WO2001098206A1 - Delivery vehicle composition and methods for delivering antigens and other drugs - Google Patents
Delivery vehicle composition and methods for delivering antigens and other drugs Download PDFInfo
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- WO2001098206A1 WO2001098206A1 PCT/US2001/020096 US0120096W WO0198206A1 WO 2001098206 A1 WO2001098206 A1 WO 2001098206A1 US 0120096 W US0120096 W US 0120096W WO 0198206 A1 WO0198206 A1 WO 0198206A1
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- delivery vehicle
- immunogen
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
- A61K39/02—Bacterial antigens
- A61K39/04—Mycobacterium, e.g. Mycobacterium tuberculosis
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K31/00—Medicinal preparations containing organic active ingredients
- A61K31/70—Carbohydrates; Sugars; Derivatives thereof
- A61K31/715—Polysaccharides, i.e. having more than five saccharide radicals attached to each other by glycosidic linkages; Derivatives thereof, e.g. ethers, esters
- A61K31/716—Glucans
- A61K31/721—Dextrans
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K31/00—Medicinal preparations containing organic active ingredients
- A61K31/70—Carbohydrates; Sugars; Derivatives thereof
- A61K31/715—Polysaccharides, i.e. having more than five saccharide radicals attached to each other by glycosidic linkages; Derivatives thereof, e.g. ethers, esters
- A61K31/716—Glucans
- A61K31/722—Chitin, chitosan
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K31/00—Medicinal preparations containing organic active ingredients
- A61K31/74—Synthetic polymeric materials
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/0012—Galenical forms characterised by the site of application
- A61K9/0043—Nose
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- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K9/00—Medicinal preparations characterised by special physical form
- A61K9/0012—Galenical forms characterised by the site of application
- A61K9/007—Pulmonary tract; Aromatherapy
- A61K9/0073—Sprays or powders for inhalation; Aerolised or nebulised preparations generated by other means than thermal energy
- A61K9/0078—Sprays or powders for inhalation; Aerolised or nebulised preparations generated by other means than thermal energy for inhalation via a nebulizer such as a jet nebulizer, ultrasonic nebulizer, e.g. in the form of aqueous drug solutions or dispersions
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
- A61K2039/555—Medicinal preparations containing antigens or antibodies characterised by a specific combination antigen/adjuvant
- A61K2039/55511—Organic adjuvants
- A61K2039/55561—CpG containing adjuvants; Oligonucleotide containing adjuvants
Definitions
- This invention relates to a delivery vehicle composition for delivery of an antigen or another active material and methods for using such a delivery vehicle composition, and especially for stimulating an immune response both systemically and mucosally.
- an immunogen composition should potentiate long-lasting expression of functionally active antibodies, elicit cell-mediated immunity ("CMI"), and enhance production of memory T- and B-lymphocytes with highly specific immunoreactivity against an invading antigen.
- CMI cell-mediated immunity
- these responses should provide protection against any future encounters of the host with a specific antigen.
- the form of the antigen includes the form of the antigen, whether soluble or particulate in nature, the foreignness of the antigen, i.e., how far removed the antigen is from the host on the phylogenetic tree, the stability of the antigen to degradative enzymes of the host and the ability of the antigen to persist in the host for long periods of time.
- the immunogenicity of an antigen that elicits a weak immune response may be improved by manipulation of one or more of these parameters.
- the immunogenicity of an antigen has been improved by injecting it in a formulation that includes an adjuvant.
- Adjuvants non-specif ⁇ cally augment immune responses and their ability to potentiate immune responses has long been recognized.
- adjuvants A wide variety of substances, both biological and synthetic, have been used as adjuvants in experimental systems. These include mycobacteria, oil emulsions, liposomes, polymer microparticles and mineral gels.
- the mechanism by which adjuvants enhance immune responses is not uniform but their effects may include retention of antigen at the site of administration such that the antigen is released to the body slowly over time or array of the antigen in a particulate form so that it is more easily recognized by lymphocytes and taken up by antigen presenting cells.
- Adjuvants consisting of microbial products generally act by enhancing the uptake of antigens by professional antigen-presenting cells and or by stimulation of the innate immune system, which in turn leads to more potent stimulation of lymphocytes themselves.
- vaccines are usually administered several times over a time span of months in order to elicit an immune response that can confer protection on the host upon subsequent encounter with the antigen, e.g., microbe, itself.
- antigen e.g., microbe
- vaccines for a variety of infectious diseases are currently available, many of these, including those for tetanus and hepatitis B, require more than one administration to confer protective benefit.
- These limitations are extremely problematic in countries where healthcare is not readily available or accessible.
- compliance is also a problem in developed countries, particularly for childhood immunization programs. For example, a child in the United States may be scheduled to receive a total of 16 vaccine injections by age 18 months and 35 vaccine injections by age five.
- Mucosal vaccine strategies have recently emerged as an attractive potential alternative to injectable vaccines.
- Mucosal administration would have many potentially desirable attributes. This form of administration is relatively easy and low cost, especially when compared to injection regimens. As such, mucosal administration has significant potential to improve compliance in both developing and developed countries relative to vaccine injections, particularly for childhood immunization programs. Another advantage of mucosal administration compared to injection is a reduced risk of contamination with elimination of the use of needles.
- mucosal vaccine delivery techniques Perhaps the most compelling reason for developing mucosal vaccine delivery techniques, however, is development of a first line of immunity defense, by generating local immunity at the mucosal site of entry for many invading pathogens. Moreover some investigators have reported that a common mucosal immune system exists, whereby mucosal immunity induced at one site can lead to immunity at a distal mucosal site (McGhee, J.R. et al. The mucosal immune system: from fundamental concepts to vaccine development. Vaccine 1992, 10:75-88). This suggests that significant benefits can be achieved by the delivering of vaccines in a non-invasive way, e.g.
- intranasally or other mucosal route to elicit immunity to a wide range of pathogens that may enter at different mucosal sites, e.g. HIN, HPN.
- delivery of an antigen via a mucosal site has the potential to generate a systemic immune response as well.
- a mucosal immune response consists of all the components of the systemic immune system including the ability to generate cell-mediated and humoral responses.
- Cells of the immune system are distributed throughout mucosal tissues and include T and B cells and cells capable of antigen presentation, such as dendritic cells and monocytes/macrophages ( ⁇ eutra, M.R. et al. Antigen sampling across epithelial barriers and induction of mucosal immune responses. 1996. Ann. Rev. Immunol.14: 275-300).
- the main antibody class present in the mucosal immune system is IgA, which is exported in polymeric form into mucosal secretions.
- IgA antibodies prevent attachment of infectious agents or their toxins to mucosal epithelia thereby providing a first line of defense against infection. Detection of IgA antibodies in washes of mucosal surfaces indicates the generation of a mucosal immune response to an antigen. Although there is great promise for mucosal administration of vaccines, delivery of many antigens, such as proteins and peptides, to the mucosal tissue does not necessarily result in the generation of an immune response. The generation of mucosal immunity to antigens is dependent upon the same criteria as is the systemic immune response, namely that the antigen must be presented appropriately in a form that will lead to stimulation of T and B lymphocytes.
