PAA, butyl-PAA and methyl-PAA. These grafted polymers were analysed by NMR (proton NMR with chemical shift calculated from TMS (0 ppm standard) in a device of 500 megacycles (BRUCKER AMX500) using
  • esterification grade (mean number of alkyl groups per total number of carboxyl groups of the native molecule) thereof.
  • the results ofthis NMR revealed esterification grades of 16 % for octyl-PAA, 16 % for butyl-PAA and 15 % for methyl-PAA.
  • PAA-907 (CARBOPOL-907 from BFGoodrich, Ohio, USA) per liter of anhydrous dimethylformamide was prepared. Fifty ml ofthis solution was then mixed with 10 ml of anhydrous pyridine to form a PAA-907 solution.
  • a solution of CH3COCI at a concentration of 71.2 ml per liter of anhydrous dimethylformamide was prepared.
  • 7.5 ml ofthis CH3COCI solution was added to the PAA-907 solution (molar ratio of 0.3 CH3COCI per COOH of PAA-907) and the reaction mixture was incubated first for 6 hours at 60°C and then for 18 hours at room temperature, thereby forming an anhydride between the COOH groups of the PAA-907 and the CH3COCI.
  • the polymer was analysed by NMR (proton NMR with chemical shift calculated from TMS (0 ppm standard) in a device of 500 megacycles (BRUCKER AMX500) using DMSO as solvent at 25°C) which revealed butyl acrylate monomers and acrylate monomers at a molar ratio of 16 butyl acrylate monomers per 84 acrylate monomers.
  • NMR proto NMR with chemical shift calculated from TMS (0 ppm standard) in a device of 500 megacycles (BRUCKER AMX500) using DMSO as solvent at 25°C) which revealed butyl acrylate monomers and acrylate monomers at a molar ratio of 16 butyl acrylate monomers per 84 acrylate monomers.
  • CTB Cholera toxin subunit B
  • Newcastle Disease Virus (NDV) strain Lasota Solvay Duphar, Weesp, The Netherlands was grown on eggs (following the procedures and under the conditions specified in Wilson, et al., Avian Diseases, 28, 1079-1085 (1984)) and was purified on sucrose gradient and inactivated by ⁇ -propiolactone (following the procedures and under the conditions specified in Wilson, et al., Avian Diseases, 28, 1079-1085 (1984)) to give a stock antigen solution.
  • the final concentration of the stock antigen solution contained 10 ⁇ -8 median embryo-infective doses per ml before inactivation.
  • mice Twenty-four female mice (NMRI, Charles River, Germany) were obtained and divided into four groups of six specimens per group.
  • each of the specimens of the remaining two groups (Groups 3 and 4) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in
  • M199/FCS medium was prepared having 500 ml of M199 medium
  • the lungs of two specimens were pooled and treated further as a single sample, yielding 3 samples per group.
  • the lungs were cut into small pieces and incubated for 2 hours at 37°C in
  • the spleen cells were treated in the same manner as the lung cells with the exception that the M199/FCS medium had not been supplemented with either collagenase or CaCl2.
  • the lung pieces were minced through a nylon sieve (Nybold, mesh opening 243 micron) and the cell suspensions were filtered through a nylon sieve (mesh opening 243 micron) and recovered in tubes.
  • the spleen cells were treated in the same manner, also being recovered in tubes.
  • the tubes (containing the lung cell suspensions and the spleen cell suspensions) were then centrifiiged for 5 minutes at 1,000 RPM (180 g) at 4°C and the supernatants were removed therefrom. The remaining cell pellets were then resuspended in 2 ml of the M199 FCS medium (described above). The cell suspensions obtained were then added to tubes containing 3 ml Ficoll-paque (Pharmacia) and the tubes were centrifiiged for 20 minutes at 18°C at 2,000 RPM (540 g).
  • the two lightest fractions resulting from the centrifugation which contained the lymphocytes were then collected in a new series of tubes.
  • the cells were then washed by adding 8 ml of the M199/FCS medium (described above) to about 2 ml of cell suspensions and centrifiiged for 5 minutes at 1,000 RPM (180 g) at 4°C.
  • the resulting supernatant was then removed and washing procedure was repeated one more time.
  • the resulting cell pellets were then resuspended in 2 ml of the M199 FCS medium (described above) and 2 ml of 0.83% (w/v) of NH4CI were added to each sample.
  • the cell suspensions were then gently mixed followed by centrifugation for 5 minutes at 1,000 RPM (180 g) at 4°C.
  • the resulting cell pellet was then immediately resuspended in 8 ml of the M199/FCS medium (described above). The tubes were then again centrifiiged for 5 minutes at 1,000 RPM (180 g) at 4°C.
  • the resulting cell pellet was then immediately resuspended in 8 ml of the M199/FCS medium (described above).
