AU2002245636A1

AU2002245636A1 - A novel proteosome-liposaccharide vaccine adjuvant

Info

Publication number: AU2002245636A1
Application number: AU2002245636A
Authority: AU
Inventors: David S. Burt; David Jones; George H. Lowell; Clement Rioux; Gregory L. White
Original assignee: ID Biomedical Corp of Quebec
Current assignee: ID Biomedical Corp of Quebec
Priority date: 2001-03-09
Filing date: 2002-03-11
Publication date: 2003-03-20
Anticipated expiration: 2022-03-11

Description

A NOVEL PROTEOSOME-LIPOSACCHARIDE VACCINE ADJUVANT

FIELD OF INVENTION This invention relates to adjuvants for enhancing the immunogenicity and improvement ofthe immune response of antigens and to methods and compositions for preparing and using them.

BACKGROUND OF THE INVENTION

The ability of antigens to induce protective immune responses in a host can be enhanced by combining the antigen with immunostimulants or adjuvants. Alum-based adjuvants are almost exclusively used for licensed injectable human vaccines, however, while alum enhances certain types of serum antibody responses (Type 2), it is poor at enhancing other types of antibody responses (Type 1) and is a poor activator of cellular immune responses that are important for protection against intracellular pathogens and for therapeutic vaccines for cancer and allergy. Furthermore, alum enhances allergic reactions due to production of IgE. Although numerous substances have been tested and shown to be potent adjuvants for antibody and cellular (Type 1) immune responses in animal models, very few have proved to be suitable for use in humans due to unacceptable levels of reactogenicity and/or disappointing immuno-enhancing abilities. Furthermore, there are currently no licensed adjuvants capable of enhancing immune responses at mucosal surfaces where the majority of infectious agents enter the host. Indeed, development ofthe most promising nasally delivered mucosal adjuvants, the bacterial enterotoxins (e.g. mutated cholera and heat-labile toxins), have been halted in North America due to their ability to be transported to, and cause inflammation in the olfactory bulb region ofthe CNS of rodents. There is a need for potent adjuvants that are safe in humans and capable of inducing protective systemic and mucosal humoral and cellular immune responses.

Lipopolysaccharides (LPS) from gram negative bacteria are potent adjuvants. LPS activates the innate immune system causing production of inflammatory cytokines such as TL- 1 , TNF- D , IL- 10 and IL- 12 from macrophages and dendritic cells; IL- 1 , IL-6 and IL-8 from endothelial cells and TL-8 from epithelial cells. In addition, LPS is a B cell activator in mice and, to a certain extent in humans, as evidenced by B cell mitogenicity and stimulation of polyclonal antibody secretion. LPS mediates it's effects by binding to CD 14 molecules and activation of toll like receptors (TLR) on the surface of antigen presenting cells leading to the initiation of a transcriptional cascade, gene expression and secretion of pro-inflammatory molecules.

Despite the adjuvant potential of LPS, its use in humans has been restricted due to the associated endotoxicity mediated by the lipid A portion ofthe molecule. Chemical modification ofthe lipid A region of LPS was shown to substantially detoxify lipid A (e.g. monophosphoryl lipid A or MPL-A or e.g. alkali-detoxification to remove certain fatty acids) while maintaining certain adjuvant properties (see Qureshi et. al. J. Biol Chem 1982; 257:11808-15). While MPL-A exhibited potent adjuvant activity in animals, the experience in humans has been inconsistent, showing poor adjuvant activity with some antigens and unacceptable reactogenicity overall in many situations.

Non-covalent proteosome-LPS complexes, containing proteosomes from Neisseria meningitidis and purified LPS from Shigella flexneri or Plesiomonas shigelloides, have been administered to humans intranasally and orally in phase 1 and phase 2 clinical trials in the context of stand-alone vaccines. These vaccines induce protective immune responses against Shigella flexneri or S. sonnei infection, respectively, in animals (Mallet et. al. Infect and Immun 1995; 63:2382-86) and humans (Fries et. al. Infect Immun. 2001; 69:4545-53) when given via the intranasal route. Further, these complexes were well- tolerated via the nasal or oral routes in humans at very high doses (up to 1.5 mg of proteosomes along with comparable amounts of LPS given intranasally and up to 2 mg of each ofthe proteosome and LPS components given orally) (Fries et. al. 2000) and showed no olfactory bulb or other CNS associated toxicity in small animal toxicity studies. Proteosomes consist predominantly of porin proteins and other outer membrane proteins. Evidence suggests that proteosome porins may also induce TL-12 from dendritic cells and induction of CD8+ T cells (Jeannin et. al. Nature hrrmunology 2000; 1:502-509) and activation of Hela cells to produce IL-8 (Pridmore et. al. J. Infect Dis 2000; 10:183). Proteosome porins also upregulate B7.2 (CD28) co-stimulatory molecules on antigen presenting cells via the activation ofthe toll-like receptor 2 (Massari et. al. J. Immunol. 2002, 168:1533-1537).

Dalseg et. al. (in Vaccines 96 pp. 177-182 (Cold Spring Harbor laboratory Press, 1996)) report the use of meningococcal outer membrane vesicles (OMV's) as a mucosal adjuvant for inactivated whole influenza virus. Dalseg and his associates and collaborators have reported that the OMV's they prepare employ a process that retains 6% to 9% of endogenous lipoohgosaccharide (LOS) remaining compared to the amount of total OMV protein by weight. These OMV preparations have also been reported to specifically retain 16% of detergent (deoxycholate) in their OMV's, an amount that may be unhealthy or toxic in toxicity studies or in humans.

BRIEF DESCRIPTION OF INVENTION:

The instant invention (IVX-908) describes compositions of and processes for production of novel formulations that are adjuvants for antigens and result in adjuvanted vaccines or immunotherapeutics when the invention and antigen(s) are combined by simple mixing and the adjuvanted vaccines or immunotherapeutics are delivered by a parenteral or mucosal route. The adjuvant consists of two major components. The first component is an outer membrane protein preparation of proteosomes prepared from gram- negative bacteria including, but not limited to Neisseria meningitidis. The second component is a preparation of liposaccharide. Liposaccharide includes native or modified lipopolysaccharide (LPS) and lipoohgosaccharide derived from S. flexneri or Plesiomonas shigelloides or other gram-negative bacteria including, but not limited to, Shigella,

Plesiomonas, Escherichia or Salmonella species. The two components may be formulated at specific initial ratios by processes described, so as to optimize interaction between the components resulting in stable non-covalent complexes ofthe components to each other. The processes generally involve the mixing ofthe components in a selected detergent solution (e.g. Empigen BB, Triton X-100, and/or Mega-10) and then effecting complexing ofthe components while removing detergent by dialysis or, preferably, by diafiltration / ultrafiltration methodologies. Mixing, co-precipitation and/or lyophilization ofthe two components may also be used to effect adequate complexing or association.

