IMMUNSTIMULATING LIPID FORMULATION

Description

[0001] The present invention relates to a novel pharmaceutical formulation for administration of antigens and/or vaccines. The preferred route of administration is via the mucosal membranes, however parenteral administration may also be used. The invention also relates to the use of certain compounds (as defined below) as adjuvants or vehicles in such formulation.

Background

[0002] An increasing number of specific antigens from different types of organisms (e.g. tumor cells, bacteria, virus and parasites) has been produced using cloning techniques over the last years. However, these antigens are frequently weak immunogens despite their high specificity.

[0003] To obtain good protection after vaccination, immune stimulating systems are needed that can enhance and activate the immune system against these weak antigens. Such immune stimulating systems are called adjuvants.

[0004] Adjuvants, presently mainly used in animal experiments, includes a highly heterogeneous group of substances; inorganic substances, oil emulsions, charged polymers, neutral substances or substances from bacteria.

[0005] There are presently large efforts in research and development in order to obtain a safe adjuvant with high efficacy to be used in humans. However, today there is presently no general adjuvant for this purpose.

[0006] Alum hydroxides and alum phosphates were the first two inorganic substances that were used in humans. The immune response obtained is a result of slow desorption of the precipitated antigen on the surface of the particle. Later it was shown that phagocyting cells were attracted by these alum salts leading to further enhancement of the immune response. However, these salts are not safe since granuloma formation has been reported (Slater et al, Br.J.Dermatol. (1982) Vol. 107, page. 103-108.). Furthermore, the alum salts can not be used for all antigens since all antigens are not adsorb on the surface.

[0007] In 1944 Freund introduced his adjuvant consisting of a mixture of vegetable oil, mineral oil, detergents and killed bacteria. The enhancement obtained was partly due to slow release of the antigen from the oil emulsion. Freunds adjuvant can however not be used in humans due to granuloma formation, induction of auto-immune reactions and the non-biodegradable mineral oil. Furthermore, the effect is difficult to control. The active substance in Freunds adjuvant has been isolated and its structure determined and shown to be N-acetyl muramyl-L-alaninisoglutamate, often called muramyl-dipeptide (MDP).

[0008] The adjuvant effect dependent of the particle size of polymetacrylate and polystyrene particles was examined on mice (Kreuter et al, Vaccine, (1986) vol 4, 125-129) by the use of ovalbumin (adsorbed on the particles) as a model antigen with subsequent assay of the immune response. The size of the particles was varied between 62 and 306 nm. The result was that smaller particles enhanced the immune response better than larger. The smaller particles gave a better effect than 0.2% Al(OH)₃ . All preparations elicited a higher response as compared to fluid preparations. Similar experiments where particulate systems with smaller size results in a higher immune response as compared to larger particles are known in the scientific literature.

[0009] Almost all systems used today for enhancement of the immune response against antigens are particles or is forming particles together with the antigen. In the book "Vaccine Design - the subunit and adjuvant approach" (Ed: Powell & Newman, Plenum Press, 1995) all known adjuvants are described both regarding their immunological activity as well as regarding their chemical characteristics. As described in the book more than 80% of the adjuvants tested today are particles or polymers that together with the antigens (in most cases proteins) are forming particles. The type of adjuvants that not are forming particles are a group of substances that are acting as immunological signal substances and which under normal conditions consists of the substances that are formed by the immune system as a consequence of the immunological activation after administration of particulate adjuvant systems.

[0010] Using particulate systems as adjuvants, the antigens are associated or mixed with or to a matrix which has the characteristics of being slowly biodegradable. Of great importance using such matrix systems are that the matrix does not form toxic metabolites. Choosing from this point of view, the main kind of matrices that can be used are mainly substances originating from a body. With this background there are only a few systems available that fulfils these demands: lactic acid polymers, poly-amino acids (proteins), carbohydrates, lipids and biocompatible polymers with low toxicity. Combinations of these groups of substances originating from a body or combinations of substances originating from a body and biocompatible polymers can also be used. Lipids are the preferred substances since they display structures that make them biodegradable as well as the fact that they are the most important part in all biological membranes.