  • the tubes were then again centrifiiged for 5 minutes at
  • ELISPOT ELISA-plaque assay
  • the plates were then covered and incubated for 4 hours at 37°C in a vibration-free incubator to avoid displacement of the cells settled on the bottom of the wells. Following incubation, demineralized water was injected into each well with sufficient force so as to remove therefrom cells that were adhering thereto. The plates were then subsequently washed five times with
  • PBS Tween 20 (described above). 50 ⁇ l of goat antimouse IgA conjugated with biotin (Zymed) which had been diluted 500 fold in M199/FCS medium (described above) was then added to each well and the plates were incubated for 2 hours at 37°C. The plates were then washed 10 times with PBS/Tween 20 (described above) and 50 ⁇ l of streptavidine-alkaline phosphate conjugate (Zymed) which had been previously diluted 500 fold in M199/FCS medium (described above) was then added to each well and the plates were incubated for 18 hours at 4°C. The plates were then washed 10 times with PBS/Tween 20 (described above).
  • the plates were then incubated for 2 hours at room temperature and the number of blue spots in the wells containing between 10 and 40 blue spots were counted under the microscope (lOOx magnification). The number of blue spots per 10 ⁇ cells were then calculated by dividing the number of spots counted in a well by the number of cells added to that well and multiplying the result by 10 ⁇ .
  • the respective lung cell suspensions (each suspension being derived from the lungs of two individual specimens) were then tested in triplicate in the ELISPOT.
  • the respective spleen cell suspensions (each suspension being derived from the spleens of two individual specimens) were then tested in triplicate in the ELISPOT.
  • Mean values and the standard error of the mean (SEM) of the three samples of the lung and spleen cell suspensions were then calculated. The results of such calculations are set forth below in Table 1.
  • [mg/ml] is mg of adjuvant/ml of adjuvant solution
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations having the concentrations of the Butyl-PAA adjuvant set forth below in Table 2.
  • SL-CD/squalane/water adjuvant formulation was prepared following the protocol described in Hilgers (Vaccine 12, 653-660, 1994) for the sulpholipo-polysucrose/squalane/water formulation with the exception that the sulpholipo-cyclodextrin (SL-CD) was synthesized by adding sulphate and lauroyl groups to beta-cyclodextrin as decribed for the synthesis of sulpholipo-polysucrose by adding sulphate and lauroyl groups to polysucrose by Hilgers (Immunology, 60, 141-146, 1987) at a molar ratio of 1 mole sulphate, 8 moles lauroyl and 1 mole cyclodextrin.
  • SL-CD phosphate buffered saline
  • PBS phosphate buffered saline
  • the mixture obtained was then emulsified by passing through a Microfluidizer (Micro fluidics Inc.) as described for SL-polysucrose/squalane/water by Hilgers (Vaccine 12, 653-660, 1994), thereby forming a SL-CD/squalane/water adjuvant emulsion.
  • Microfluidizer Micro fluidics Inc.
  • the final concentrations of SL-CD, Tween 80 and squalane present in the SL-CD/squalane/water adjuvant formulations used in the respective examples below were 2.5 grams SL-CD per liter of adjuvant emulsion, 5.0 grams of
  • mice Eighteen female mice (NMRI, Charles River, Germany) were obtained and divided into three groups of six specimens per group. On day 0, the specimens of each of the three groups were narcotized slightly with ether.
  • each of the specimens of the remaining two groups (Groups 2 and 3) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 2, by dropping 20 ⁇ l of a particular vaccine formulation in each nostril of each specimen.
  • Administration of either the pure NDV stock antigen solution (to the specimens of Group 1) or the antigen/adjuvant vaccine formulations (to the specimens of Groups 2 and 3) was repeated on day 14 with the same mixture and using the same protocol as described above for day 0.
  • Part 4 Preparation of cell suspensions
  • the specimens were then sacrificed by cervical dislocation and the lungs thereof were carefully removed, so as to avoid the entrance of blood therein.
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 2 were determined.
  • mice Forty-two female mice (NMRI, Charles River, Germany) were obtained and divided into seven groups of six specimens per group.
  • Each of the specimens of the remaining six groups (Groups 2, 3, 4, 5, 6 and 7) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 3, by dropping 20 ⁇ l of a particular vaccine formulation in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • the specimens were then sacrificed by cervical dislocation and the lungs thereof were carefully removed, so as to avoid the entrance of blood therein.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • [mg/ml] is mg of adjuvant/ml of adjuvant solution
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations having the concentrations of the Butyl-PAA adjuvant set forth below in Table 4.
  • PAA-907 CARBOPOL-907; BFGoodrich
  • Part 2 Preparation of the vaccine formulations The Newcastle Disease Virus stock antigen solution and the various vaccine formulations, specified below in Table 4, were prepared as described above in Example 4.