- mucosal delivery of antigens may result in low bioavailability and also may induce immunological tolerance (e.g. Lowrey, J.L. et al. Induction of tolerance via the respiratory mucosa. Int. Arch. Allergy Immunol. 1998, 116: 93-102).
- Monophosphoryl lipid A enhances mucosal and systemic immunity to vaccine antigens following mtranasal administration. 2000. Vaccine 18: 2416-2425), immunostimulatory DNA sequences (Horner, A.A. et al. Immunostimulatory DNA is a potent mucosal adjuvant. 1998. Cell. Immunol. 190: 77-82; McCluskie, M.J. et al. mtranasal immunization of mice with CpG DNA induces strong systemic and mucosal responses that are influenced by other mucosal adjuvants and antigen distribution. 2000. Mol. Med.
- mice outer membrane proteins of Neiserria meningitidis serogroup B (Levi, R. et al. 1995. mtranasal immunization of mice against influenza with synthetic peptides anchored to proteosomes. Vaccine 13: 1353-9), and bacterial toxins such as cholera toxin (CT) subunit B and E. coli enterotoxin (ET) (Isaka, M. et al. Systemic and mucosal immune responses of mice to aluminum- adsorbed or aluminum-non-adsorbed tetanus toxoid administered intranasally with recombinant cholera toxin B subunit.
- CT cholera toxin
- ET E. coli enterotoxin
- Vaccine 18 2164-2171; and Barchfeld, G. L. et al.
- the adjuvants MF59 and LT-K63 enhance the mucosal and systemic immunogenicity of subunit influenza vaccine administered intranasally in mice. 1999. Vaccine 17: 695-704).
- the inherent toxicity of bacterial toxins generally precludes their use in human vaccines.
- Detoxified mutants of both CT and ET have been produced (Pizza, M., et al. A genetically detoxified derivative of heat-labile Escherichia coli enterotoxin induces neutralizing antibodies against the A subunit. 1994. J Exp Med 180, 2147-53; Yamamoto, S., et al.
- chitosan a cationic biopolymer derived from deacetylated chitin. Chitosan has been shown to act as a penetration enhancer to the extent its presence appears to improve the uptake of at least some drugs through the nasal mucosa.
- chitosan has been shown to have pro-inflammatory activity, activating macrophages and stimulating secretion of pro-inflammatory cytokines such as TNFo; and IL1 3 from monocytes in vitro. Therefore it appears to act as an immunological adjuvant in at least some circumstances.
- pro-inflammatory cytokines such as TNFo
- IL1 3 from monocytes in vitro. Therefore it appears to act as an immunological adjuvant in at least some circumstances.
- These properties of chitosan have been exploited in the development of vaccines for both intransal and systemic (e.g. intraperitoneal) delivery (McNeela, E. A. et al. 2001.
- a mucosal vaccine against diphtheria formulation of cross reacting material (CRM197) of diphtheria toxin with chitosan enhances local and systemic antibody and ThJ responses following nasal delivery.
- the present invention provides a delivery vehicle composition for delivery of a drug and methods for administering the delivery vehicle composition to effect a desired biological response in the host.
- the delivery vehicle composition comprises at least one drug, at least one biocompatible polymer and at least one liquid vehicle, with the polymer and the liquid vehicle being of such a type and being present in such proportions that the delivery vehicle composition exhibits reverse-thermal viscosity behavior, meaning that the viscosity of the composition increases with increasing temperature over at least some temperature range.
- the delivery vehicle composition also typically includes at least one additive selected from the group consisting of an adjuvant, a penetration enhancer and combinations thereof.
- the delivery vehicle composition is such that it will typically be administered to the host in the form of a flowable medium at a temperature below the physiological temperature of the host.
- the viscosity of the composition then increases as the composition is warmed inside the host, and preferably the composition converts to a substantially immobile gel form so that the composition is retained at the desired location for delivery of the drug.
- the delivery vehicle composition is administerable to a host in any convenient way for example by injection or direct application to the desired site.
- One advantage of the delivery vehicle composition is that it is particularly well suited for mucosal delivery.
- the delivery vehicle composition is in the form of dispersed droplets in a mist.
- the mist is introduced into the appropriate cavity of administration. Such a mist is typically generated by a nebulizer.
- the delivery vehicle composition is exemplified herein by an immunogen composition of the invention in which the drug is an antigen for stimulating an immune response, and preferably without the use of adjuvants, such as alum, of questionable safety.
- the biocompatible polymer helps to protect the antigen from possible degradation and to promote prolonged release of the antigen into the host following administration.
- a preferred liquid vehicle is water or another aqueous liquid and the biocompatible polymer is typically a reverse-thermal gelation polymer, with polyoxyalkylene block polymers being particularly preferred.
- the biocompatible polymer is dissolved in the liquid vehicle when the temperature of the immunogen composition is at some temperature or temperatures below the physiological temperature of the host (approximately 37°C for humans) so that the biocompatible polymer/liquid vehicle solution is in the form of a flowable liquid.
- the antigen is also preferably dissolved in the liquid vehicle along with the biocompatible polymer.
- the antigen may be in the form of a particulate suspended in the biocompatible polymer/liquid vehicle solution.
- the composition should be in the form of a flowable medium sufficient for nebulization to produce a spray and/or for injectability.
- the immunogen composition is in the form of a gel (semi- solid gelatinous substance) when the composition is at the physiologic temperature of the host (approximately 37 °C for humans).
- the gel is formed by the interaction between the polymer and the liquid vehicle.
- the antigen should be uniformly dispersed throughout the gel, which is preferably accomplished by initially preparing the immunogen composition at a temperature at which the polymer is dissolved in the liquid vehicle. The antigen can be dissolved in or uniformly dispersed throughout the solution, and then the temperature of the composition can be raised to convert the immunogen composition to a gel form.
- the immunogen composition exhibits reverse-thermal gelation properties, in that the polymer, as incorporated in the immunogen composition, has a gel-liquid transition temperature such that the biocompatible polymer is in solution in the liquid vehicle of some temperature below the transition temperature and the biocompatible polymer and liquid vehicle form a gel, i.e., become gelatinous, as the temperature is raised above the transition temperature.
- a gel-liquid transition temperature may be referred to as a reverse-thermal liquid-gel transition temperature.
- the reverse-thermal liquid-gel transition temperature should typically be below, and more preferably just below, the physiological temperature of the host.
- the composition is administrable to a host at a temperature at which the composition is in the form of a flowable medium and after administration the immunogen composition then converts to a gel form as it warms inside the host to above the transition temperature.
- the composition can be placed in a syringe or syringe-like device then administered to the host and it can also be placed in a spray device and administered to the host.
- the immunogen composition preferably has an affinity to adhere to mucosal surfaces, and conversion to a gel form helps to immobilize the immunogen composition at the mucosal surface to retain the antigen in the vicinity of the mucosal surface, thereby permitting the antigen to be effectively delivered to penetrate the mucosal tissue to induce the desired immune response.