[0011] Lipids are characterized as polar or non-polar. The lipids that are of most importance in the present invention are the polar lipids since they have the capacity to form particulate systems in water. Another way of defining these lipids are as amphifilic due to their chemical structure with one hydrophobic and one hydrophilic part in the molecule thereby being useable as surface active substances. Examples of main groups of polar lipids are mono-glycerides, fatty acids, phospholipids and glycosphingolipids. These main groups can be further characterized depending on the length of the acyl chain and the degree of saturation of the acyl chain. Since the number of carbon atoms in the acyl chain can be in the range of 6 to 24 and the number of unsaturated bonds can be varied there are an almost infinite number of combinations regarding the chemical composition of the lipid.

[0012] Particulate lipid systems can be further divided into the different groups as discussed in the scientific literature such as liposomes, emulsions, cubosomes, cochleates, and micelles

[0013] In a number of systems the lipids may spontaneously form, or can be forced to form, stabile systems. However, under certain circumstances other surface active substances has to be introduced in order to achieve stability. Such surface active systems can be of non-lipid character but possess the characteristics of the polar lipids having hydrophobic and hydrophilic parts in their molecular structure.

[0014] Another factor that has been shown to be of importance is that lipids exhibit different physical chemical phases, these phases has in different test systems been shown to enhance uptake of biological substances after administration to mucosal membranes.

[0015] In the classical immunology and in combination with vaccination against different types of infectious agents e.g. bacteria, virus or parasites the prevailing dogma has been to administrate the vaccine subcutanously or intramuscularly. However, research has during the last years shown that the body has a very effective immunological system that resides in the mucosa. It has been shown that you can administrate vaccines orally, nasally, rectally and vaginally. In the same way as for the classical immunization it has been shown that by mucosal vaccination there is also a need for enhancement of the immunological response by the addition of adjuvants.

[0016] In the same way as within the classical immunology where vaccines (antigens) are administrated parenterally, there is within mucosal immunization a great interest in directing the immunological response towards development of humoral and/or cellular response. If you obtain a humoral response it would be important to direct the response in a way that a certain class of antibodies would be obtained. In order to obtain such a goal, specific immune stimulating agents can be added to the formulation of antigens and adjuvants.

[0017] Different types of immune stimulating substances are available. One type is represented by proteins e.g. phytohemaglutinin (PHA), Concanavilin A (Con A), Staphyllococcus Enterotoxin A (SEA) or different types of interferons or interleukines. Another type of substance is represented by MDP, as mentioned above. Additional groups can be characterized as lipid derivatives since they show molecular structures which are amphiphilic. One example of such a substance is called monophosphoryl Lipid A (MPL). Another similar substance is Quil A saponin (Quil A). A number of substances that can be classified within these categories are described in the book "Vaccine Design - the subunit and adjuvant approach" as discussed above.

[0018] It would be extremely valuable to be able to make the immunization procedures more effective directing the immunological response towards a certain class or subclass of antibodies and/or to be able to induce a strong T-cell response against the antigens.

Description of the invention

[0019] It has now surprisingly been found that parenteral or mucosal administration of a vaccine composition containing the following adjuvant with admixed antigens improves the immune response against the admixed antigens. Said adjuvant for parenteral or mucosal administration of antigens and/or vaccines to an animal comprises

i) a monoglyceride having a purity of at least 80% w/w, the monoglyceride having the formula

wherein R is selected from H and an acyl group containing from 6 to 24 carbon atoms with the proviso that two of the R groups are H, and

ii) a fatty acid with 6 to 24 carbon atoms, the acyl chain of the fatty acid being saturated or unsaturated,

iii) water,

and wherein the concentration of i) is from 0.1 g to 50 g per 100 ml of water, and the concentration of ii) is from 1 g to 50 g per 100 ml of water, and wherein the administration of the adjuvant to a human or animal elicits an immune response in the human or animal to an antigen administered to the human or animal.

[0020] In a preferred embodiment, the acyl group of the monoglyceride may contain from 8 to 20 carbon atoms, and in a more preferred embodiment, the acyl group may contain from 14 to 20 carbon atoms. The acyl group may also contain unsaturated bonds.

[0021] The acyl group is normally placed at the first or third R position, i.e. the first or third - C(=O)- group of the glycerol backbone. However, there is normally an acyl migration between the first or third and the second position resulting in approximately 90% in the first or third position and approximately 10% in the second position.