  • mice Fifty-four female mice (NMRI, Charles River, Germany) were obtained and divided into nine groups of six specimens per group.
  • each of the nine groups were narcotized slightly with ether.
  • the precise dilution of the pure NDV stock antigen solution administered to the specimens of each of the Groups 1, 2 and 3 are set forth below in Table 4.
  • Each of the specimens of the remaining six groups (Groups 4, 5, 6, 7, 8 and 9) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 4, by dropping 20 ⁇ l of a particular vaccine formulation in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • the specimens were then sacrificed by cervical dislocation and the lungs thereof were carefully removed, so as to avoid the entrance of blood therein.
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 4 were determined.
  • [mg/ml] is mg of adjuvant/ml of adjuvant solution
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations having the concentrations of the Butyl-PAA adjuvant set forth below in Table 5.
  • PAA-907 (CARBOPOL-907; BFGoodrich) and the adjuvant formulations thereof were prepared as described above in Example 6 having the concentrations of the PAA-907 adjuvant set forth below in Table 5. Part 2 : Preparation of the vaccine formulations
  • mice Forty-two female mice (NMRI, Charles River, Germany) were obtained and divided into seven groups of six specimens per group.
  • Each of the specimens of the remaining six groups (Groups 2, 3, 4, 5, 6 and 7) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 5, by dropping 20 ⁇ l of a particular vaccine formulation in each nostril of each specimen.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations having the concentrations of the Butyl-PAA adjuvant set forth below in Table 6.
  • PAA-907 (CARBOPOL-907; BFGoodrich) and the adjuvant formulations thereof were prepared as described above in Example 6 having the concentrations of the PAA-907 adjuvant set forth below in Table 6.
  • CTB and the adjuvant formulations thereof were prepared as described above in Example 4 having the concentrations of the CTB adjuvant set forth below in Table 6.
  • PAA-934PH adjuvant solutions having the varying concentrations of the PAA-934PH adjuvant set forth below in Table 6.
  • Liposomes consisting of egg-yolk phosphatidylcholine (Sigma), cholesterol (Sigma) and cetylphosphate (Sigma) in a molar ratio of 4:5: 1, respectively, were prepared as described by de Haan et al. (Vaccine 13, 155-162, 1995).
  • liposome adjuvant suspensions (formulations) having the varying concentrations of the liposome adjuvant set forth below in Table 6.
  • Part 2 Preparation of the vaccine formulations The Newcastle Disease Virus stock antigen solution and the various vaccine formulations, specified below in Table 6, were prepared as described above in Example 4.
  • mice Forty-two female mice (NMRI, Charles River, Germany) were obtained and divided into seven groups of six specimens per group.
  • Each of the specimens of the remaining six groups (Groups 2, 3, 4, 5, 6 and 7) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 6, by dropping 20 ⁇ l of a particular vaccine formulation in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • the specimens were then sacrificed by cervical dislocation and the lungs thereof were carefully removed, so as to avoid the entrance of blood therein.
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 2 were determined.
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations having the concentrations of the Butyl-PAA adjuvant set forth below in Table 7.
  • PAA-907 CARBOPOL-907; BFGoodrich
  • the adjuvant formulations thereof were prepared as described above in Example 6 having the concentrations of the PAA-907 adjuvant set forth below in Table 7.
  • CTB and the adjuvant formulations thereof were prepared as described above in Example 4 having the concentrations of the CTB adjuvant set forth below in Table 7.
  • PAA-934PH (CARBOPOL-934PH; BFGoodrich) and the adjuvant formulations thereof, liposome and the adjuvant formulations thereof and Al(OH)3 (SUPERFOS) and the adjuvant formulations thereof were all prepared as described above in Example 9 having the concentrations of the respective said adjuvants, set forth below in Table 7.
  • mice Forty-two female mice (NMRI, Charles River, Germany) were obtained and divided into seven groups of six specimens per group.
  • each of the seven groups were narcotized slightly with ether.
  • Each of the specimens of the remaining six groups (Groups 2, 3, 4, 5, 6 and 7) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 7, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • the specimens were then sacrificed by cervical dislocation and the lungs thereof were carefully removed, so as to avoid the entrance of blood therein.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • the determination of the number of antigen specific IgA-producing cells in the lung cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the lung cell suspensions of only two samples of Groups 1 were determined.
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 2 were determined.
  • Part 1 Preparation of adjuvant formulations
  • BTYL-PAA polyacrylic acid
  • PAA-907 (CARBOPOL-907; BFGoodrich) and the adjuvant formulations thereof were prepared as described above in Example 6 having the concentrations of the PAA-907 adjuvant set forth below in Table 8.