- the biocompatible polymer is bioadhesive, so that when the immunogen composition is contacted with a mucosal surface, at least a portion of the biocompatible polymer readily adheres to the mucosal surface.
- the biocompatible polymer and the antigen are closely associated with each other in the immunogen composition so that when the biocompatible polymer adheres to a mucosal surface, the antigen is held in the vicinity of the surface for effective delivery of the antigen across the mucosal epithelium. This will typically be the case, for example, in a preferred embodiment when the carrier liquid is an aqueous liquid and the biocompatible polymer has surfactant properties.
- the immunogen composition comprises, in addition to the biocompatible polymer and the antigen, a penetration enhancer that aids rapid transport of the composition across the mucosal epithelium.
- a penetration enhancer that aids rapid transport of the composition across the mucosal epithelium.
- the penetration enhancer has been found to improve the immune response following administration of the immunogen composition.
- the combination of the penetration enhancer and the polymer provide for significant protection of the antigen from degradation and promote release of the antigen from the composition in an advantageous manner.
- the immunogen composition includes an adjuvant to nonspecifically enhance the immune response.
- a particularly advantageous aspect of the present invention is that adjuvant-type enhancements are achievable without the use of alum or other known adjuvant materials of questionable safety.
- an additive is included in the immunogen composition that acts as both a penetration enhancer and adjuvant, with chitosan materials being particularly preferred for use as the additive for this purpose.
- the immunogen composition is administrable mucosally to stimulate both a strong mucosal immune response and also a strong systemic immune response.
- the immunogen composition provides the added immunity protection at the site for entry for many major pathogenic organisms, as a first line of defense against and infection by such organisms.
- the use of the immunogen composition therefore, has the potential to replace current injection regimens that are effective at developing only systemic immunity, and are not effective at developing mucosal immunity.
- the immunogen composition has been found to be particularly advantageous for developing rapid, high levels of immunity when delivered non- mucosally and with fewer administrations than has traditionally been the case with conventional multiple injection regimens. In one embodiment, sufficient immunization is achievable with only a single administration of the immunogen composition.
- the invention provides a method for delivering the immunogen composition to a host.
- a method for administering an antigen to a host to induce a systemic immune response comprises administering the immunogen composition to a host by injection.
- a method for administering an antigen to a host to induce a mucosal immune response comprises administering the immunogen composition to a host, preferably by intranasal administration, such as from a nebulizer, syringe, catheter, bulb or other device.
- the composition is administered in the form of a flowable medium in which at least the polymer, and optionally also the antigen, is dissolved in the liquid carrier.
- the immunogen composition converts to a gel form, which is substantially not flowable, inside the host following administration. This is accomplished, for example, when the polymer, as formulated in the composition, exhibits reverse-thermal gelation properties with a reverse- thermal liquid-gel transition temperature that is at or below the physiologic temperature of the host.
- a host is administered one or more, but preferably only one, mucosal administration after having already received a systemic administration of the same antigen in the same or different composition, with the mucosal administrations) eliciting a mucosal immune response sufficient to provide the host with mucosal immunity to at least one pathogen without disturbing the integrity of the mucosal membrane.
- the host is administered one or more mucosal applications of the immunogen composition to elicit an immune response without having previously received a systemic administration. This is particularly advantageous for replacement of injection regimens for hosts that are being initially immunized, and to also provide the hosts with both systemic and mucosal immunity.
- the invention provides a method for manufacturing an immunogen composition in which the antigen is dissolved in or dispersed throughout a solution of the polymer dissolved in the liquid vehicle.
- the present invention provides a method for packaging and storing an antigen in the protective environment of the immunogen composition. Handling and storage may be in a gel or liquid form, as desired.
- Figure 1 is a graph of IgA anti-tetanus toxoid (TT) antibody response measured in the lung and nasal washes of inbred mice immunized intraperitoneally (i.p.) with 1.5 Lf TT in PBS at day 0 and boosted intranasally (i.n.) 4 weeks later with 1.5 Lf TT/F127/chitosan or F127/chitosan without TT (vehicle control). A group of mice is also immunized and boosted i.p with 1.5 Lf TT in PBS as a control.
- Figure 2 is a graph of IgA anti-TT antibody response measured in the lung and nasal washes of inbred mice immunized i.n. three times with 1.5 Lf TT in either PBS or F127/chitosan.
- Figure 3 is a graph of the IgG anti-TT antibody response over time in sera of inbred mice immunized i.p. at day 0 with 1.5 Lf TT in PBS and subsequently boosted i.n. four weeks later with 1.5 Lf TT in either PBS or F127/chitosan.
- Figure 4 is a graph of the IgG anti-TT antibody response over time in sera of inbred mice after i.n. immunization at week 0 followed by i.n. booster immunization at weeks 1 and 3 with TT in various formulations.
- Figure 5 is a graph of the IgG anti-TT antibody response over time in sera of inbred mice immunized i.p. at day 0 with 1.5 Lf TT in PBS and subsequently boosted i.n. four weeks later with 1.5 Lf TT in either F127/chitosan or chitosan alone.
- Figure 6 is a graph of the IgG anti-TT antibody response over time in sera of inbred mice immunized once subcutaneously (s.c.) with 1.5 Lf TT in various formulations.
- Figure 7 is a graph of IgG anti-TT antibody response in outbred mice over time after a single s.c. immunization with TT in F127/chitosan or mixed with chitosan only or after three s.c. immunizations with TT adsorbed to aluminum salts (alum).
- Figure 8 is a graph of the antibody response in outbred mice 4 weeks after a single s.c. injection of 1.5 Lf TT in various formulations.
- Figure 9 is a graph of the IgG anti-chicken ovalbumin (OVA) antibody response in inbred mice after one s.c. immunization with either 1 milligram (mg) or 0.1 mg of OVA in either F127/chitosan or PBS.
- OVA IgG anti-chicken ovalbumin
- Figure 10 is a graph of the IgG anti- ONA antibody response in inbred mice after two s.c. immunizations with either 1 mg or 0.1 mg of ONA in either F127/chitosan or PBS.
- Figure 11 is a graph of the IgG anti-diphtheria toxoid (DT) antibody response in outbred mice after a single s.c. immunization with 5 Lf DT in either DT/ F127/chitosan ( ⁇ ) or DT/ PBS (A).
- DT IgG anti-diphtheria toxoid
- Figure 12 is a graph of survival of inbred mice over an eight day period after being immunized once i.p. with 0.5 Lf TT in F127/chitosan or in PBS and then challenged 6 weeks later i.p. with 100 x LD 50 of tetanus toxin.
- transition temperature and “liquid-gel transition temperature” each refer to a temperature at which, or a temperature range across which, a material, such as a biocompatible polymer or the immunogen composition as the case may be, changes physical from a liquid form to a gel, or vice versa.
- thermal gelation property refers to a property of a material, such as the polymer or the immunogen composition as the case may be, to change physical form from a liquid to a gel, or vice versa, due to a change in temperature.