The end result of the process is the production of an adjuvant that when administered together with antigens forms an adjuvanted vaccine or immunotherapeutic that can be delivered by a mucosal route (such as nasal, oral, oropharyngeal, ocular, geniturinary mucosal including vaginal, sublingual, intrapulmonary, intratracheal or rectal) or a parenteral route (such as intramuscular, subcutaneous, intravenous, intraperitoneal, submucosal, intradermal) or a transdermal, topical or transmucosal route to induce enhanced levels of serum and/or mucosal antibodies and or type 1 cellular immune responses against the antigen compared with the antigen alone given by the same routes. In the following examples, mixtures containing proteosome-LPS (using LPS from either Shigella or Plesiomonas or Escherichia or Salmonella) and a mono or multivalent split or purified recombinant influenza antigen and delivered by liquid or spray or by injection as an adjuvanted influenza vaccine induced specific anti-influenza immune responses including, for example one or more ofthe following: a) serum IgG antibodies or serum antibodies measured in functional assays including, but not limited to, hemagglutination inhibition (HAI) antibodies; it is noted that HAI responses are significant since their induction is known to correlate with protection against influenza in humans; b) mucosal antibodies including IgA in mucosal secretions collected from the respiratory, gastrointestinal or genitourinary tracts including, but not limited to the nasopharynx, lungs and vagina and c) correlates of cell-mediated immunity (CMI) including the switch or decrease from higher or predominant type 2 responses to result in mixed, balanced, increased or predominant type 1 responses, for example, as measured by the induction of cytokines such as IFN- γ without comparable increases in induction of certain type 2 cytokines such as IL-5 whose levels may, for example, be maintained, decreased, or absent. Such Type 1 responses are predictive ofthe induction of other CMI associated responses such as development of cytotoxic T cells (CTLs) indicative of Thl immunity. The ability ofthe adjuvant given nasally or intramuscularly to elicit these three types of responses against the antigen indicate that the vaccine can provide immunity against infectious diseases since functional serum antibodies (including HAI antibodies) and virus specific lung antibodies are generated. Also, the induction of vaginal IgA for mucosally administered adjuvanted vaccines using the adjuvant ofthe instant invention supports utilization against mucosal infections or allergies distal from the site of immunization such as at the gastrointestinal or genitourinary tracts. Furthermore, the induction of type 1 of responses assists the elimination of residual or intracellular virus, parasite or certain bacterial pathogens. In addition the ability ofthe adjuvant to produce type 1 immune responses against the antigen will be beneficial for producing effective therapeutic vaccines for example against cancer, autoimmune diseases and allergy where CTL and Thl cytokine responses are important.

For example, allergic rhinitis can often be effectively controlled by immunotherapy - a series of injections with increasing doses ofthe substance against which the individual is allergic. Allergic rhinitis can be cured in approximately 50% of individuals who undergo classic immunotherapy. Successful immunotherapy is associated with one or more ofthe following: a switch from T cell responses that result in the production of type 2 cytokines (e.g. IL-5 and JL-4) to those that produce type 1 cytokines (e.g. IFN- γ) and/or an increase in IgG and/or reduction in IgE specific for the allergen. However, in order to achieve these results, up to three years of repeated immunizations are required. The use of allergens together with adjuvants that promote type 1 immune responses may enhance the effectiveness of such immunotherapy and reduce the number of immunizations required.

In the following example we show the results of studies in mice immunized intranasally with TNX-908 together with rBet v 1 a as a recombinant protein representing the major allergen of Birch tree pollen or Birch tree pollen extract. The results for both the recombinant protein and allergen extract demonstrate that IVX-908 converts T cell cytokine production against Bet v ia from a type 2 to a predominately type 1 phenotype. Furthermore, the type 1 response is associated with the increased production of allergen- specific serum IgG compared with the allergen alone, and a reduction in Bet v la-specfic serum IgE compared with allergen administered with aluminum phosphate, a depot and Type 2 adjuvant known to sensitize mice for allergic responses against an allergen. Importantly, the increase in the type 1 cytokine, IFN γ was also observed following the immunization of allergic mice with the same allergen given with IVX-908. The pre- allergic state ofthe mice mimics the situation in allergic humans, suggesting that 1VX- 908/allergen formulations may be candidates for therapeutic allergy vaccines.

It is noted that the instant invention can readily adjuvant vaccines containing single, monovalent or multi-component antigens such as peptides, proteins, toxoids, glycoproteins, glycolipids, carbohydrates and/or polysaccharides, isolated from biologic organisms ofthe animal or plant kingdom that may be infectious organisms, such as parasites, viruses and bacteria, or may be extracts or purified or chemically modified extracts of allergens derived from unicellular or multicellular organisms or may be chemical material. It is also envisioned that whole or disrupted microorganisms including viruses, bacteria or parasites, attenuated or inactivated could be used as antigen. These materials may also be produced by synthetic or recombinant molecular procedures to induce immunity to and protect against several strains of a particular organism or multiple organisms or disease-causing agents or against allergies, cancer or auto-immune diseases. The utility in human and veterinary fields is proposed. Furthermore, the invention can be used to enhance immunity when given together with the antigen as an adjuvanted vaccine or immuiiotherapeutic as priming or boosting immunizations prior to or subsequent to administering the antigen (by mucosal or parenteral routes) without the instant invention.

For parenteral, nasal, oral or suppository use, the adjuvant may be given together with amounts of a variety of excipients or other adjuvants including oils, emulsions, nano- emulsions, fats, waxes, buffers, or sugars, as diluents or vehicles customary in the art to provide stable delivery ofthe product in the desired delivery format. Of particular note, it is emphasised that using the instant invention as an adjuvant is particularly novel since it may, in a preferred embodiment, combine the adjuvant effect of proteosomes together with the immunostimulatory potential of LPS. This complex would not have been predicted to be effective from prior art since it contains full-length LPS that is normally toxic when given alone. As a stable proteosome complex LPS is non-toxic by the nasal and parenteral routes in the given examples as verified by both pre-clinical safety, immunogenicity and toxicity as well as in clinical studies in FDA-approved phase I and phase π clinical trials.

The instant invention may be composed of purified or recombinant bacterial outer- membrane proteins from gram-negative bacteria species including but not limited to

Neisseria meningitidis strains. The LPS can be derived from gram negative bacteria such as, but not limited to Shigella or Plesiomonas or Escherichia or a salmonella species and can be from the same or different species ofthe bacteria used to provide the outer membrane protein proteosomes. In the preferred embodiment the final liposaccharide or LPS content by weight as a percentage ofthe total proteosome protein can be between about 13% and 300%o and, depending on the specificity ofthe application and route of administration may be effective and practical for use at liposaccharide or LPS percentages of 20% to 200%, or may be further distinguished in a particular application at a liposaccharide percentage of between 30% to 150%. The instant invention together with antigen is designed to deliver adjuvanted vaccines by mucosal (nasal, sub-lingual, oral or rectal) or parenteral (intramuscular, subcutaneous, intradermal or transdermai) routes for use in the prevention or treatment of cancer, autoimmune, viral or microbial diseases or against certain toxins or biologic threat agents or allergies whether acquired by mucosal routes such as and specially by inhalation, or by ingestion or sexual transmission, or by parenteral routes such as transdermai, intradermal or subcutaneous or intramuscular.

An embodiment ofthe instant invention is a process for preparing proteosomes with endogenous lipooligosaccharide (LOS) content of between 0.5 % up to about 5% of total protein. Another embodiment ofthe instant invention specifies a process for preparing proteosomes with endogenous liposaccharide of between about 12% to about 25%, and in a preferred embodiment, between 15% and 20% of total protein.

The instant invention specifies a composition containing liposaccharide derived from any gram negative bacterial species which may preferably be naturally or recombinantly different from or the same as the gram negative bacterial species which is the source ofthe proteins in the invention. The composition ofthe present invention maybe optimised, specifically specified by the formulators and varied at will to contain amounts of proteosomes and liposaccharide such that the resultant composition ofthe instant invention contains liposaccharide to an amount that is at least about 13% by weight ofthe weight of total proteosome protein and in a preferred embodiment, may be from 15% to 300% and may be further preferred, depending on the application, to be between 20% to 200%» ofthe total protein on a weight:weight basis or even between 30% and 150% ofthe total protein.

A most preferred embodiment ofthe instant invention is the adjuvant composition wherein the proteosomes are prepared from Neisseria meningitides and the liposaccharide is prepared from Shigella flexneri or Plesiomonas shigelloides and the final liposaccharide content is between 50% to 150% ofthe total proteosome protein by weight.

BRIEF DESCRIPTION OF THE FIGURES

Figure 1 A and B show, respectively two embodiments for the manufacture of proteosome bulk material (Flow Chart 1 A and Flow Chart IB).