  • CTB and the adjuvant formulations thereof were prepared as described above in Example 4 having the concentrations of the CTB adjuvant set forth below in Table 8.
  • PAA-934PH CARBOPOL-934PH; BFGoodrich
  • mice Forty-two female mice (NMRI, Charles River, Germany) were obtained and divided into seven groups of six specimens per group. On day 0, the specimens of each of the seven groups were narcotized slightly with ether.
  • the specimens of the remaining seven groups were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 8, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 2 were determined.
  • [mg/ml] is mg of adjuvant ml of adjuvant solution
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations having the concentrations of the Butyl-PAA adjuvant set forth below in Table 9.
  • PAA-907 CARBOPOL-907; BFGoodrich
  • the adjuvant formulations thereof were prepared as described above in Example 6 having the concentrations of the PAA-907 adjuvant set forth below in Table 9.
  • PAA-934PH (CARBOPOL-934PH; BFGoodrich) and the adjuvant formulations thereof and Al(OH)3 (SUPERFOS) and the adjuvant formulations thereof were all prepared as described above in Example 9 having the concentrations of the PAA-934PH adjuvant or the Al(OH)3 adjuvant, set forth below in Table 9.
  • Part 2 Preparation of the vaccine formulations The Newcastle Disease Virus stock antigen solution and the various vaccine formulations were prepared as described above in Example 4. Part 3 : Immunization of the specimens
  • mice Sixty female mice (NMRI, Charles River, Germany) were obtained and divided into ten groups of six specimens per group. On day 0, the specimens of each of the ten groups were narcotized slightly with ether.
  • Each of the specimens of the remaining eight groups (Groups 3, 4, 5, 6, 7, 8, 9 and 10) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 9, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions The determination of the number of antigen specific IgA-producing cells in the lung cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the lung cell suspensions of only two samples of Groups 6 and 8 were determined. The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1-4 were determined. The results of such calculations are set forth below in Table 9. TABLE 9
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations having the concentrations of the Butyl-PAA adjuvant set forth below in Table 10.
  • PAA-907 (CARBOPOL-907; BFGoodrich) and the adjuvant formulations thereof were prepared as described above in Example 6 having the concentrations of the PAA-907 adjuvant set forth below in Table 10.
  • the Newcastle Disease Virus stock antigen solution and the various vaccine formulations were prepared as described above in Example 4. Part 3 : Immunization of the specimens Eighty-four female mice (NMRI, Charles River, Germany) were obtained and divided into fourteen groups of six specimens per group.
  • each of the fourteen groups were narcotized slightly with ether.
  • Each of the specimens of the remaining sixteen groups (Groups 3, 4, 5, 6,
  • the determination of the number of antigen specific IgA-producing cells in the lung cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the lung cell suspensions of only two samples of Groups 10 and 12 were determined.
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of three samples of only Groups 1-4 were determined.
  • Sulpholipo-cyclodextrin/squalane/water (SL-CD/squalane/water) adjuvant formulations were prepared as described above in Example 5 having the concentrations of the SL-CD/squalane/water adjuvant set forth below in Table
  • Newcastle Disease Virus stock antigen solution and the various vaccine formulations were prepared as described above in Example 4.
  • mice Seventy-two female mice (NMRI, Charles River, Germany) were obtained and divided into twelve groups of six specimens per group.
  • Each of the specimens of the remaining eight groups (Groups 5, 6, 7, 8, 9, 10, 11 and 12) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 11, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cells suspensions The determination of the number of antigen specific IgA-producing cells in the lung cells suspensions was performed as described above in Example 4.
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of three samples of only Groups 1-8 were determined.
  • [mg/ml] is mg of adjuvant/ml of adjuvant solution
  • Sulpholipo-cyclodextrin/squalane/water (SL-CD/squalane/water) adjuvant formulations were prepared as described above in Example 5 having the concentrations of the SL-CD/squalane/water adjuvant set forth below in Table 12. Part 2 : Preparation of the Vaccine Formulations
  • the Newcastle Disease Virus stock antigen solution and the various vaccine formulations were prepared as described above in Example 4. Part 3 : Immunization of the specimens
  • mice Eighteen female mice (NMRI, Charles River, Germany) were obtained and divided into three groups of six specimens per group.
  • each of the three groups were narcotized slightly with ether.
  • Each of the specimens of the remaining two groups (Group 2 and Group 3) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation), as specified below in Table 12, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the stock antigen solution and 20 ⁇ l of a particular adjuvant formulation
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cells suspensions The determination of the number of antigen specific IgA-producing cells in the lung cells suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the lung cell suspensions of only two samples of Group 1 were determined.
  • the Newcastle Disease Virus stock antigen solution and the various vaccine formulations were prepared as described above in Example 4. Part 3 : Immunization of the specimens
  • mice Eighteen female mice (NMRI, Charles River, Germany) were obtained and divided into three groups of six specimens per group.