- reverse-thermal gelation property refers to a property of a material, such as the polymer or the immunogen composition as the case may be, to change from a liquid to gel form as the temperature is raised from below to above a transition temperature.
- reverse thermal viscosity property and “reverse thermal viscosity behavior” each refer to a property of a material, such as the polymer or the immunogen composition as the case may be, to undergo a viscosity increase with increasing temperature across at least some temperature range.
- reverse-thermal gelation polymer refers to a polymer capable of interacting with a liquid vehicle so that the polymer/liquid vehicle combination exhibits a reverse-thermal gelation property at least at some proportions of the polymer and the liquid vehicle.
- antigen refers to any material that is capable under appropriate conditions of causing an immune response in a host. Exemplary antigens include polypeptides, peptides, proteins, glycoproteins and polysaccharides that are obtained from animal, plant, bacterial, viral, protozoan and parasitic sources or are produced by synthetic methods, including epitopes of proteins.
- immunogen and “immunogen composition” as used herein refer to a composition formulated with an antigen for administration to a host in order to elicit an immune response in the host.
- a “penetration enhancer” refers to any substance or material that assists or aids in the uptake of a drug across a mucosal surface.
- a “penetration enhancer” assists in moving an antigen across a cellular membrane increasing the likelihood of the antigen reaching its target.
- an “adjuvant” refers to any substance or material that assists or aids the performance of a drug.
- an “adjuvant” is a material that nonspecifically enhances or stimulates an immune response to the antigen.
- mucosal immunity and “mucosal immune response” each means an immune response that is generated at least at one mucosal site (e.g. sublingual, buccal, oral, aural, ocular, intranasal, gastrointestinal, pulmonary, vaginal or rectal).
- biocompatible means not having toxic or injurious effects on biological function in a host.
- nebulization means formation, in any manner and by any technique, of a spray or mist of dispersed droplets, such as droplets including the immunogen composition of the present invention, and a “nebulizer” is any apparatus capable of producing such a spray or mist.
- “Spray” and “mist” are used interchangeably to refer to a dispersion of fine droplets or particles in a carrier gas.
- the carrier gas may be any gas, such as for example air or a non-air propellant gas exiting a nebulizer.
- bioadhesive means having an affinity to adhere to a biological surface, such as for example mucous membranes or other tissues, for an extended period of time.
- the immunogen composition of the present invention typically includes at least one antigen, at least one biocompatible polymer, and at least one liquid vehicle and exhibits reverse thermal viscosity behavior over at least some temperature range.
- the immunogen composition may optionally also include other components that may enhance performance of the composition.
- the immunogen composition is in the form of a flowable medium, while in another embodiment the immunogen composition is in the form of a gel. In either case, the antigen should be homogenously dispersed throughout the composition.
- the immunogen composition is capable of converting from the gel form to the flowable medium form, and vice versa, by a change in temperature across a reverse-thermal liquid-gel transition temperature, so that the immunogen composition is in the form of a flowable medium below the transition temperature and a gel form above the transition temperature.
- a medium is "flowable", when it has sufficiently low viscosity to be syringable and/or nebulizable, depending upon the specific application.
- a flowable medium may, for example, be in a liquid form, or may include a liquid in which fine particulate material is suspended, with the medium retaining sufficient fluidity to be syringible and/or nebulizable.
- the biocompatible polymer When the immunogen composition is in the flowable medium form, the biocompatible polymer will typically be substantially all dissolved in the liquid vehicle, and the antigen will also preferably be substantially all dissolved in the liquid vehicle along with the biocompatible polymer. Alternatively, some or all of the antigen may be in the form of a fine particulate, such as a fine precipitate, dispersed throughout the biocompatible polymer/liquid vehicle solution. When present, other components are dissolved in the liquid vehicle or are otherwise preferably uniformly dispersed throughout the composition. When the immunogen composition is in a gel form, the antigen, and other components, when present, will preferably be uniformly dispersed throughout the gel.
- the immunogen composition of the present invention is useful for delivering an antigen to a host to treat or prevent an infectious disease.
- a microbial infection can be prevented by administering an antigen corresponding to that organism to a host animal as a vaccine to elicit a protective immune response.
- the host is typically a mammal, and more typically a human.
- the immunogen composition can be used for the treatment of cancers such as those caused by human papilloma virus.
- the immunogen composition can be used to alter the mammalian reproductive cycle.
- Antigens useful in the immunogen composition of the present invention include antigens from bacteria, protozoa and viruses that invade their host via a mucosal surface.
- antigens from rotavirus hookworm, Neisseria meningitiditis, Streptococcus pneumoniae, Bordatella pertussis, M. tuberculosis, Epstein-Ban virus, Hepatitis C virus, HIN, influenza and tumor-specific antigens, tetanus toxoid, diphtheria toxoid and other non-pathogenic mutants of these toxins, other toxins or non-pathogenic versions of these toxins that cause disease such as anthrax toxic complex, polysaccharides or peptide mimetics of polysaccharides from Neisseria meningitiditis, or Streptococcus pneumoniae.
- the antigen is selected from the group consisting of tetanus toxoid, diphtheria toxoid, and other non-pathogenic mutants of these toxins, other toxins or non-pathogenic versions thereof that cause disease such as anthrax toxic complex, antigens from Bordatella pertussis, rotavirus, hookworm, M.
- tuberculosis Epstein-Ban virus, Hepatitis C virus, HIN, Neisseria meningitiditis, Streptococcus pneumoniae, polysaccharides or peptide mimetics of polysaccharides from Neisseiria meningitiditis, or Streptococcus pneumoniae, antigens from other blood-borne pathogens, tumor-specific antigens and antigens from viruses or bacteria against which vaccines are currently available.
- the antigen is selected from the group consisting of tetanus toxoid, diphtheria toxoid and other mutants of these toxins, anthrax toxic complex, antigens from Bordatella pertussis, M.
- the immunogen composition may include two or more antigens.
- one prefened immuogen composition includes tetanus toxoid (or a non-pathogenic mutant of tetanus toxoid) and diphtheria toxoid (or a non-pathogenic mutant of diphtheria toxoid).
- the amount of antigen in the immunogen composition of the present invention varies depending on the nature and potency of the antigen. Typically, however, the amount of antigen present in the immunogen composition of the present invention is from about 0.000001% by weight of the immunogen composition to about 5% by weight of the immunogen composition, more typically from about 0.0001% by weight to about 5% by weight, and more typically from about 0.005% by weight to about 5% by weight.
- the amount of tetanus toxoid present in the immunogen composition is typically from about 0.0001% by weight to about 0.05% by weight, preferably from about 0.0005% by weight to about 0.01% by weight, and more preferably from about 0.0005% by weight to about 0.003% by weight.
- the immunogen composition of the present invention provides a delivery system that typically elicits stimulation of an immune response, which will typically include a systemic immune response when the immunogen composition is administered for systemic delivery of the antigen.