Figure 2 shows a scheme for the manufacture of S. flexneri 2a LPS (Flow Chart 2).

Figure 3 shows a scheme for the manufacture of IVX-908 proteosome-LPS adjuvant (Flow Chart 3). Figure 4 a) and b) show the levels of specific serum IgG (a) and lung lavage IgA

(b) elicited when a constant amount of HA was mixed with different amounts of 1NX-908 and used to immunize mice intranasally. Figure 4 c) and d) show the levels of specific serum IgG (c) and lung lavage IgA (d) elicited when a constant amount of IVX-908 (either 1 or 0.3 ug) was mixed with different amounts of HA and used to immunize mice intranasally.

Figure 5 a) shows the numbers of immunized (n=10) or control (n=9) mice surviving challenge with a live, mouse-adapted, homotypic variant influenza virus. Figure

5 b) shows mean weight loss (a measure of morbidity associated with infection by influenza virus) in the survivors in each group. Error bars indicate standard errors on the mean.

Figure 6 shows specific antibody responses in serum of mice immunized i.n. or i.m. with Ovalbumin with or without IVX-908. Titers are expressed as geometric mean concentrations of specific IgG (ug/ml) with 95% confidence limits indicated by error bars.

DETAILED DESCRIPTION OF THE INVENTION

Results show the following activities of IVX-908 adjuvant when mixed with recombinant and split antigens from influenza virus:

A. By the injectable route:

1. Induces up to eight-fold increases in serum HAI and IgG compared with injectable split flu influenza vaccine alone 2. Shifts elicited immune responses to Type 1 (CMI) responses compared to split flu influenza vaccine alone B. By the nasal route:

1. Induces >100- fold increases in serum HAI and IgG responses, compared with split flu influenza antigen alone given by the nasal route 2. Induces up to 10-fold higher specific serum HAI and IgG compared with split flu given by injection

3. Induces > 100- 1000 fold higher specific IgA in lung and or nose compared with split flu influenza antigen alone given nasally or by injection

4. Induces up to 160-fold higher specific IgA in genital tract compared with split flu influenza antigen alone given nasally or by injection

5. Shift to Type 1 (CMI) responses compared to split flu alone

6. Amounts of TVX-908 as little as 0.3 ug to lug are sufficient to achieve optimal enhancement of serum IgG responses against split-flu HA

7. Recombinant influenza HA co-administered with INX-908, induces responses which are protective against mortality and morbidity, and superior to those induced by injection or i.n. administration ofthe antigen alone

8. INX-908 prepared at protein:LPS ratios of 3:1 to 1:3 using LPS from Shigella, Escherichia and Salmonella species were effective.

The results show that respiratory or parenteral immunization with the instant invention and influenza split flu antigen induces enhanced specific anti-influenza HA antibody formation in each of the serum and mucosal bio-samples compared to immunizing with the influenza split product without adjuvant.

Results show the following activities of IVX-908 adjuvant when mixed with rBet v la, the major allergen from Birch pollen as either recombinant allergen or Birch pollen allergen extract and administered via the nasal route.

1. The nasal IVX-908 and rBet v la mixture enhanced induction of the type 1 cytokine, IFN-γ by 50- and 74-fold compared with Bet v ia alone and Bet v ia formulated in aluminium phosphate respectively. The nasal IVX-908 and Birch pollen extract (BPEx) mixture enhanced induction of the type 1 cytokine, IFN-γ by >44- and 3-fold compared with Bet v la alone and Bet v la formulated in aluminium phosphate respectively. 2. The increases in IFN-D production by the lNX-908/Bet v la and INX-908/ BPEx mixtures were not associated with an increase in IL-5 secretion, indicating that INX- 908 directed the immune response against Bet v la towards a type 1 -biased T cell response.

3. Serum IgE induced by the INX-908 Bet v la and TVX-908/BPEx mixtures were approximately 37- and 44-fold lower than that induced by the allergens given with aluminium phosphate respectively.

4. Allergen-specific serum IgG was increased by >400-fold and 22-fold for mice immunized with the IVX-908/Bet v la and IVX-908/ BPEx mixtures compared with Bet v ia and BPEx alone, respectively. 5. In mice sensitized with Bet v la plus alum, the production ofthe type 1 cytokine, IFΝ- γ was increased by 4.7- and 33-fold following immunization with IVX-908/rBet v la and INX-908/BPEx respectively compared with the corresponding allergens alone. In these mice, the levels ofthe type 2 cytokine, IL-5 were reduced compared to the corresponding allergens alone. 6. In mice immunized nasally with IVX-908/allergen mixtures and subsequently given a sensitizing injection with Bet v la plus alum the type 1 cytokine, IFΝ-γ increased by 10-fold compared with birch pollen extract alone. In these mice, the levels ofthe type 2 cytokine, IL-5, were not similarly elevated and indeed were somewhat reduced compared to birch pollen extract alone.

The results demonstrate that lNX-908/allergen formulations induce strong type 1 cytokine responses in allergen naive and sensitized mice, suggesting that these formulations prepared with purified or recombinant proteins or extracts of allergens may be used as vaccines or therapeutics for specific immunotherapy for allergic diseases. Results show the following activities of INX-908 adjuvant when mixed with ovalbumin (ON A), a known poor immunogen and given by the nasal or injectable route.

1. Enhances ONA-specific serum IgG titers by greater than 60- and 75-fold via the nasal and injectable routes respectively compared with antigen alone,

2. Enhances the secretion of OVA-specific IFΝ-γ and IL-5 from re-stimulated splenocytes compared with antigen alone resulting in a balanced type of immune response.

EXAMPLES

Example 1: Production of proteosomes

Two examples of outer membrane protein proteosome preparations are shown. These preparations were purified from type 2 Νeisseria meningitidis by extraction of phenol- killed bacterial paste with a solution of 6% Empigen BB (EBB) (Albright and Wilson, Whithaven, UK) in 1 M calcium chloride followed by precipitation with ethanol, solubilization in 1% EBB-Tris/EDTA-saline and then precipitation with ammonium sulphate. The precipitates were re-solubilized in the 1% EBB buffer, diafiltered and stored in an EBB buffer at -70°C. A flow chart of this process, which resulted in proteosomes having a liposaccharide content of between 0.5% and 5%, is shown in Flowchart 1 A (Figure 1 A) on the following pages. Proteosomes may also be prepared by omitting the ammonium sulphate precipitation step to shorten the process as desired with resultant proteosomes having a liposaccharide content of between 12% and 25%, and may, depending upon the materials, be between 15% and 20% as shown in Flowchart IB (Figure IB).

Example 2: Production of liposaccharides

The example in Flowchart 2 (Figure 2) shows the process for the isolation and purification of LPS from S. flexneri or P. shigelloides bacteria. This process can similarly be used for preparing LPS from other gram-negative bacteria including, but not restricted to Shigella, Plesiomonas, Escherichia and Salmonella species. Following growth of the bacteria by fermentation, the cell paste was re-hydrated with 3 mL 0.9M NaCl, 0.005 M EDTA/g paste. Ten mg lysozyme /g paste was also added. Lysozyme digestion was allowed to proceed for 1 hour at room temperature. Fifty U/mL Benzonase (DNase) was then added with 0.025M MgCl₂. DNase digestion was allowed for 30 minutes to proceed at room temperature. The suspension was then cracked by passage through a microfluidizer at 14,000 to 19,000 psi. Fresh DNase (50 U/mL) was added and the suspension was digested for a further 30 min at room temperature. The digested cell suspension was heated to 68°C in a water bath. An equal volume of 90% phenol (at the same temperature) was added and the mixture was incubated with shaking at 68°C for 30 min. The mixture was centrifuged at 4°C to separate the aqueous and organic phases. The aqueous phase was harvested and the organic phase was re-extracted with WFI (water for injection) at 68°C for 30 min. The mixture was centrifuged at 4°C to separate the aqueous and organic phases and the aqueous phases were combined. Twenty percent ethanol and 10 mM CaCl₂ were added to the combined aqueous phase to precipitate nucleic acids. The mixture was stirred at 4°C overnight. Precipitated nucleic acids were then pelleted by centrifugation at 10,000XG for 30 minutes and the supernatant was collected.