  • each of the three groups were narcotized slightly with ether.
  • Each of the specimens of the remaining two groups (Group 2 and Group 3) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant solution), as specified below in Table 13, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant solution
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cells suspensions
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 2 were determined.
  • [mg ml] is mg of adjuvant/ml of adjuvant solution
  • Liposome and the adjuvant formulations thereof were prepared as described above in Example 9 having the concentrations of the liposome adjuvant set forth below in Table 14.
  • Part 2 Preparation of the vaccine formulations The Newcastle Disease Virus stock antigen solution and the various vaccine formulations were prepared as described above in Example 4. Part 3 : Immunization of the specimens
  • mice Eighteen female mice (NMRI, Charles River, Germany) were obtained and divided into three groups of six specimens per group. On day 0, the specimens of each of the three groups were narcotized slightly with ether.
  • Each of the specimens of the remaining two groups (Group 2 and Group 3) were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant solution), as specified below in Table 14, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant solution
  • Example 4 The determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 2 were determined.
  • [mg/ml] is mg of adjuvant/ml of adjuvant solution
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations thereof having the concentrations of the Butyl-PAA adjuvant set forth below in Table 15.
  • PAA-907 (CARBOPOL-907; BFGoodrich) adjuvant formulations were prepared as described above in Example 6 having the concentrations of the PAA-907 adjuvant set forth below in Table 15.
  • PAA-934PH (CARBOPOL-934PH; BFGoodrich) adjuvant formulations and Al(OH)3 (SUPERFOS) adjuvant formulations were prepared as described above in Example 9 having the concentrations of the respective adjuvant therein set forth below in Table 15.
  • CTB and the adjuvant formulations thereof were prepared as described above in Example 4 having the concentrations of the CTB adjuvant set forth below in Table 15.
  • Liposome and the adjuvant formulations thereof were prepared as described above in Example 9 having the concentrations of the liposome adjuvant set forth below in Table 15. Part 2 : Preparation of the vaccine formulations
  • the vaccine formulation to be used was then obtained by mixing 1 volume of antigen solution with 1 volume of adjuvant solution.
  • Part 3 Immunization of the specimens Thirty-six female mice (NMRI, Charles River, Germany) were obtained and divided into six groups of six specimens per group.
  • Each of the specimens of the remaining five groups were then immunized intranasally with respective 40 ⁇ l doses of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant solution) as specified below in Table 15 (which vaccine formulations were obtained as described above) by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • the vaccine formulations antigen/adjuvant mixtures containing 20 ⁇ l of the antigen solution and 20 ⁇ l of a particular adjuvant solution
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cells suspensions
  • the determination of the number of antigen specific IgA-producing cells in the lung cells suspensions was performed as described above in Example 4, with the exception that, the number of antigen specific IgA-producing cells in the lung cell suspensions of only two samples of Groups 1 were determined and that, for the ELISPOT, the plates were coated with 25 ⁇ g purified inactivated influenza virus strain MRC-11 per ml coating buffer.
  • the determination of the number of antigen specific IgA-producing cells in the spleen cell suspensions was performed as described above in Example 4, with the exception that the number of antigen specific IgA-producing cells in the spleen cell suspensions of only two samples of Groups 1 and 2 were determined and that, for the ELISPOT, the plates were coated with 25 ⁇ g purified inactivated influenza virus strain MRC-11 per ml coating buffer.
  • [mg/ml] is mg of adjuvant/ml of adjuvant solution
  • the butyl-ester of polyacrylic acid (BUTYL-PAA), synthesized as described above in Example 2, was prepared as described above in Example 4 to form the adjuvant formulations thereof having the concentrations of the Butyl-PAA adjuvant set forth below in Table 16.
  • PAA-907 (CARBOPOL-907; BFGoodrich) adjuvant formulations were prepared as described above in Example 6 having the concentrations of the
  • PAA-907 adjuvant set forth below in Table 16.
  • Bovine serum albumin (BSA) (from BSA, Fraction V, SIGMA) was prepared by dissolving in PBS at a final concentration of 500 ⁇ g/ml.
  • Each of the specimens of Group 4 were then administered respective 40 ⁇ l doses of the pure BSA stock antigen solution by dropping 20 ⁇ l of the said stock antigen solution in each nostril.
  • Each of the specimens of the remaining four groups (Groups 2, 3, 5 and 6) were then immunized intranasally with 40 ⁇ l of the vaccine formulations (antigen/adjuvant mixtures containing 20 ⁇ l of a particular antigen solution and 20 ⁇ l of a particular adjuvant solution), as specified below in Table 16, by dropping 20 ⁇ l of the mixture in each nostril of each specimen.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cells suspensions The determination of the number of antigen specific IgA-producing cells in the lung cells suspensions was performed as described above in Example 4, with the exception that, for the ELISPOT for the specimens of Groups 4, 5 and 6, the plates were coated with 25 ⁇ g of BSA per ml coating buffer.