- the immunogen composition of the present invention provides a delivery system that elicits stimulation of a strong immune response, which will typically include both a strong systemic immune response and a strong mucosal immune response when the immunogen composition is administered for mucosal delivery of the antigen. Furthermore, the immunogen composition when administered for mucosal delivery can act as a boost to an existing immune response. Without being bound by any theory, it is believed that the immunogen composition of the present invention reduces or eliminates degradation of the antigen and allows for a relatively slow sustained administration of antigens to the host. The antigen is at least partially protected by the biocompatible polymer, thereby reducing susceptibility of the antigen to degradation and promoting increased effectiveness of the antigen.
- the immunogen composition of the present invention promotes improved bioadhesion onto and permeation into and across the mucous membrane, or mucosa, thus allowing the immunogen composition to exert its actions more efficaciously at the target site.
- the immunogen composition includes an adjuvant and/or penetration enhancer that further enhances performance.
- stabilizing agents may be incorporated into the immunogen composition to further reduce the susceptibility of the antigen to degradation, tending to further enhance the effectiveness of the immunogen composition to stimulate mucosal immunity and to also enhance stability of the antigen during storage and transportation of the composition.
- the biocompatible polymer in the immunogen composition of the present invention typically is a reverse-thermal gelation polymer.
- the biocompatible polymer is selected and the immunogen composition is formulated with relative proportions of the liquid vehicle and the biocompatible polymer so that the immunogen composition exhibits reverse-thermal viscosity behavior across at least some temperamre range, preferably a temperature range below 40 °C, more preferably a temperature range below 37 °C and even more preferably a temperature range within a range of from 10 °C to 37 °C.
- the immunogen composition exhibits reverse-thermal viscosity behavior over some temperature range within a range of 1°C to 20 °C.
- the immunogen composition can be administered to the host at a cooler temperature where the composition has a lower viscosity, with the viscosity of the composition then increasing in the host following administration, whereby the mobility of the composition is severely reduced within the host following administration.
- the immunogen composition has a reverse thermal gelation property
- the immunogen composition will exist in the form of a flowable medium at least at a first temperature and in the form of a gel at least at a second temperature that is higher than the first temperamre.
- both the first and second temperatures are below 40 °C, and more preferably the second temperature is no higher than 37 °C.
- a prefened situation is when the first temperature is in a range of 1 °C to 20 °C and the second temperature is in a range of 25 °C to 37 °C.
- the immunogen composition is formulated with relative proportions of liquid vehicle and biocompatible polymer so that the immunogen composition has a reverse-thermal gelation property, preferably with a reverse-thermal liquid-gel transition temperature so that when the immunogen composition is administered to a host, the biocompatible polymer and also the immunogen composition becomes a gel or gelatinous in vivo, thus reducing or eliminating degradation of the antigen and/or achieving the ability for slow release, i.e., sustained administration, of the antigen for a time period of many hours, days, weeks or even months, depending upon the specific application.
- any biocompatible polymer may be used that, as formulated in the immunogen composition, is capable of interacting with the liquid vehicle to impart the desired reverse- thermal viscosity behavior to the immunogen composition.
- some reverse-thermal gelation polymers useful for preparing the immunogen composition include certain polyethers (preferably polyoxyalkylene block copolymers with more prefened polyoxyalkylene block copolymers including polyoxyethylene-polyoxypropylene block copolymers refened to herein as POE-POP block copolymers, such as PluronicTM F68, PluronicTM F127, PluronicTM L121, and PluronicTM LlOl, and TetronicTM T1501); certain cellulosic polymers, such as ethylhydroxyethyl cellulose; and certain poly (ether-ester) block copolymers (such as those disclosed in U.S.
- polystyrene resin polystyrene resin
- PluronicTM and TetronicTM are trademarks of BASF Corporation.
- more than one of these and/or other biocompatible polymers may be included in the immunogen composition to provide the desired characteristics and other polymers and/or other additives may also be included in the immunogen composition to the extent the inclusion is not inconsistent with performance requirements of the immunogen composition.
- these polymers may be mixed with other polymers or other additives, such as sugars, to vary the transition temperature, typically in aqueous solutions, at which reverse-thermal gelation occurs.
- Polyoxyalkylene block copolymers are particularly prefened to use as the biocompatible reverse-thermal gelation polymer.
- a polyoxyalkylene block copolymer is a polymer including at least one block (i.e.
- POE-POP block copolymers are one class of prefened polyoxyalkylene block copolymers for use as the biocompatible reverse-thermal gelation polymer in the immunogen composition.
- POE-POP block copolymers include at least one block of a polyoxyethylene and at least one block of a polyoxypropylene, although other blocks may be present as well.
- the polyoxyethylene block may be represented by the formula (C 2 H 4 0) b when b is an integer.
- the polyoxypropylene block may be represented by the formula (C 3 HeO) a when a is an integer.
- the polyoxypropylene block could be for example (CH 2 CH 2 CH 2 O) a , or could be
- POE-POP block copolymers are known to exhibit reverse-thermal gelation properties, and these polymers are particularly preferred for imparting reverse-thermal gelation properties to the immunogen composition of the present invention.
- Examples of POE-POP block copolymers include PluronicTM F68, PluronicTM F127, PluronicTM L121, PluronicTM LlOl, and TetronicTM T1501.
- TetronicTM T1501 is one example of a POE-POP block copolymer having at least one polymer segment in addition to the polyoxyethylene and polyoxypropylene segments.
- TetronicTM T1501 is reported by BASF Corporation to be a block copolymer including polymer segments, or blocks, of ethylene oxide, propylene oxide and ethylene diamine.
- biocompatible polymers may now or hereafter exist that are capable of imparting the desired reverse-thermal viscosity behavior and/or reverse-thermal gelation properties for the immunogen composition of the present invention, and such polymers are specifically intended to be within the scope of the present invention when incorporated into the immunogen composition.
- Some prefened POE-POP block copolymers have the formula:
- a particularly prefened POE-POP block copolymer for use with the present invention has the following formula: HO(CH 2 CH 2 O) b (CH 2 (CH 3 )CHO) a (CH 2 CH 2 0) b H II wherein a and b are integers such that the hydrophobe base represented by (CH 2 (CH 3 )CHO) a has a molecular weight of about 4,000, as determined by hydroxyl number; the polyoxyethylene chain constituting about 70 percent of the total number of monomeric units in the molecule and where the copolymer has an average molecular weight of about 12,600.
- PluronicTM F-127 also known as Poloxamer 407, is such a material.
- PluronicTM F-68 may also be used.
- the procedures used to prepare aqueous solutions which form gels of polyoxyalkylene block copolymer are well known and are disclosed in U.S. Patent No. 5,861,174, which is incorporated herein by reference in its entirety.
- the relative proportions of the liquid vehicle and the biocompatible polymer, as formulated in the immunogen composition should be selected so that the resulting immunogen composition has reverse- thermal gelation properties with a reverse-thermal liquid-gel transition temperature of less than about 37 °C, preferably between about 10 °C and 37 °C, and more preferably between about 20 °C to about 37 °C.
- the amount of biocompatible polymer in the immunogen composition of the present invention is typically from about 1% by weight to about 50% by weight of the immunogen composition, preferably from about 8% by weight to about 33% by weight, and more preferably from about 13% by weight to about 25% by weight.