The supernatant was concentrated and diafϊltered using a 30,000 MW hollow fiber cartridge into 0.15M NaCl, 0.05M Tris, 0.01M EDTA and 0.1% Empigen BB, pH 8.0. Finally, the LPS was sterile-filtered using a 0.22 urn Millipak 60 filter unit aliquoted into sterile storage containers and frozen at -80°C.

Example 3: Preparation and characterisation of a proteosome-liposaccharide adjuvant complex

The adjuvant is manufactured by non-covalently complexing Proteosomes to LPS. The LPS can be derived from any of a number of gram negative bacteria including, but not limited to Shigella or Plesiomonas or Escherichia or Salmonella species as described in Flowchart 3. Briefly, Proteosomes and LPS were thawed overnight at 4°C and adjusted to 1% Empigen BB in TEEN buffer. Proteosomes were thawed overnight and adjusted to 1% Empigen BB in TEEN buffer. The two components were mixed at quantities resulting in a final Proteosome:LPS wt/wt ratio of between 10:1 and 1:3 and stirred for 15 minutes at room temperature. The LPS-Proteosome mixture was diafiltered on an appropriately sized (e.g. Size 9) 10,000 MWCO hollow fiber cartridge into TNS buffer (0.05 M Tris, 150 mM NaCl pH 8.0). The diafiltration was stopped when Empigen content in the permeate was < 50 ppm (by Empigen Turbidity Assay or by a Bradford Reagent Assay). The bulk adjuvant IVX-908 was concentrated and adjusted to 5 mg/mL protein (by Lowry assay). Finally, the adjuvant was sterile- filtered using a 0.22 urn Millipak 20 filter unit. The bulk adjuvant was aliquoted into sterile storage containers and frozen.

The Proteosome-LPS complex was tested for Empigen (400 ppm) using reverse- phase HPLC; protein content by Lowry, LPS content by measurement of 2-keto-3- deoxyoctonate (KDO) assay. The said invention was further characterised for particle size distributions as determined by quantitative number weighted analysis using a particle sizer (Brookhaven Instruments model 90 plus or similar machine) (10-100 nm). However, the particle size for the complex will increase with a higher proteosome to LPS ratio. Stability of the complex formulations should be consistent with the previously demonstrated S. flexneri LPS vaccine. These data demonstrate complex stability at both refrigerated and accelerated temperature (25 and 37°C).

Example 4: Preparation of fVX-908 influenza antigen or Birch pollen allergen or ovalbumin mixtures

The current invention was prepared by mixing the IVX-908 Proteosome-LPS adjuvant (Example 3) with antigen in proportions that promote optimal formulations for stability and immunological outcomes. Example 5: Mouse immunization protocols for influenza antigen studies

BALB/c mice were immunized intranasally or intramuscularly on days 1 and 21 with antigens in volumes of 25 or 100D1 respectively containing between 0.3 and 3ug influenza hemagglutinin (HA) as A/Beijing/262/95 or an A/Beijing/262/95 plus A Sydney/5/97 bivalent detergent split antigen (GMP commercial licensed antigen) either alone or mixed with 0.3-3 ug IVX-908 adjuvant (containing LPS at various Proteosome:LPS wt/wt ratio). Control mice were given intranasal immunizations with phosphate buffered saline. Animals were bled on day 35 via the saphenous vein or by cardiac puncture. Nasal or lung lavage or vaginal washes were taken on day 35. The lungs of each mouse were surgically exposed and a canula inserted in the trachea. Using a syringe containing phosphate buffered saline supplemented with 0.1% bovine serum albumin and protease inhibitors (0.2 mM AEBSF, 1 Dg/ml Aprotinin, 3.25 uM Bestatin and 10 uM Leupeptin), 1 nasal lavage sample (approximately 1 ml) and 2 lung lavage samples (2 1 ml) were collected. The lung lavage fluids from individual animals were combined, vortexed and centrifuged to remove cell debris, and supernatants stored at - 70°C until assayed by ELISA. Vaginal washes were performed by inserting a tampon wetted with 25 ul of supplemented phosphate buffered saline (as above), into the vagina of the mouse for 30 seconds. After removing the tampon, the procedure was repeated with the opposite end ofthe tampon. The tampon was stored frozen at -70°C and reconstituted in ELISA blocking buffer (see Example 8) at time of assay.

Example 6: Serum hemagglutination inhibition assay (HAT)

Prior to determination of HAI activity, mouse sera were heated at 56°C to inactivate complement. Elimination of non-specific agglutination was achieved by treating mouse sera with receptor destroying enzyme (RDE). To 0.1 ml of serum was added 0.4 ml of RDE (100 units/ml) for 12 to 18 hr at 37°C. 0.3 ml of sodium citrate (2.5%) was added for 30 min at 56°C to inactivate the RDE. The sample volume was made up to 1 ml with PBS (to give final sample dilution of 1 : 10). Two-fold serial dilutions of each sample were tested for their ability to inhibit the agglutination of 0.5% chick red blood cells by whole influenza virus in a standard HAI assay.

Example 7: Measurement of specific anti-flu antibodies in sera, in lung, nasal and vaginal fluids

Sera were collected after each immunization; lung and nasal cavity lavage fluids and vaginal washes were collected after the last immunization. ELISA was performed using whole virus or detergent split antigen as the detecting antigen. Briefly, 96 well round bottom microtiter plates (e.g. Costar EIA RIA 96 well Easywash Plates, Corning, NY) were coated with antigen and incubated overnight. After aspiration ofthe antigen using a plate washer, plates were washed once with PBS containing 0.1% Tween (PBS-T) and incubated with blocking buffer containing PBS-T plus 2% powdered milk. After aspirating the blocking buffer and washing with PBS-T, samples of sera, lung or nasal cavity lavage fluids, or vaginal washes serially diluted 2-fold in blocking solution, were added and the plates were incubated for two hours at 37°C. After washing with PBS-T, affinity purified horseradish peroxidase (HRP)-labelled goat anti-mouse IgG or IgA was added and plates were incubated at 37°C for 30 min. After aspirating and washing twice with PBS-T, developing solution was added and plates were incubated for 30 min at r.t. and stopped by addition of H₂SO₄ prior to determining the absorbance values using a microtiter ELISA plate reader (Molecular Devices, Menlo Park, California). Antibody titers in the Tables are expressed as ng/ml of specific IgG or IgA determined from a standard curve produced using an ELISA capture assay using affinity purified mouse IgG and IgA standards (Sigma).

Example 8: Enhanced immunogenicity and immunity elicited by IVX-908 Adjuvanted influenza vaccines This example shows the serum and mucosal antibody responses induced following nasal immunization with monovalent (A/Beijing/262/95) or nasal or intramuscular immunization with bivalent (A/Beijing/262/95 plus A/Sydney/5/97) antigens given with or without IVX-908 adjuvants. Mice received 2 doses of antigen containing 0.3 ug HA and IVX-908 (which IVX-908 consists of a 1:1 wt/wt proteosome to LPS ratio with 1.2 ug of proteosome protein for every 0.3 ug of HA) per strain of influenza antigen used. Anti- influenza IgG antibodies in sera were analysed by HAI; IgG in sera and IgA antibodies in lung and nasal cavity fluids were analysed by ELISA. Results are shown and summarised in Tables 1-3. Briefly:

INX-908 ADJUVANTED INFLUENZA VACCINE given nasally:

1. elicited between 50 to 250-fold higher serum IgG responses than the split Flu influenza antigen alone given nasally and up to 10-fold greater than the influenza vaccine given by injection (i.m.) (Tables 1-3), 2. elicited 16 to 100-fold higher serum HAI responses than split Flu alone given nasally and up to 8-fold higher than elicited by giving the split product influenza vaccine alone by injection (Tables 1-3 ), 3. elicited between 20 to 120-fold higher IgA responses in the nasal cavity than the split Flu influenza vaccine alone given nasally or by injection (i.m.) (Table 1), 4. elicited 50 to >600-fold higher specific IgA responses in the lung than split Flu influenza vaccine alone given nasally or by injection (i.m.) (Tables 1-3), 5. induced 30 to >160-fold increases in specific vaginal IgA compared with split Flu influenza vaccine alone given nasally or by injection (Table 2).