  • [mg/ml] is mg of adjuvant/ml of adjuvant solution
  • p(A-c-AMPS) copolymers Two p(A-c-AMPS) copolymers were synthesized as described by Iliopoulos and Audebert in Macromolecules 24, 2566-2575 (1991). Briefly, monoacrylic acid (AA; Merck) and acrylamidomethylpropanesulphonic acid (AMPS; Merck) were dissolved in ultrapure water, pH was adjusted at 7.4 with 10 N NaOH solution and ultrapure water was added to final total monomer concentration of 2 M. Air was removed from the solution by passing through nitrogen for at least 20 min.(NH4)2S2 ⁇ 8 and Na2S2 ⁇ 5 were added to final concentrations of 1.46 mM and 2.91 mM, respectively.
  • AA monoacrylic acid
  • AMPS acrylamidomethylpropanesulphonic acid
  • the mixture was incubated for 2.25 at 24 °C or 3 h at 20 °C under nitrogen and continuous stirring. After incubation, an excess of methanol was added and the mixture was kept overnight at ambient temperature.
  • the precipitate formed was recovered in a solution of 9 g NaCl per L ultrapure water and dialyzed (Spectro Por; MWCO 12,000 - 14,000 D) at 4 °C until no monomers were detected in the diafiltrate (absorbance at 210 nm ⁇ 0.1 absorption units) and then dialyzed (Spectro/Por; MWCO 12,000 - 14,000 D) against ultrapure water.
  • the retentate was lyophilized and the copolymers was recovered as powder and stored at ambient temperature until use.
  • the molecular weight of the polymers was determined by gel permeation chromatography on a Sephacryl S400 column (Pharmacia, Sweden) using polyacrylate polymers with MW of 5, 90, 450, 750, 1000 and 3000 kD (Aldrich) as standards and absorbance at 210 nm as detection system.
  • the percentage of AMPS monomer in the copolymer obtained was determined by element analysis. Details of the preparation procedure of copolymers and of the copolymers obtained are set forth below in Table 17.
  • a p(A-c-VS) copolymer was synthesized as described above for p(A-c-AMPS) in
  • Example 20 Briefly, monoacrylic acid (AA; Merck) and vinylsulphonic acid sodium salt (VS; Fluka) were dissolved in ultrapure water, pH was adjusted at 7.4 with 10 N NaOH solution and ultrapure water was added to final total monomer concentration of 2 M. Air was removed by saturating the solution with nitrogen. (NH4)2S2 ⁇ 8 and Na2S2 ⁇ 5 were added to final concentrations of 1.46 mM and 2.91 mM, respectively. The mixture was incubated for 6 h at 19 °C under nitrogen and continuous stirring. After incubation, an excess methanol was added and the mixture was kept overnight at ambient temperature.
  • AA monoacrylic acid
  • VS vinylsulphonic acid sodium salt
  • the precipitate formed was recovered in a solution of 9 g NaCl per L ultrapure water and dialyzed (Spectro/Por; MWCO 12,000 - 14,000 D) at 4 °C until no monomers were detected in the diafiltrate (absorbance at 210 nm ⁇ 0.1 absorption units) and then dialyzed (Spectro/Por; MWCO 12,000 - 14,000 D) against ultrapure water.
  • the retentate was lyophilized and the copolymer was recovered as powder and stored at ambient temperature until use.
  • the molecular weight of the polymer was determined by gel permeation chromatography on a Sephacryl S400 column (Pharmacia, Sweden) using polyacrylate polymers with MW of 5, 90, 450, 750, 1000 and 3000 kD (Aldrich) as standards and absorbance at 210 nm as detection system.
  • the percentage of VS monomer in the copolymer obtained was determined by element analysis. Details of the preparation procedure of the copolymer and of the copolymer are set forth below in Table 18. Table 18: Preparation of copolymer p(A-c-VS) #3 by copolymerisation of monoacrylic
  • p( ⁇ -c-VBS) copolymers were synthesized as described above for p(A-c-AMPS) in Example 20. Briefly, monoacrylic acid (AA) and vinylbenzenesulphonic acid sodium salt (VBS) were dissolved in ultrapure water, pH was adjusted at 7.4 with 10 N NaOH solution and ultrapure water was added to final total monomer concentration of 2 M. The solutions of the two monomers were saturated with nitrogen for at least 20 min. (NH4 2S2 ⁇ 8 and Na2S2 ⁇ 5 were added to final concentrations of 1.46 mM and 2.91 mM, respectively.