- the immunogen composition includes an additive that is an adjuvant and/or a penetration enhancer.
- a single compound may act both as a penetration enhancer and an adjuvant when incorporated into the immunogen composition.
- chitosan is a polysaccharide derived from deacetylation of chitosan.
- chitosan materials include chitosan, derivatives of chitosan and other derivatives originating from chitin that provide adjuvant and/or penetration enhancer properties similar to chitosan.
- the use of chitosan material as a combined penetration enhancer/adjuvant is especially preferred when the immunogen composition is administered mucosally.
- Non-limiting examples of penetration enhancers include various molecular weight chitosan materials, such as chitosan and N,0-carboxymethyl chitosan; poly-L-arginines; fatty acids, such as lauric acid; bile salts such as deoxycholate, glycolate, cholate, taurocholate, taurodeoxycholate, and glycodeoxycholate; salts of fusidic acid such as taurodihydrofusidate; polyoxyethylenesorbitan such as TweenTM 20 and TweenTM 80; sodium lauryl sulfate; polyoxyethylene-9-lauryl ether (LaurethTM-9); EDTA; citric acid; salicylates; caprylic/capric glycerides; sodium caprylate; sodium caprate; sodium laurate; sodium glycynhetinate; dipotassium glycyrrhizinate; glycynhetinic acid hydrogen succinate, disodium salt (Carbenox
- the penetration enhancer is selected from the group consisting of chitosan materials, and fatty acids, polyethylene sorbitol and caprylic/capric glycerides. More preferably, the penetration enhancer is selected from the group consisting of chitosan materials, fatty acids and caprylic/capric glycerides. Particularly preferred as the penetration enhancers are the chitosan materials.
- a "penetration enhancer" is any substance or material that, when added to a formulation including an active agent, such as the antigen in the immunogen composition, enables or enhances permeation of the active agent across biological membranes thereby increasing absorption and systemic bioavailability of the active agent.
- the penetration enhancer enables or enhances permeation of the active agent across the mucosal epithelium where the active agent is to be delivered.
- adjuvants for use in the immunogen composition include those materials that exhibit adjuvantic properties in mucosal tissues including chitosan materials, bacterially derived products such as monophosphoryl lipid A, CpG motifs, detoxified mutants of CT and ET, and outer membrane proteins of Neisseria meningitidis serogroup b.
- adjuvants for use in the immunogen composition include those materials that exhibit adjuvantic properties in non-mucosal tissues including dimethyl dioctadecyl ammonium bromide (DDA), CpG motifs, cytokines such as IL-12 and IL-6, as well as chitosan materials.
- DDA dimethyl dioctadecyl ammonium bromide
- CpG motifs CpG motifs
- cytokines such as IL-12 and IL-6
- chitosan materials include those materials that exhibit adjuvantic properties in non-mucosal tissues including dimethyl dioctadecyl ammonium bromide (DDA), CpG motifs, cytokines such as IL-12 and IL-6, as well as chitosan materials.
- the amount of penetration enhancer and/or adjuvant in the immunogen composition of the present invention generally varies depending on the particular additive(s) used.
- a typical amount of penetration enhancer present in the immunogen composition of the present invention is from about 0.001% by weight to about 10% by weight of the immunogen composition, preferably from about 0.01% by weight to about 5% by weight, and more preferably from about 0.01% by weight to about 1.0% by weight.
- the amount of the chitosan or chitosan material present in the immunogen composition is typically from about 0.01% by weight to about 10% by weight of the immunogen composition, preferably from about 0.1% by weight to about 1% by weight, and more preferably from about 0.1% by weight to about 0.5% by weight.
- the immunogen composition comprises from 60 weight percent to 85 weight percent of the liquid vehicle, from 0.0001 weight percent to 5 weight percent of the antigen and from 0.01 weight percent to 1.0 weight percent of at least one of the adjuvant an/or penetration enhancer additive.
- the immunogen composition of the present invention can also include other additives besides adjuvant and/or penetration enhancer.
- the immunogen composition can include polymer or protein stabilizers such as trehalose, sucrose, glycine, mannitol, albumin, and glycerol.
- any suitable liquid vehicle can be used that is capable of interacting with the biocompatible polymer to impact the desired reverse thermal viscosity behavior.
- the biocompatible polymer, and also preferably the antigen is soluble in the liquid vehicle at least at a temperature at which the immunogen composition is in the form of a flowable medium suitable for administration.
- the adjuvant and/or penetration enhancer are also preferably soluble in the liquid vehicle in the flowable medium form suitable for administration.
- the immunogen composition is typically prepared in water, a saline solution or other aqueous liquid as the liquid vehicle, although any solvent, including mixtures of multiple solvent liquids, can be used, depending upon the specific circumstances of the application.
- the immunogen composition may also contain a preservative to prevent the growth of microorganisms
- the immunogen composition is sterile, and is fluid, i.e., in the form of a flowable liquid or suspension, when administered to accommodate easy syringability and/or nebulization.
- the immunogen composition should preferably be stable under the conditions of manufacture and storage and should also preferably be preserved against the contaminating action of microorganisms such as bacteria and fungi.
- the liquid vehicle can be a solvent or dispersion medium containing, for example, water, ethanol, polyol (e.g., glycerol, propylene glycol, and liquid polyethylene glycol, and the like), and suitable mixtures thereof.
- microorganisms can be brought about by various antibacterial and antifungal agents, for example, parabens, chlorobutanol, phenol, sorbic acid, thimerosal, and the like.
- antibacterial and antifungal agents for example, parabens, chlorobutanol, phenol, sorbic acid, thimerosal, and the like.
- isotonic agents e.g., sugars, phosphate buffers, sodium chloride, or mixtures thereof.
- antigen-stabilizing solutes are incorporated into the immunogen composition.
- protein-stabilizing solutes such as sucrose
- protein-stabilizing solvents permits the composition to exhibit desired reverse-thermal gelation behavior at lower polymer concentration and/or at an altered reverse-thermal gelation temperature than when the protein-stabilizing is not used, especially when using the prefened polyalkoxyalkylene block copolymers.
- the working range of polymer concentration can be widened and the transition temperature modified.
- the transition temperature may be manipulated, while also lowering the concentration of polyoxyethylene-polyoxypropylene block copolymer that is necessary to form a gel.
- prefened protein-stability solvents are sugars, such as, for example, sucrose.
- the immunogen composition of the present invention is particularly effective for stimulating or upregulating a antibody response to a level greater than that seen with conventional formulations and administration schedules. More preferably the immunogen composition of the present invention, upon administration, stimulates a systemic immune response that protects the host from at least one pathogen. Most preferably the immunogen composition of the present invention, upon administration, stimulates a systemic and mucosal immune response that protects the host from at least one pathogen.
- a immune response involves generation of one or more antibody classes, such as IgM, IgG and/or IgA, and typically for mucosal responses at least IgA.
- the invention provides a method for delivery of an antigen to a host to stimulate an immune response in the host.
- the method involves administering the immunogen composition of the present invention to the host, which is usually accomplished by introducing the immunogen composition into the host in a manner to stimulate a desired immune response.