IVX-908 ADJUVANTED INFLUENZA VACCINE given intramuscularly:

1. induces up to 5-fold increases in specific serum IgG and up to 8-fold increase in serum HAI compare to the split Flu influenza vaccine alone given by injection (table 3) The data demonstrates that IVX-908 prepared with LPS from either P. shigelloides (Tables 1 and 3) or S. flexneri (Table 2) when mixed with influenza split antigens, enhances both the serum and mucosal antigen-specific immune responses. Furthermore, JNX-908 adjuvanted the HA-specific immune responses against each ofthe individual monovalent HA antigens when given as a multivalent preparation (Tables 2 and 3).

Table 1. Adjuvant effect of JNX-908 via the intranasal route with monovalent antigen. Murine serum HAI, IgG and mucosal IgA induced by split flu antigen (A/Beijing/262/95) mixed with INX-908 adjuvant (3 ug HA per dose at 4:1 IVX-908 :HA ratio) following nasal immunization.

All samples taken 14 days post 2 ^■>nd immunization.

JNX-908 prepared with P. shigelloides LPS .

* are Geometric Means for 10 mice/group** HAI for sera pooled from 10 mice/group

Table 2. Adjuvant effect via the nasal route with bivalent antigen. Murine anti- A/Beijing/262/95 (HI) serum HAI, IgG and mucosal IgA induced by bivalent split flu antigen (AJBeijing/262/95 HI and A/Sydney/5/97 (H3) mixed with IVX- 908 adjuvant (0.3 ug HA/strain per dose at 4:1 INX-908 :HA ratio) given nasally

A. Anti- A/Beijing/262/95 (HI) response

B. Anti-A/Sydney/5/97 (H3) response

JNX-908 prepared with S. flexneri LPS .

• are Geometric Means for 10 mice/group

• ** HAI for sera pooled from 10 mice/group

Table 3. Adjuvant effect via the nasal or intramuscular route. Murine anti-

A/Beijing/262/95 (HI) serum HAI, IgG and mucosal IgA induced by bivalent split flu antigen (A/Beijing/262/95 HI and A/Sydney/5/97 (H3) mixed with IVX-908 adjuvant (0.3 ug HA/strain per dose at 4:1 INX-908 :HA ratio) given nasally or intramuscularly

A. Anti- A/Beijing/262/95 (HI) response

Lung IgA (ng/mL)* 1,006 16 10

B. Anti- A/Sydney/5/97 (H3) response

All samples taken 14 days post 2^nd immunization. Adjuvant prepared with P. Shigelloides LPS .

• are Geometric Means for 10 mice/group

• ** HAI for sera pooled from 10 mice/group

Example 9: The shift of immune responses from type 2 to type 1 by nasal Proteosome influenza vaccines

Spleen cell cultures from mice immunized with Proteosome-LPS adjuvanted and non-adjuvanted influenza split antigens were analyzed for their production of T cell cytokines interferon gamma (IFΝ-γ) and JL-5 as an indicator of induction of Thl or Th2 type immune responses, respectively. Briefly, Balb/c mice were immunized either intranasally or intramuscularly as described in Example 6 with a bivalent formulation containing 3 ug influenza HA from with A/Beijing/262/95 plus A/Sydney/5/97 with or without 24 ug INX-908 Proteosome-LPS. Mice were euthanized 14 days after the second immunization and the spleens from 5 mice from each group were harvested and cells teased into a single cell suspension using a 100-μm nylon cell strainer (Becton Dickinson, NJ). Spleen cells were cultured at 2.0 10⁶ cells/ml (200 μl/well) in RPMI 1640 medium (Gibco BRL, Life technologies, Burlington, ON) containing 8% fetal bovine serum (heat- inactivated for 1 hr at 56°C; Gibco BRL), 2 mM glutamine (Gibco BRL), 50 μM 2- mercaptoethanol (Sigma Chemical Co., St-Louis, MO) and 50 μg/ml gentamycin (Gibco BRL) with or without UV-inactivated, purified A/Beijing/265/95 (H1N1) and JNR-108 reassortant (H3Ν2) influenza viruses (NIBSC, Hertfordshire, UK) in 96-well cell culture cluster (Corning, NY). Cells were incubated for 72 hrs at 37°C and supernatants harvested and frozen at -80°C. Murine cytokines levels were measured using sandwich ELISA kits (OptEIA set, purchased from Pharmingen, San Diego, CA) according to manufacturer's instructions. Recombinant cytokines were used as standards.

Briefly, results in Table 4 demonstrate that INX-908 given together with a multivalent bivalent split flu antigen to form an adjuvanted influenza vaccine given either nasally or intramuscularly induces uniquely the type 1 cytokine, IΝF D, without detectable JL-5, a type 2 cytokine. Conversely, bivalent influenza antigen alone given nasally or intramuscularly induces a mixed type 1 and type 2 immune response as evidenced by the production of both IΝF-γ and IL-5. These results indicate that JNX-908 induces enhanced antigen-specific serological responses and biases T cell responses against antigens towards the type 1 of immunity. Type 1 immune responses are important for the clearance of intracellular pathogens, for the development of anti-tumor responses and in the control of allergic responses.

Table 4. Murine cytokine induction from spleen cells. Mice were immunized with bivalent split flu antigen (A/Beijing/262/95 HI and A/Sydney/5/97 H3) and JNX-908 adjuvant (3 ug HA/strain per dose at 4:1 JNX-908 :HA ratio) given nasally or intramuscularly. JNX-908 adjuvant was prepared with P. shigelloides LPS. Spleen cells were re-stimulated with whole inactivated A/Beijing/262/95 (HI) or a Sydney (H3) reassortant. A. A/Beijing/262/95 (HI) immunization and re-stimulation

B. A/Sydney/5/97(H3) immunization and re-stimulation

IΝF-γ and JL-5 were determined in supernatants of mouse spleen cells re-stimulated as described in Example 10 with whole inactivated virus (1.25 ug/rnL) and are expressed in pg/mL of culture supernatant. Results are the means of triplicate cultures, and have had the values obtained for IFΝ-γ and JL-5 (pg/mL) from spleen cells of PBS immunized mice already subtracted.

Example 10: Defining optimal amounts and ratios of INX-908 and Hemagglutinin antigen to maximise adjuvantation

Mice were immunized i.n. on days 0 and 14 with lug of HA (H3Ν2 strain, A/Sydney/5/97) mixed with INX-908 (proteosome protein:S. flex LPS, 1:1) in decreasing amounts from 10 ug to 0.03 ug. A subsequent study varied the amount of HA from 3 to 0.3 ug while keeping the amount of INX-908 constant at 1 or 0.3 ug. In both studies, blood, lung lavage, nasal wash fluid and spleens were collected at euthanasia on day 21 and analyzed for IgG or IgA content, or used to prepare splenocytes for in vitro stimulation as appropriate (as described in Example 9 above). Significance of the data was assessed by AΝOVA analysis using Tukey-Kramer pair-wise comparisons.