[0022] In the present invention distilled 1-monoglyceride from Danisco Ingredients (Denmark) with a purity of more than 80%, preferably more than 90% and more preferably over 95% is used. The diglyceride content is maximum 3% and the content of triglycerides and fatty acid are less than 1.0%. The monoglycerides according to the invention normally contain more than 80% of a specific fatty acid, preferably over 90%.

[0023] In one embodiment of the invention the acyl chain of the fatty acid may contain from 8. to 20 carbon atoms, and in a further embodiment the acyl chain may contain between 14 and 20 carbon atoms.

[0024] The vaccine composition according to the invention may comprise additional pharmaceutical excipients selected from the one or several of the following groups; preservatives and osmotic pressure controlling agents, pH-controlling agents, organic solvents, hydrophobic agents, enzyme inhibitors, water absorbing polymers, surfactants and absorption promoters, anti-oxidative agents, and the like.

[0025] The vaccine composition according to the invention may comprise any antigen selected among all the antigens relevant to humans or animals, including marine animals. Examples are antigens from pathogenic and non-pathogenic bacteria, viruses, parasites and tumor cells.

[0026] This application discuss lipids which, when mixed with antigens, enhance the immune activity against the antigens thereby functioning as an adjuvant in various vaccine formulations. Especially the invention comprise the use of a formulation for vaccination of the mucosa which can be immunologically activated by nasal, oral, vaginal or rectal administration. The invention also comprise the use of the lipid system for parenteral administration. The use of an adjuvant such as described in the present invention, which can be used both for parenteral as well as for mucosal administration is not limited to humans. Equally important is the use within the veterinary field for the immunization of e.g. cattle, pigs and chickens. Furthermore, there is a large and growing interest in applying both parenteral as well as mucosal vaccines in the field of fish farming. In this area the administration can be performed by incorporation of the formulation in the food. Furthermore, the fish may be allowed to swim for a limited period of time in the vaccine formulation containing the antigens and the adjuvants thus being immunized by the mucosal route via the gills.

[0027] In the scientific literature there are reports showing how to enhance the uptake of a biologically active substance after administration to the mucosa together with certain lipids. As an example Li & Mitra (Pharm.Res. vol 13:1, 1996) describes the administration of insulin mixed with phospholipids in the form of liposomes to the lung. They show that the effect is dependent on the length of the acyl chain and the charge of the particle. Optimal length was 10 carbon atoms and the charge preferably positive. Even negatively charged particles were effective but neutral system were inferior.

[0028] In the same way de Haan et al (Vaccine, 13:2, 155-62, 1995) describes a mixture of liposomes and the antigen hemeagglutinin. The mixture was administrated nasally to rats whereafter a positive immunological response could be detected. Gupta et al (Vaccine, 14:3, 219-25, 1995) describes that a mixture of diphtheria toxoid together with a non-phospholipid based liposom system administrated parenterally to rabbits results in an immune response which was at the same level as the marketed product which was Alum-adsorbed diphtheria toxoid.

[0029] A number of scientific reports also show that good immunological reponses are obtained after administration of liposomes to the mucosa where the antigen is entrapped or adsorbed to liposomes.

[0030] Studies in vitro on a human cell line obtained from a colon cancer (Caco-2) shows that the best penetrating effect, tested with the model substance mannitol, can be seen with a chain length of 10 carbon atoms. In this case the lipids consisted of the salts of fatty acids. The obtained mixture of these lipids forms together with water micelles (Lindmark et al, J.Pharm.Exp.Ther. 275, 958-65, 1995).

[0031] Liposomes consists of phospholipids and are formulated by a relatively lengthy and cumbersome process which i.a. involves organic solvents. Furthermore, the phospholipids are expensive.

[0032] As described below in the present invention, a similar immunological response can be obtained only by mixing the antigen with a lipid formulation which contains less complicated lipids having a substantially lower price and which can be formulated on a commercial basis in a very simple way.

[0033] Another systems that to some extent are similar to the present invention are formulations based on triglycerides. However, these systems are scientifically defined as emulsions of triglycerides where surfactants are used for stabilization. As stabilizers phospholipids or any other type of amphiphilic molecules such as Tween® are normally used. Furthermore, the appearance of such emulsions are normally milky, indicating a size of the oil droplets of about 1 µm. It is well-known for the person skilled in the art that these surfactants are excellent adjuvants. Thus, the adjuvant properties of oil emulsions are primarily due to the characteristics of the surfactant and not of the triglyceride composition.