- the immunogen composition can be introduced into the host by any suitable technique.
- the immunogen composition is introduced into the host by injection, such as, for example, subcutenously, intramuscularly, or intraperitoneally.
- the injection may be accomplished using any suitable injection device, such as, for example, a syringe.
- the immunogen composition is introduced into the host for delivery of the antigen via a mucosal route.
- the immunogen composition is introduced into the host in a manner so that at least a portion, and preferably most or all, of the administered immunogen composition contacts a mucosal surface within the host. At least a portion, and more preferably at least a significant portion, of the immunogen composition adheres to the mucosal surface, thereby retaining the antigen, and also any adjuvant and/or penetration enhancer in the vicinity of the mucosal surface to promote uptake of the antigen across the mucosal surface.
- the immunogen composition should be in the form of a flowable medium immediately prior to introduction of the immunogen composition into the host. This will typically require that the immunogen composition be at a temperature that is lower than the physiologic temperature of the host. In the case of a human host, having a physiologic temperature of 37 °C, the temperature of the immunogen composition immediately prior to administration will frequently be 25 °C or less and more often 20°C or less. In most instances, the temperature of the immunogen composition immediately prior to introduction into the host will be in a range of from about 1°C to about 20 °C.
- the immunogen composition After introduction into the host, the immunogen composition is warmed to the physiologic temperature of the host and, due to the reverse-thermal viscosity behavior of the immunogen composition, the viscosity of the immunogen composition increases inside the host as the temperature of the immunogen composition increases.
- the immunogen composition has a reverse-thermal liquid-gel transition temperature between the temperature of administration and the physiologic temperature of the host, then the immunogen composition will convert from the form of a flowable medium to a gel form inside the host following administration.
- the reverse-thermal gelation property of the immunogen composition is advantageous to permit easy administration of the immunogen composition to the host as a flowable medium and the viscosity then advantageously increases after administration at least partially to immobilize the immunogen composition at the location where delivery of the antigen is desired.
- This is particularly advantageous when the antigen is to be delivered via a mucosal route, because the high viscosity/gel nature of the immunogen composition following administration causes the immunogen composition to readily adhere to mucosal surfaces, so that the immunogen composition, including the antigen and any additives are retained in the vicinity of the mucosal surface to facilitate delivery of the antigen across the mucosal surface.
- the immunogen composition may be directed to contact any desired mucosal surface to permit delivery of at least a portion of the antigen across the mucosal epithelium at that location to elicit an immune response.
- the mucosal surface may, for example, be a sublingual, buccal, oral, intranasal, gastrointestinal, pulmonary, vaginal, rectal, aural, or ocular mucosal surface.
- the immunogen composition is introduced into the host in the form of a mist containing a dispersion of fine droplets of the immunogen composition.
- the mist will be produced by a nebulizer actuatable to produce the mist.
- a nebulizer actuatable to produce the mist.
- one prefened mucosal delivery route is intranasal and the mist could be generated by a nasal nebulizer.
- the spray is directed into the nasal cavity to introduce the immunogen composition into the host to contact a mucosal surface within the nasal cavity.
- the biocompatible polymer, and preferably also the antigen and any adjuvant and/or penetration enhancer are dissolved in the liquid vehicle.
- the composition gels within the host, at least a portion of the polymer, and potentially also some or all of the antigen and other additives come out of solution.
- a method for packaging and storing the immunogen composition.
- the immunogen composition is placed in a container when the composition is in the form of a flowable medium.
- the temperature of the composition is then raised so that the immunogen composition converts to a gel form within the container for storage.
- the immunogen composition in the container can be converted back to a flowable medium for administration to the host at the appropriate time by lowering the temperature of the composition in the container.
- the immunogen composition is easy to handle during manufacturing and packaging operations, but can be stored in the highly stable form of a gel.
- the composition can be converted back to a flowable medium for ease of administration.
- the immunogen composition be stored at a temperature below the transition temperature.
- the immunogen composition may be stored in a gel form above the transition temperature and then cooled to below the transition temperature prior to administration. This ability to store the antigen in a gel form of the immunogen composition prior to use is a distinct advantage with the present invention.
- the immunogen composition could be stored in the form of a flowable medium at a temperature below the reverse-thermal liquid-gel transition temperature, but such a fluid form is often not as convenient for handling and storage as a gel form. In either case, the immunogen composition is advantageous for storing the antigen in a highly protective environment prior to use.
- a method for making the immunogen composition comprising dissolving the biocompatible polymer in a liquid vehicle and suspending or codissolving the antigen in the liquid vehicle.
- both the antigen and the biocompatible polymers are dissolved in the liquid vehicle.
- the present invention has been described primarily with reference to the immunogen composition.
- the principles discussed with respect to formulation, manufacture, storage, and administration of the immunogen composition apply equally to the delivery of other drugs.
- the aspects of the present invention as described above can be applied to formulate, prepare, restore, and administer a delivery vehicle composition for delivering any drug in a therapeutically effective amount for treatment of at least one condition in the host.
- the delivery vehicle includes at least the drug, the biocompatible polymer and the liquid vehicle, with the proportions of the liquid vehicle and the biocompatible polymer being such that the delivery vehicle composition exhibits reverse-thermal viscosity behavior, and preferably, a reverse-thermal gelation property, as discussed above specifically with respect to the immunogen composition.
- the delivery vehicle composition includes as an additive at least one of an adjuvant and a penetration enhancer for the drug to be delivered.
- Tetanus Toxoid (TT) solution was obtained (Accurate Chemical, Accurate & Scientific Corp., Westerbury, NY) containing 961 Lf TT per mL of solution and 1884 Lf TT per mg of protein nitrogen.
- Pluronic ® F127 BASF, Washington, NJ
- Stock solution was prepared at 30 or 34%(w/w) by dissolving the polymer ⁇ in ice-cold phosphate buffer solution (PBS) with complete dissolution achieved by storing overnight at 4°C.
- PBS ice-cold phosphate buffer solution
- mice Balb/c mice, 6-8 weeks of age (Taconic Farms Incorp., Germantown, N.Y.), were used for the study. Intranasal immunization was performed under anesthesia with Ketamine/Xylazine 80mg/16mg/kg.
- Nasal and pulmonary IgA anti-TT antibody assays Post mortem lung washes were obtained by gently injecting 300 ⁇ L of cold solution consisting of 5mM EDTA, 0.5 % gelatin, 0.05% TweenTM 80 in PBS into the lungs through a syringe connected to the trachea. The lavage fluid was aspirated and the procedure was repeated once (total of 600 ⁇ L is collected). Nasal washes were performed by injection of 300 ⁇ L cold solution as above retrograde via the trachea into the nasopharynx. The lavage fluid was collected at the nostrils. The IgA anti-TT antibody response was determined by ELISA.
- IgA anti-TT antibody response in lung and nasal washes after i.n. boost Mice were primed intraperitoneally (i.p.) with 1.5 Lf TT in PBS. Four weeks later they were boosted intranasally (i.n.) with either 1.5 Lf TT formulated in F127/chitosan or a formulation of F127/ chitosan alone (vehicle control) or boosted i.p. with 1.5 Lf TT in PBS (control).