  • AA monoacrylic acid
  • VBS vinylbenzenesulphonic acid sodium salt
  • the mixtures were incubated for 6 or 24 h at 20 °C under nitrogen and continuous stirring of the solution. After incubation, an excess of methanol was added and the mixtures were kept overnight at ambient temperature.
  • the precipitates formed were recovered in a solution of 9 g NaCl per L ultrapure water and dialyzed (Spectro/Por; MWCO 12,000 - 14,000 D) at 4 °C until no monomers were detected in the diafiltrate (absorbance at 210 nm ⁇ 0.1 absorption units) and then dialyzed (Spectro/Por; MWCO 12,000 - 14,000 D) against ultrapure water.
  • the retentates were lyophilized and the copolymers were recovered as powder and stored at ambient temperature until use.
  • the molecular weight of the polymers were determined by gel permeation chromatography on a Sephacryl S400 column (Pharmacia, Sweden) using polyacrylate polymers 5, 90, 450, 750, 1000 and 3000 kD (Aldrich) as standards and absorbance at 210 nm as detection system.
  • the percentage of VBS monomer in the copolymer obtained was determined by element analysis. Details of the preparation procedure of the copolymers and of the coplymers obtained are set forth below in Table 19. Table 19: Preparation of copolymer p(A-c-VBS) #4, #5, #6 and #8 by copolymerisation of monoacrylic acid (AA) and vinylbenzenesulphonic acid sodium salt (VBS).
  • Example 22 VBS in Example 22 with the exception that incubation time was between 24 and 168 h, incubation temperature was 37 °C, and copolymers were recovered by diafiltration over a 100 kD (UFP-100-E6, AGFiltration) and 10 kD (UFP-10-E6, AGFiltration) giving two fractions of polymers with MW > 100 kD and 10-100 kD.
  • the polymer were lyophilized and stored at ambient temperature until use. Details of the copolymers and their preparation procedure are set out in Table 20.
  • Table 20 Preparation of copolymer p(A-c-VBS) #11 to #18 by copolymerisation of monoacr lic acid (AA) and vin lbenzenesul honic acid sodium salt (VBS).
  • AA monoacr lic acid
  • VBS vin lbenzenesul honic acid sodium salt
  • Example 24 Effects of BUTYL-PAA. p(A-c-VS) and p(A-c-VBS)copolvmers and polystyrene sulphonate CPSS) on numbers of anti-NDV IgA-producing cells in lung cell suspensions
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • Example 24 was repeated and the results are set forth below in Table 22.
  • Antigen preparation A/Swine influenza virus strain A/Swine, was grown in embryonic eggs, purified by centrifugation on a sucrose gradient and inactivated by incubation with
  • Antigen stock solution of 250 ⁇ g HA per ml was prepared.
  • the various vaccines formulations, specified below in Table 23, were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Swine antigen solution.
  • mice Thirty-six female mice (BALB/c, Charles River, Germany) were obtained and divided into 6 groups of six specimens per group and treated with the vaccines set out in Table
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • Butyl-PAA, p(A-c-VBS) and PSS were obtained as described above in Examples 4, 22 and 24 respectively.
  • Stock A/Swine antigen solution prepared as decribed above in Example 26 was adjusted at final concentrations of of 50 ⁇ g HA per ml.
  • the various vaccines formulations, specified below in Table 24, were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Swine antigen solution described above.
  • mice Thirty-six female mice (BALB/c, Charles River, Germany) were obtained and divided into 6 groups of six specimens per group and treated with the vaccines set out in Table
  • Part 4 Preparation of the cell suspensions As described in Example 4.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • BUTYL-PAA was synthesized and prepared as described above in Example 4 to form the adjuvant formulation having the concentration of BUTYL-PAA set forth below in Table 25. Part 2 : Preparation of the vaccine formulations
  • mice Thirty-six female mice (BALB/c, Charles River, Germany) were obtained, divided into 6 groups of 6 specimens per group and treated with the vaccines set out in Table 25 according to the general methodology of Example 4.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • Example 4 As described in Example 4 except that the plates were coated with 50 ⁇ g of influenza strain A/Swine per ml coating buffer described in Example 4.
  • BUTYL-PAA was synthesized and prepared as described above in Example 4 to form the adjuvant formulation having the various concentrations set forth below in Table 26.
  • the various vaccines formulations were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Swine antigen solution prepared as described above in
  • mice Twenty-four female mice (BALB/c, Charles River, Germany) were obtained, divided into four groups of six specimens per group, and treated with the vaccines set out in
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • BUTYL-PAA was synthesized and prepared as described above in Example 4 to form the adjuvant formulation having the concentration set forth below in Table 27.