[0034] In PCT/DK94/00062 is disclosed a formulation for the topical administration of antigens and/or vaccines to mammals via the mucosal membranes. Said application disclose in the examples that the only formulation that enhances the immune response is a combination of caprylic/capric acid glycerides with polyoxyethylene sorbitan monoester (Tween 20®).

[0035] As exemplified in the present invention it is shown that a combination between a monoglyceride and a fatty acid can stimulate the immune system to produce antibodies and induce protective immunity. Furthermore the present invention shows that the disclosed formulation is able to produce high antibody titers by parenteral administration.

[0036] Thus, it was surprisingly found that the administration of antigens and/or vaccines to an animal either via the mucosal route or parenterally using a formulation comprising monoglycerides and or fatty acids as a particulate lipid system can improve the immunological response towards the admixed antigens and/or vaccines. The monoglycerides are selected from a group with the general formula of 1-acyl-glyceride, wherein the number of carbon in the acyl chain may be varied between 6 and 24, preferably between 8 and 20. The acyl chain may be either saturated or unsaturated. The concentration of the monoglyceride may be in the range of 0.1-50g per 100 ml of water, preferably in the range of 1 - 20 g per 100 ml of water. The fatty acid concentration may be in the range of 0.1 - 50 g per 100 ml formulation, preferably in the range of 1 - 20 g per 100 ml water. When monoglycerides and fatty acids are formulated together the percent ratio of monoglyceride in fatty acid may be varied between 1 to 99 %, preferably between 10 to 90 %.

[0037] The invention also relates to a vaccine composition containing, in 100 g of the final composition:

from 0.1 to 50 g of a monoglyceride i)

from 1 to 50 g of a fatty acid ii)

from 0.01 to 90 g of the antigen component

from 0.01 to 99 g of water

from 0.01 to 99 g of PBS or saline

[0038] The vaccine composition according to the invention may also comprise additional adjuvants.

[0039] An enhancement of the immunological response after administration of monoglycerides and/or fatty acids together with antigens and/or vaccines has not been suggested anywhere in the prior art.

[0040] The present invention describes that mixtures of antigens with relevant lipids stimulates the body to generate protective immunity. Another advantage of the present invention is the simple formulation process and as compared to entrapment no material (antigen) is lost in the process. As an example can be mentioned that in the process of entrapment in liposomes the recovery is normally 10-20%. The rest is lost in the process.

[0041] Reports in the literature as discussed above, shows that by mixing liposomes and antigen an immune response is detected after administration to the mucosa.

[0042] However, the examples in this invention as described below shows that the system can be even more simplified by the use of lipids that are more stable, cheaper and which can be formulated to particles in a more convenient and simplified way.

[0043] The invention is exemplified by the following examples showing that the principle of co-administration of antigens, immune stimulating substances associated or in combination with particles function as an adjuvant.

Example 1.

[0044] A suspension of mono-olein was produced by adding 3 g mono-olein to 50 ml of a 0.6 % Pluronic-127® solution in phosphate buffered saline pH 7.4, whereafter the mixture was sonicated with a probesonicator for 4 minutes. The obtained milky suspension contained particles with a maximal size of about 2 µm as determined by light microscopy.

Example 2.

[0045] A negatively charged micelle suspension of mono-oleate was produced by mixing of 0.5 g of oleic acid with 5 ml of 0.35 M NaOH and sonicated with a probesonicator for 5 seconds. Thereafter 3 g mono-olein and 50 ml 0.9 % NaCl was added whereafter the mixture was probesonicated for 4 minutes. The monester content of the mono-oleate was over 95 % with a acyl chain containing 92 % oleate and 6% linoleic acid. The pH was adjusted to 8.3. The obtained completely clear homogenous solution contained particles with a size of below approximately 0.2 µm as determined by visual inspection. It is known that if a clear solution is obtained the particle size is below approximately 0.2 µm, a slightly opalescent bluish appearance indicated a size of approximately 0.2 - 0.5 µm and if the appearance is milky the size is above approximately 0.8 µm.

Example 3.