Figure 4 a) and b) show that above a threshold at 0.3-1 ug of JNX-908, the elicited immune responses leveled-off, and below this threshold, the elicited responses diminished significantly. Keeping the amount of INX-908 constant at this threshold, a second study was performed varying the amount of HA between 3 ug and 0.3 ug. The results in Figure 4 c) and d) show that maximal systemic and mucosal immune responses were obtained when HA was mixed with JNX-908 above a threshold of l-3Dg of HA (administered i.n. with either 0.3 ug or 1 ug of JNX-908). The results indicate that in order to elicit optimal immune responses in mice, 1-3 ug of HA should be mixed with 0.3-1 ug of JNX-908.

As in other studies, analysis of the cytokines released from in vitro stimulated splenocytes showed that i.n. administration of HA with INX-908 elicited responses primarily of type 1 phenotype.

Example 11 : Enhancement of systemic and mucosal immune responses, and protection against live virus challenge, elicited by intranasal administration of recombinant hemagglutinin mixed with IVX-908

Baculo virus-derived recombinant influenza hemagglutinin (rHA; H1Ν1 strain A/Texas/36/91), supplied as a full-length uncleaved protein (HAO), was purchased from a commercial source. The immunogenicity of the rHA was assessed by immunization of groups of 15, 6-8 week old female BALB/c mice. For intranasal (i.n.) immunizations, mice were lightly anesthetized, 25 ul of vaccine containing 2D g of rHA with or without INX- 908 (8 ug proteosome protein and 8 ug S. flex LPS), or PBS was applied to the nares (12.5 Dl per nostril) and the mice allowed to inhale the droplets. Intramuscular (i.m.) immunization was achieved by injection of 25 ul (2 ug rHA) into the hind limbs. All mice were immunized on days 0 and 21. Ten animals from each group were challenged on day 48 by i.n. instillation of 8 LD₅₀ of mouse-adapted homotypic variant influenza virus (A/Taiwan/ 1/86) to assess protection. Any deaths were recorded, and weight loss was used as a surrogate for morbidity; mice were weighed immediately before and every 2 days after challenge. Mice losing > 30% of their pre-challenge body weight or showing a lesser weight loss (> 20%) in conjunction with other clinical signs of distress and or morbidity (e.g. pilo-erection, hunched posture, reduced mobility) were deemed to have met the experimental endpoint criteria and were euthanized. The 5 non-challenged mice from each group were euthanized on day 51 and exsanguinated by cardiac puncture. Serum was separated from clotted blood and stored at -70 °C until assay. Spleens were removed aseptically and processed for in vitro re-stimulation (as described in Example 9 above). Nasal washes and lung lavage were performed as previously described.

Table 5a shows the systemic and mucosal responses in samples collected on day 51, and Table 5b shows the amounts of IFN-γ and JL-5 released from splenocytes following specific in vitro stimulation. Figure 5 a) shows the protection against mortality, and b) protection against morbidity, in immunized or control mice following challenge with live, homotypic variant, mouse-adapted virus.

The results demonstrate that:

1 Serum responses elicited by JNX-908 + rHA were 4 x and 100 x higher respectively than the responses induced by rHA alone given i.m. or i.n.

2 Only i.n. rHA administered with IVX-908 elicited detectable mucosal IgA responses. 3 In. immunization with JNX-908 + rHA induced responses of type 1 phenotype in contrast to i.m. rHA alone which induced responses of type 2 phenotype. 4 In contrast to rHA immunized or control mice, all mice (10/10) immunized i.n. with JNX-908 + rHA survived live virus challenge. 8/10 and 1/10 mice immunized i.m. or i.n. with rHA alone survived whilst no control mice survived. 5 Mice immunized i.n. with IVX-908 + rHA suffered no weight loss following challenge. The surviving mice immunized with rHA alone by either i.n. or i.m. routes, all lost significant amounts of weight, indicating morbidity as a result of infection following challenge. Thus i.n. JNX-908 + rHA protected mice against morbidity as well as mortality following challenge.

Table 5 a shows the systemic and mucosal responses elicited by immunization of mice with 2 ug of rHA, with or without IVX-908, as described in example 11. HI titer is the reciprocal of the maximum dilution of serum which will inhibit hemagglutination, and immunoglobulin levels (IgG or IgA) are expressed as Geometric Mean Concentrations with 95% confidence limits in parentheses. ΝD = not detected.

Table 5b shows the amounts (pg/ml; determinations performed in triplicate) of JFN-γ and JL-5 released into culture supernatants following in vitro stimulation of splenic T cells from mice immunized with 2 ug of vaccine or control material. Splenocytes were restimulated with inactivated mouse-adapted A/Taiwan influenza virus.

Example 12: Induction of serum and mucosal antibodies and shift of immune responses from type 2 towards type 1 by nasal IVX-908/Bet v ia allergen formulation

Recombinant Bet v ia protein was expressed in E. coli with a His-Tag (His) added at the amino terminus and purified by affinity chromatography on nickel columns. BALB/c mice were immunized intranasally (in volumes of 28 μl (Table 6) or 36 μl (Table 7) three times at two (Table 7) or three (Table 6) weeks apart with either lOμg Bet v la as purified recombinant protein (rBet v la) or birch pollen extract (BPEx) (Greer Labs. Inc.) alone or as a mixture of 1 Oμg rBet v 1 a or BPEx plus 1 Oμg of IVX-908 (Tables 6 and 7). Control mice were given intranasal immunizations with phosphate buffered saline (PBS). Other mice were given 10 μg Bet v la in 2 mg aluminum phosphate intraperitoneally in a volume of 150μl on days 0 and 21 (Table 6), or 3 μg birch pollen extract (BPEx) (Greer Labs. Inc.) in 1 mg aluminum phosphate on day 0 (Table 7). One (Table 6) or three (Table 7) weeks after the final immunization, animals were bled by cardiac puncture subsequent to obtaining lung lavage fluids. Bet v la-specific IgE (OptEIA Mouse IgE Set; BD Pharmingen, Mississauga, Ontario), IgG, IgGl and IgG2a in serum, and IgA and total IgA in broncho-alveolar lavages were measured by ELISA. The levels of secreted IFN-γ and JL-5 were determined in the supernatants from spleen cell cultures (10 x 10⁶ splenocytes/mL) after two and three days respectively following re-stimulation in vitro with 10 μg/ml Bet v ia. Cytokines were detected by ELISA (BD Pharmingen; Mississauga, Ontario). In table 8, an example is shown for cytokine induction in mice injected intraperitoneally on day 71 with a single dose of 10 μg rBet v la in 2 mg aluminum phosphate following 3 nasal immunizations on days 0, 17 and 29 with 10 μg birch pollen extract (BPEx) (Greer Labs. Inc.) alone or as a mixture with lOμg of JNX- 908. In Table 9, an example is shown for cytokine induction following 3 immunizations of rBet v la or BPEx with or without TVX-908 in mice previously sensitized intraperitoneally with a single dose of 10 μg Bet v la in 2 mg aluminum phosphate.

Results for T cell cytokine and serum and mucosal immunoglobulin responses following intranasal immunization with an INX-908/rBet v la or an JNX-908/BPEx mixture are shown in Tables 6, 7, 8 and 9.

JNX-908 ADJUVANTED rBet v la or BPEx given nasally to naϊve mice (Tables 6 and 7):

1. directed the T cell response induced by Bet v ia allergen from a type-2 biased to a higher or predominantly type-1 phenotype. This was due to the enhanced production of IFN-γ by spleen cells from mice given JNX-908 formulated allergen compared to rBet v la or BPEx alone or with aluminum phosphate with a lowering (for INX-908/BPEx) or maintenance (for JNX-908/rBet v ia) ofthe production of IL-5, 2. enhanced production of Bet v la-specific serum IgG compared with rBet v la or BPEx given alone, and, 3. produced a 37-43 fold reduction in levels of serum IgE levels compared with that induced by rBet v la in aluminium phosphate, an immunizing regime known to sensitize animals for allergic responses on subsequent challenge with antigen.