- the secretory IgA anti-TT antibody titers in lung washes and nasal secretions were measured at week 10 (6 weeks after boosting).
- Figure 1 is a bar graph showing average reciprocal titer IgA levels in lung and nasal washes for test conditions summarized in Table 1.
- Balb/c mice were immunized i.n. at week 0 and boosted i.n. at weeks 1 and 3 with 1.5 Lf TT in PBS (controls) or 1.5 Lf TT formulated with F127/ chitosan.
- IgA anti-TT antibody levels were measured by ELISA, as described for Example 1, at 4 weeks (i.e. one week after the final boost injection).
- Figure 2 is a bar graph showing average reciprocal titer IgA anti-TT antibody levels in lung and nasal washes for test conditions using the formulations summarized in Table 2.
- mice used in this example were the same as those used in Example 1, except as specifically noted.
- Measurement of IgG antibody responses in sera The serum antibody response to TT was measured by ELISA on a weekly basis. Sera was obtained by tail vein bleeding and stored at -20°C until assay. Wells of 96 well Maxisorb microtiter plates were coated with 100 ⁇ l of 1 ⁇ g/ml TT in PBS overnight at 4°C. Plates were washed with PBS/0.05% Tween 20 and blocked with 200 l of 1 % bovine serum albumin (BSA) (Fisher Scientific) in ultrapure water for 2 hr at 37°C.
- BSA bovine serum albumin
- Serum samples were serially diluted in PBS with 0.1% BSA/0.05% Tween 20, 50 ⁇ l of sample was added per well. Following incubation overnight at 4°C, plates were washed and horseradish peroxidase-labeled anti-mouse IgG ⁇ D chain-specific antibody conjugate (Southern Biotechnology Associates, Inc.) was added diluted to 1:3000 in PBS with 0.1% BSA and 0.05% Tween 20. The plates were incubated for 2 hr at 37°C and antibody binding was detected with substrate buffer containing 0.02% o-phenylenediamine (Sigma-Aldrich). Absorbance was read at 450 nm with an EIA reader (Bio-Tek Instruments).
- Immunoglobulin titers are calculated as follows. For serum antibodies the titer is defined as the reciprocal of the dilution that would yield an optical density of 0.5. Geometric mean titers, averages and standard deviations are calculated using Microsoft Excel. Mann Whimey U is used to calculate statistical difference between titers of groups, values are significant when P ⁇ 0.05.
- IgG anti-TT antibody response in sera after i.n. boost mice were primed i.p. with 1.5 Lf TT in PBS at week 0 and boosted i.n. at week 4 with 1.5 Lf TT in PBS or in F127/chitosan.
- the serum IgG anti-TT antibody response was analyzed on a biweekly basis for 10 weeks.
- a group of mice was both primed and boosted i.p. with 1.5 Lf TT in PBS.
- the results of the IgG anti-TT response from 4 weeks (pre-boost) to 10 weeks (6 weeks post-boost) is shown in Figure 3.
- the IgM anti-TT antibody response is not shown as it was present in all groups, in equal amounts and comprises ⁇ 10% of the immune response.
- the IgG anti-TT response of the mice boosted i.n. with TT in PBS is not significantly statistically different from the negative controls, i.e. mice boosted i.n. with vehicle.
- mice boosted i.n. with TT in F127/chitosan manifested an IgG anti-TT antibody response significantly higher than all negative controls and the animals boosted i.n. with TT in PBS.
- IgG anti-TT antibody response in sera to intranasal immunization and boost.
- the IgG antibody response to i.n. immunization and booster was assessed by treating groups of Balb/c mice via i.n. immunization at week 0 followed by i.n. booster immunization at weeks 1 and 3.
- the IgG anti-TT responses of mice immunized and boosted i.n. with TT in PBS, TT in F127/chitosan and TT in F127/LPC were compared. The results of these studies are shown in Figure 4 and indicate that the animals treated i.n. with TT in PBS failed to generate a significant anti-TT immune response, with a geometric mean titer of 159.6.
- the group immunized with TT in F127/LPC had a measurable anti-TT IgG response with a geometric mean titer of 544.
- the group immunized with TT in F127/chitosan clearly demonstrated a significant systemic anti-TT IgG response with a geometric mean titer >5000.
- Example 3 As shown in Figure 6, the combination of TT/F127/chitosan elicited a very long- lasting antibody response with titers persisting at levels above 90,000 for at least 10 months.
- Serum samples were collected at weeks 1, 2, 4 and 8 and analyzed for the presence of IgG anti-DT antibodies by ELISA as described in Example 3 except that 1 ug/ml DT was used to coat the wells of microwell plates.
- the IgG anti-DT antibody response looked similar to that of TT inasmuch as the IgG appeared rapidly (within one week) and continued to increase rapidly for at least 4 weeks after a single immunization (see Figure 11).
- mice Protection of mice from lethal challenge with tetanus toxin.
- mice were challenged i.p. with 100 x LD 50 tetanus toxin (List Biological Laboratories Inc., Campbell, CA).
- Figure 12 shows the percent survival over an eight day period following challenge. Mice receiving TT/F127/chitosan were completely protected against this otherwise lethal challenge with 8 out of 8 mice surviving whereas all 8 animals in the TT/PBS group succumbed. Therefore protective immunity was induced by TT/F127/chitosan immunization.
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AU2001276831A AU2001276831A1 (en) | 2000-06-22 | 2001-06-22 | Delivery vehicle composition and methods for delivering antigens and other drugs |
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EP1494633A4 (en) * | 2002-03-28 | 2005-09-28 | Chitogenics Inc | Adherent n,o-carboxymethylchitosan drug delivery devices for moist tissue and methods of their use |
US7588774B2 (en) | 2003-05-12 | 2009-09-15 | Becton, Dickinson And Company | Molecules enhancing dermal delivery of influenza vaccines |
EP2699318A1 (en) * | 2011-04-18 | 2014-02-26 | University Of Georgia Research Foundation, Inc. | Vaccine delivery method |
EP2699318A4 (en) * | 2011-04-18 | 2015-04-29 | Univ Georgia | Vaccine delivery method |
US9566338B2 (en) | 2011-04-18 | 2017-02-14 | University Of Georgia Research Foundation, Inc. | Vaccine delivery method |
EP3275507A3 (en) * | 2011-04-18 | 2018-04-18 | University Of Georgia Research Foundation, Inc. | Vaccine delivery method |
US11524072B2 (en) | 2011-04-18 | 2022-12-13 | University Of Georgia Research Foundation, Inc. | Vaccine delivery method |
Also Published As
Publication number | Publication date |
---|---|
EP1315672A4 (en) | 2006-04-26 |
AU2001276831A1 (en) | 2002-01-02 |
US7767197B2 (en) | 2010-08-03 |
EP1315672A1 (en) | 2003-06-04 |
US20020025326A1 (en) | 2002-02-28 |
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