[0046] A positively charged micelle suspension of mono-olein was produced by mixing 0.5 g lauryl-amine and 3.5 ml of 0.5 M HCl followed by sonication for 5 seconds. Thereafter 3 g mono-olein and 50 ml of water was added whereafter the mixture was probesonicated for 4 minutes. The pH was adjusted to between 4 and 5 using 0.5 M HCl. The obtained completely clear homogenous solution contained particles with a size of below approximately 0.2 µm.

Example 4.

[0047] A mixture of particles according to Example 1 and diphtheria toxoid was administrated subcutanously to mice followed by a booster after 21 days. After 30 days blood samples were obtained which were assayed for IgG antibodies against diphtheria toxin as well as Neutralization titers (NT) using Vero cells. The serum from Alum (n=5) and monoolein (n=5) groups was pooled and assayed. The mice receiving nasal boost and responded (= 3 of 5) were assayed on an individual basis. In arbitrary units is shown in Table 1 the IgG titers and neutralization titers The results showed that both IgG as well as protective antibody titers were at the same level as compared to the control group which received the marketed product comprising diphtheria toxoid adsorbed on Alum (Al(PO₄)₃). Also seen is that high IgG titers always were accompanied by high neutralization titers indicating that the formulation does not destroy the antigenic sites that are important for protective immunity.

Table 1.

	Dose diphtheria toxoid µg	IgG titer (arb.units)	NT titer arb.units)
Alum	13+15	32000	40000
Alum	3.5+3.5	22000	20000
Mono-olein suspension	15+15	24000	20000
Mono-olein suspension	3.5+3.5	3500	5000
Nasal boost	7+4	45000	10000
Nasal boost	7+4	19000	2500
Nasal boost	7+4	19500	5000

Example 5.

[0048] Particles were prepared according to Example 2 with a final concentration of monoglyceride of 200 mM and of fatty acid of 200 mM. Diphtheria toxoid (2.9 µl, 4.4 mg/ml) was mixed with 200 µl of the micelle suspension and administrated subcutanously to mice followed by a subcutaneous booster after 21 days. Both the primary and the booster dose of the toxoid was 10 µg. After 30 days blood samples were obtained which were assayed for IgG antibodies against diphtheria toxin. The result showed (Table 2) that the arbitrary IgG titers with respect to the formulation with mono-olein (MO) and oleic acid (C 18:1) were at the same level as compared to the control group which received the present marketed product comprising diphtheria toxoid adsorbed on Alum (Al(PO₄)₃). The other combinations of monoglycerides and fatty acids gave slightly declining responses which correlated to declining length of the acyl chain (M 12 = lauryl-1-glycerate; M 10 = capric-1-glycerate; C12 = lauric acid; C10 = capric acid; C8 = caprylic acid). N.D. = Not Done; indicates that there were only five mice in these groups.

Table 2.

IgG response of individual mice (n = 5 or 6) after sc/ sc administration of different formulations containing monoglycerides and fatty acids.
	1	2	3	4	5	6
Alum	19200	19200	9600	9600	19200	N.D.
MO / C18:1	19200	19200	19200	19200	9600	N.D.
MO / C8	9600	9600	4800	9600	4800	9600
M12 / C12	19200	9600	4800	18200	9600	19200
M10 / C10	4800	110	2400	1200	2400	4800

Example 6.

[0049] The same procedure as in Example 4 with the difference that the booster dose was given nasally instead of subcutanously. The dose of diphtheria toxoid was 10 µg both at the primary immunization as well as at the nasal booster administration. In the same experiment a dose-response is demonstrated that is obtained when tree different amounts of lipid (see Table 3) was administrated. The arbitrary IgG titer is seen in Table 4. Besides the dose-response effect where lower IgG titers is seen at lower concentrations of lipids there is also seen a higher variability regarding response in the groups receiving lower doses. This variability is not seen at higher dose levels indicating that an adjuvant effect is not only seen with respect to obtaining high titers but also regarding reduction of the variability of the response.

Table 3.

Amount of lipids in µmol administrated to mice sc or nasally.
Dose level	Dose lipid (µmol) sc	Dose Lipid (µmol) nasally
high	40	1.5
medium	4	0.15
low	0.4	0.015

Table 4.