Table 6. Induction of murine cytokines and serum and mucosal antibodies by 10 ug rBet v la alone or formulated with JNX-908 (10 ug 1 : 1 protei LPS) via the nasal route, or with 2 mg aluminium phosphate by the intraperitoneal route as described in Example 10.

Results for IFN-γ and JL-5 are expressed as the mean pg/mL for triplicate cultures from spleens pooled from 5 mice/group. Serum IgG is expressed as the sum of IgGl and IgG2a titers. Lung IgA is shown as specific IgA expressed as % total IgA. All immunoglobulin titers were calculated using geometric mean titers for samples from 7 to 10 (IgG and IgE) or 5 (IgA) mice/group. INX-908 was prepared with S. flexneri LPS.

Table 7. Induction of murine cytokines and serum IgG by 10 ug birch pollen extract (BPEx) alone or formulated with 10 ug JNX-908 via the nasal route as described in Example 12. For BPEx + alum, mice were given a single i.p. immunization of 3 ug birch pollen extract together with 1 mg aluminum phosphate.

Results for JFΝ-γ and JL-5 are expressed as the mean pg/mL for triplicate cultures from spleens pooled from 4-5 mice/group. Serum IgG is for sera pooled from 15 mice except for the BPEx + INX-908 group where the geometric mean of results from 15 individual mice were calculated. Serum IgE for the BPEx + JNX-908 group represents the geometric means from sera from 15 individual mice while BPEx + Alum results are geometric means for 86 individual mice. Serum IgE levels for BPEx and PBS were measured in sera pooled from 15 animals. JNX-908 was prepared with S. flexneri LPS.

JNX-908 adjuvanted BPEx given nasally to mice and subsequently injected with rBet v ia plus alum (Table 8):

1. increased the production ofthe type 1 cytokine, IFΝ-γby 10-fold compared with BPEx given alone 2. and slightly lowered the levels ofthe type 2 cytokine, IL-5.

Table 8. Induction of cytokines in mice injected intraperitoneally with rBet via plus alum following 3 nasal immunizations with 10 ug birch pollen extract alone or formulated 1:1 with JNX-908 (10 ug protein:LPS) as described in Example 12.

Results for IFΝ-γ and JX-5 are expressed as the geometric means (pg/mL) from spleen cultures from 8-10 individual mice/group. INX-908 was prepared with S. flexneri LPS.

INX-908 adjuvanted rBet v la or BPEx given nasally to rBet v ia sensitized mice (Table 9):

1. increased the production ofthe type 1 cytokine, IFΝ-γby 4.7- and 33-fold for JNX- 908/rBet v la and JNX-908/BPEx respectively compared with the corresponding allergens alone and

2. lowered the levels ofthe type 2 cytokine, JL-5 Table 9. Induction of murine cytokines by 10 ug rBet v la or birch pollen extract given nasally alone or with 10 ug JVX-908 in rBet v la-sensitized mice as described in Example 12.

Results for JFΝ-γ and IL-5 are expressed as the geometric means (pg/mL) from spleen cultures from 4-5 mice/group. IVX-908 was prepared with S. flexneri LPS.

The data in Tables 6, 7, 8 and 9 demonstrate that allergens (purified recombinant proteins or extracts) formulated with JNX-908 induce type 1 immune responses in mice. These formulations maintained the production of type 1 cytokines in mice subsequently injected intraperitoneally with a sensitizing injection of rBet v ia plus alum. Importantly, these formulations also enhanced the production of type 1 cytokines in mice that had previously been sensitized or made allergic to the allergen. These results suggest the potential utility of INX-908/allergen formulations as therapeutic vaccines for allergic diseases.

Example 13: Enhancement of immune responses against a poor immunogen.

Mice were immunized as above by either the i.n. or i.m. routes, with Ovalbumin (OVA - a poorly immuno genie, soluble protein) in decreasing amounts from 100 ug to 5 ug, with or without 1 ug of IVX-908 ( proteosome protei LPS 1:1, using P. shig LPS). Following immunization on days 0 and 14, mice were euthanized on day 21 and serum, lung lavage fluids and spleens collected for analysis. Serum GMCs are shown in Figure 6.

The data confirms that unadjuvanted OVA is poorly immunogenic and elicited barely detectable serum IgG titers even when mice were immunized with 100 ug of OVA by either i.n. or i.m. routes. However when mixed with INX-908, over 60-fold rises in titers were observed by both routes of immunization, albeit at higher concentrations (> 25 ug) of OVA. No mucosal responses were detected in any ofthe immunized mice. Analysis of the cytokine profiles elicited by OVA or OVA + IVX-908 showed that when immunized i.n., co-administration of IVX-908 induced the secretion of elevated levels of IFN-γ, IL-2, JL-4 and JL-5 from splenocytes. Thus unlike HA which induced release of cytokines indicative of a type 2 phenotype response which switched to a type 1 phenotype when HA was administered with IVX-908, adjuvanting of the poorly immunogenic, soluble OVA appeared to be associated with induction of a balanced type 1/type 2 phenotype response.

Example 14: Effect of varying the amount of LPS in INX-908 on elicited immunity.

To determine the effects of varying the ratio of proteosome to LPS in INX-908 on elicited immunity, a study was performed in which mice were immunized i.n. as above with 3 ug of HA (H3Ν2 strain A Sydney) mixed with 1 ug (as LPS) of INX-908 (1:1 or 1:2 complex of proteosomes and P. shigelloids LPS). At euthanasia, blood and lung washes were collected and analyzed by ELISA for specific IgG or IgA respectively. The results are shown in table 9, and indicate that although both INX-908s elicit virtually identical levels of specific serum IgG, there is a highly significant difference (P < 0.001) between the mucosal IgAs elicited by the different INX-908s. Clearly the INX-908 comprising proteosomes complexed 1:1 with P. shigelloids LPS elicited higher titers of specific mucosal IgA in lung lavage fluids and therefore possesses more mucosal adjuvant activity than the 1 :2 proteosome protein:LPS complex.

Table 9 shows immunoglobulin levels (IgG or IgA) expressed as geometric mean concentrations with 95% confidence limits in parentheses, in serum and lung washes from mice immunized i.n. with HA + JNX-908 (Pr:LPS 1 : 1 or 1 :2).

Example 15: Adjuvant effects of JNX-908 prepared with LPS from different organisms.

To determine the adjuvanticity of INX-908 made by complexing proteosomes to LPS from novel organisms, IVX-908 preparations were made using LPS from a non- pathogenic E. coli (017) and from Salmonella essen. INX-908 preparations were made by mixing proteosomes and the LPS in 3:1, 1:1 and 1:3 (w/w) ratios in the presence of Empigen, and removal of detergent by dialysis in dialyzing cassettes. Mice were immunized i.n. on day 0 and 14 with 3 ug of HA (B/Guangdong) mixed with 3 ug or 0.3 ug (as LPS) of INX-908. Control mice received 3 ug HA i.n. At euthanasia on day 21, blood was collected and analyzed by ELISA for specific IgG. The results are shown in Table 10, and indicate that JNX-908 preparations made with LPS from pathogens other than Shigella species are capable of enhancing immune responses to a vaccine antigen. For JNX-908 prepared with E. coli LPS, the 1:1 and 1:3 ratios of proteosomes to LPS at a dose of 0.3 ug LPS gave significant (P < 0.001) enhancement of the anti-HA serum IgG response compared with HA alone given i.n. All ratios of Pr:LPS (S. essen) at both doses tested elicited significant (P < 0.001) enhancenment of serum anti-HA responses over HA alone given i.n. The results for IVX-908 made with S. essen were comparable to those obtained for INX-908 made with LPS from Shigella species.