  • Antigen preparation A/Texas influenza virus strain A/Texas (Texas), was grown in embryonic eggs, purified by centrifugation on a sucrose gradient and inactivated by incubation with 0.05% (v/v) beta-propiolactone plus 0.01% (w/v) thimerosal for 4 days at 4 °C and subsequently for 3 days at room temperature as described in Vaccine 12, 653-660 (1994).
  • Haemagglutinin/neuraminidase (HA/NA) subunits of the virus were isolated from the virus by using detergent(s). An antigen stock solution of 250 ⁇ g HA per ml was prepared. Part 2 : Preparation of the vaccine formulations
  • the various vaccines formulations were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Texas antigen solution prepared as described above.
  • mice Twelve female mice (BALB/c, Charles River, Germany) were obtained, divided into two groups of six specimens per group and treated with the vaccines set out in Table 27, according to the general methodology of Example 4.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • Example 4 The results are set forth below in Table 2 7 .
  • Example 30 The experiment of Example 30 was repeated and the results are set forth below in Table 28. Table 28.
  • Part 2 Preparation of the vaccine formulations
  • the various vaccines formulations specified below in Table 29, were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Texas antigen solution prepared as described above in
  • mice Twenty-four female mice (BALB/c, Charles River, Germany) were obtained, divided into four groups of six specimens per group and treated with the vaccines set forth in
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • Example 33 Effects of BUTYL-PAA and pfA-c-VBS) copolymers on numbers of anti-A/Texas IgA- producing cells in lung cell suspensions Preparation of adjuvant formulations
  • Example 32 was repeated with two formulations of the p(A-c-VBS) copolymer adjuvant. The results are set forth below in Table 30. Table 30.
  • the various vaccines formulations were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Texas antigen solution prepared as described above in
  • mice Twenty-four female mice (BALB/c, Charles River, Germany) were obtained, divided into four groups of six specimens per group and treated with the vaccines set forth in
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • Example 4 As described in Example 4 with the exception that, for the Elispot the plates were coated with 50 ⁇ g of influenza strain A/Texas per ml coating buffer described in Example 4.
  • BUTYL-PAA and p(A-c-VBS) copolymers were synthesized as described above in
  • Example 4 and 23 to form the adjuvant formulations having the concentrations set forth below in Table 32.
  • Part 2 Preparation of the vaccine formulations
  • the various vaccines formulations were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Texas antigen solution prepared as described in Example
  • mice Forty eight female mice (BALB/c, Charles River, Germany) were obtained, divided into
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • Example 4 and 23 to form the adjuvant formulations having the concentrations set forth below in Table 33.
  • the various vaccines formulations were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Texas antigen solution prepared as described above in
  • mice Forty eight female mice (BALB/c, Charles River, Germany) were obtained, divided into 6 groups of six specimens per group and treated with vaccines as set out in Table 33, according to the general methodology of Example 4.
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • BUTYL-PAA and p(A-c-VBS) copolymer #5 were synthesized and prepared as described above in Example 4 and 22, to form the adjuvant formulations having the concentrations set forth below in Table 34.
  • the various vaccines formulations were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock A/Texas antigen solution prepared as described in Example
  • mice Eighteen female mice (BALB/c, Charles River, Germany) were obtained, divided into three groups of six specimens per group and treated with vaccines as set out below in
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions
  • the various vaccines formulations were then prepared by mixing one volume of the respective adjuvant formulations, prepared as described above, with one volume of the stock antigen solution.
  • mice Eighteen female mice (BALB/c, Charles River, Germany) were obtained, divided into three groups of six specimens per group and treated with the vaccines set forth in Table
  • Part 5 Determination of the number of antigen specific IgA-producing cells in the cell suspensions

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EP97950021A EP0934077B1 (en) 1996-10-24 1997-10-23 Polyanionic polymers as adjuvants for mucosal immunization
BR9712436-2A BR9712436A (pt) 1996-10-24 1997-10-23 Polìmeros polianiÈnicos como adjuvantes para imunização da mucosa
DE69737658T DE69737658T2 (de) 1996-10-24 1997-10-23 Polyanionische polymere als adjuvantien zur mukosalen immunisierung
JP51897598A JP4344014B2 (ja) 1996-10-24 1997-10-23 粘膜性免疫用アジュバントとしてのポリアニオン性ポリマー
US09/297,214 US6610310B2 (en) 1996-10-24 1997-10-23 Polyanionic polymers as adjuvants for mucosal immunization
CA002269780A CA2269780C (en) 1996-10-24 1997-10-23 Polyanionic polymers as adjuvants for mucosal immunization
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FR2922767A1 (fr) * 2007-10-24 2009-05-01 Seppic Sa Procede de preparation d'une composition vaccinale comprenant au moins un antigene et au moins un adjuvant.
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ES2285741T3 (es) 2007-11-16
DE69737658D1 (de) 2007-06-06

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