Table 10 shows serum anti-HA IgG titers expressed as geometric mean concentrations (ug/ml) with 95% confidence limits in parentheses for 8 mice per group immunized i.n. with HA + IVX-908 preparations containing LPS from different gram negative bacteria and at different Pr:LPS ratios.

To the extent necessary to understand or complete the disclosure ofthe present invention, all publications, patents, and patent applications mentioned herein are expressly incorporated by reference therein to the same extent as though each were individually so incorporated.

Claims

Claims:

1. An adjuvant composition comprising an outer membrane protein proteosome preparation prepared from a first gram-negative bacteria and a liposaccharide preparation derived from a second gram-negative bacteria, wherein the outer membrane protein proteosome and liposaccharide preparations form a stable non-covalent adjuvant complex, and wherein a final liposaccharide content by weight as a percentage of the total proteosome protein is at least about 13 %.

2. The adjuvant composition of claim 1 wherein the first and second gram- negative bacteria are the same.

3. The adjuvant composition of claim 1 wherein the first and second gram- negative bacteria are different.

4. The adjuvant composition of claim 1 wherein the first gram-negative bacteria is selected from genus Neisseria.

5. The adjuvant composition of claim 4 wherein the Neisseria is Neisseria meningitides

6. The adjuvant composition of claim 1 wherein the second gram-negative bacteria is selected from the following genera: Escherichia, Shigella, Plesiomonas, or Salmonella.

7. The adjuvant composition of claim 6 wherein the second gram-negative bacteria is selected from E. coli, S. flexneri, P. shigelloides, or S. essens.

8. The adjuvant composition of claim 1 wherein the final liposaccharide content by weight as a percentage ofthe total proteosome protein is between 15% to 300%.

9. The adjuvant composition of claim 1 wherein the final liposaccharide content by weight as a percentage ofthe total proteosome protein is between 20% to 200%.

10. The adjuvant composition of claim 1 wherein the final liposaccharide content by weight as a percentage ofthe total proteosome protein is between 30% to 150%>.

11. The adjuvant composition of claim 1 wherein the proteosome preparation has a liposaccharide content between about 0.5 % and about 5 % of total protein.

12. The adjuvant composition of claim 1 wherein the proteosome preparation has a liposaccharide content between about 12 % and about 25 % of total protein.

13. The adjuvant composition of claim 1 wherein the proteosome preparation has a liposaccharide content between about 15 % and about 20 % of total protein

14. The adjuvant composition of claim 1 wherein the first gram-negative bacteria is Neisseria memngitides and the second gram-negative bacteria is Shigella flexneri and the final liposaccharide content is between 50% to 150%.

15. The adjuvant composition of claim 1 wherein the first gram-negative bacteria is Neisseria meningitides and the second gram-negative bacteria is Plesiomonas shigelloides and the final liposaccharide content is between 50% to 150%.

16. An immunogenic composition comprising the adjuvant complex of any one of claims 1-15 and an antigen.

17. The immunogenic composition of claim 16 wherein the antigen is selected from peptides, proteins, toxoids, glycoproteins, glycolipids, lipids, carbohydrates, and/or polysaccharides.

18. The immunogenic composition of claim 16 wherein the antigen is derived from a biologic or infectious organism ofthe animal or plant kingdom, are allergens or chemically or biologically modified allergens, or are chemical materials.

19. The immunogenic composition of claim 16 wherein the antigen is whole or disrupted microorganisms including viruses, bacteria or parasites, attenuated and/or inactivated.

20. The immunogenic composition of claim 16 wherein the antigen is produced by synthetic or recombinant molecular procedures.

21. The immunogenic composition of claim 16 wherein the antigen is Bet v ia.

22. The immunogenic composition of claim 16 wherein the antigen is rBet v ia.

23. The immunogenic composition of claim 16 wherein the antigen is recombinant influenza antigen.

24. The immunogenic composition of claim 16 wherein the antigen is influenza split antigen.

25. The immunogenic composition of claim 16 wherein the antigen is birch pollen extract.

26. The immunogenic composition of claim 16 wherein the antigen is an immunogen extract.

27. The immunogenic composition of claim 16 wherein the composition is a specific immunotherapeutic, adjuvanted prophylactic vaccine or therapeutic vaccine.

28. A process for preparing the adjuvant composition of any one of claims 1-15 comprising mixing the outer membrane protein proteosome preparation prepared from a first gram-negative bacteria and the liposaccharide preparation derived from a second gram-negative bacteria to effect complexing of the components to form the adjuvant composition.

29. The process of claim 28 wherein the proteosome preparation and the liposaccharide preparation are mixed in a detergent solution.

30. The process of claim 29 wherein the detergent solution is Empigen BB, Triton

X-100, Mega-10.

31. The process of claim 29 further comprising removing detergent by dialysis, diafiltration, or ultrafiltration methodologies or combinations thereof.

32. The process of claim 29 wherein the removal step includes diafiltration, ultrafiltration methodologies or combinations thereof.

33. The process of claim 28 wherein the mixing includes co-precipitation and/or lyophilization of both preparations.

34. A process for preparing an immunogenic composition comprising mixing the adjuvant complex of any one of claims 1-15 with antigen to form the composition.

35. The process of claim 34 wherein the antigen is selected from peptides, proteins, toxoids, glycoproteins, glycolipids, , lipids, carbohydrates, and/or polysaccharides.

36. The process of claim 34 wherein the antigen is derived from a biologic or infectious organism ofthe animal or plant kingdom, are allergens or chemically or biologically modified allergens, or are chemical materials.

37. The process of claim 34 wherein the antigen is whole or disrupted microorganisms including viruses, bacteria or parasites, attenuated and/or inactivated.

38. The process of claim 34 wherein the antigen is produced by synthetic or recombinant molecular procedures.

39. The process of claim 34 wherein the antigen is Bet v la.

40. The process of claim 34 wherein the antigen is rBet v ia.

41. The process of claim 34 wherein the antigen is recombinant influenza antigen.

42. The process of claim 34 wherein the antigen is influenza split antigen.

43. The process of claim 34 wherein the antigen is birch pollen extract.

44. The process of claim 34 wherein the antigen is an immunogen extract.

45. A process for inducing an immune response comprising administering the composition of any one of claims 16-27 to a subject.

46. The process of claim 45 wherein the composition is administered by a route selected from the group consisting of mucosal, enteral, parental, fransdermal/transmucosal, and inhalation to induce serum or mucosal antibodies or Type 1 cellular immune response against the antigen.

47. The process of claim 46 wherein the mucosal route is via the nasal, oropharyngeal, ocular, or genitourinary mucosa.

48. The process of claim 46 wherein the enteral route is oral, rectal or sublingual.

49. The process of claim 46 wherein the parenteral route is any one of intraarterial, intradermal, intramuscular, intraperitoneal, intravenous, subcutaneous, and submucosal injection or infusion.

50. The process of claim 46 wherein the transdermal/transmucosal route is topical.

51. The process of claim 46 wherein the inhalation route is intranasal, oropharyngeal, intratracheal, intrapulmonary or transpulmonary.

52. The process of claim 45 wherein the amount administered enhances an immune response.

53. The process of claim 45 wherein the enhanced immune response includes one or more of the following: a) serum IgG antibodies or serum antibodies measured in functional assays; b) mucosal antibodies including IgA in mucosal secretions collected from respiratory, gastrointestianl or genitourinary tracts and c) correlates of cell-mediated immunity (CMI) including a shift from higher or predominant Type 2 responses to mixed, balanced, increased or predominant Type 1 responses as measured by cellular or antibody assays or Type 1 cytokine assays such as IFN-γ with maintained, decreased or absent Type 2 cytokines such as JL-5.

54. The process of claim 45 wherein administration includes a series of administration steps.