IgG titers in individual mice (n = 6) after administration of 2 x 10 µg of diphtheria toxoid to mice either sc/sc or sc/nasally.
	1	2	3	4	5	6
MO/C8 sc/sc high	4800	4800	9600	4800	9600	9600
MO /C8 sc/nas high	9600	1200	4800	4800	4800	9600
MO /C8 sc/sc medium	4800	1200	9600	2400	4800	4800
MO/C8 sc/nas medium	2400	600	2400	600	2400	4800
MO / C8 sc/sc low	300	2400	9600	2400	4800	2400
MO/C8 sc/nas low	600	600	1200	150	4800	150

Example 7.

[0050] Two different lipid formulation were tested. The compositions are seen in Table 5.

Table 5.

	Monoglyceride	Fatty acid
Composition A	Monooleate 25 mM	Caprylic acid 90 mM
	Monomyristate 25 mM
	Monolaurate 25 mM
	Monocaprate 25 mM
Composition B	Monooleate 200 mM	Oleic acid 200 mM

[0051] The formulations were administrated to mice s.c. or nasally with a booster after three weeks s.c. or nasally. Blood samples were taken after another week. The arbitrary IgG titers are seen in Table 6.

[0052] The results in Table 6 demonstrates that in order to achieve a good response after primary as well as booster administration by the nasal route Compositions B is to be preferred.

Table 6.

	1	2	3	4	5	6
Composition A sc/nas	2400	4800	4800	19200	4800	4800
Composition A nas/nas	< 100	36400	< 100	< 100	300	< 100
Composition B sc/nas	19200	19200	36400	19200	< 100	N.D.
Composition B nas/nas	4800	9600	19200	19200	2400	9600

Example 8.

[0053] A mixture of mono-olein (200 mM) and caprylic acid (200 mM) was mixed with formalin inactivated influenza virus (strain SDA/94) and administrated s.c. at the first occasion to mice followed by a nasal booster three weeks later. The dose was 0.05 µg Hemaglutinin (HA) and blood sample were taken 3 weeks after the booster dose and assayed for agglutination titers (HI) against HA. The results (Table 7) showed that the HI titers in the group receiving the virus together with the adjuvants was at a higher level as compared to the group receiving the virus in PBS.

Table 7.

HI titers in mice receiving formalin inactivated influenza virus after s.c. primary injection and nasal booster.
	1	2	3	4	5	6
PBS	N.D.	80	N.D.	40	N.D.	80
MO/C8	320	320	640	160	320	*
N.D. = not detected
* = dead

Example 9.

[0054] Micelles according to Example 2 was mixed with formalin killed rota virus particles and subsequently administrated to female mice. After three immunizations the mice were made pregnant whereafter the new-born mice were challenged nasally with live rota virus. The figures indicate the animals that acquired protection after challenge as compared to the total number of animals in that group. The result from this challenge is seen in Table 8.

Table 8.

Protection after challenge of rota virus to baby mice where the mother was vaccinated with a lipid formulation according to the invention.
Group	Administration	Protection
Saline	im/im/im	2/8
Micelles	im/im/im	4/4
Micelles	im/nas/nas	6/7

[0055] As can be seen from the results there is a good protection both after three intramuscular administrations as well as after a primary intramuscular immunization followed by two nasal administrations.

Example 10.

[0056] To evaluate the toxicity of the lipid formulations these were administrated into the rat nasal cavity whereafter the rats were killed and the nasal mucosa were prepared for light, fluorescence as well as scanning electron microscopy (SEM). Formulations according to Example 1 and Example 2 were tested. Only the mono-olein/pluronic suspension showed minor changes in the mucosal surface using the SEM. No effects could be detected under light or fluorescence microscopy. The micelles containing mono-olein and oleic acid were unable to provoke any changes in the mucosal membranes.

Example 11.

[0057] Caco-2 cells, which are a human cell line originating from a colon cancer can be made to grow as a epithelial mono layer. These cells are frequently used to examine different substances ability to influence the transport of biological substances through epithelial cells and has in a number of experimental systems been shown to give a good correlation to in vivo data regarding uptake from the gut into the bloodstream. As marker substances for transport through the cells Na-flouresceine or mannitol is used. The experiments with the lipid formulations according to this invention showed an enhanced transport through the Caco-2 cells at non-toxic concentrations.

Claims

1. An adjuvant for use in a vaccine, the adjuvant containing

i) a monoglyceride having a purity of at least 80% w/w, the monoglyceride having the formula

wherein R is selected from H and an acyl group containing from 6 to 24 carbon atoms with the proviso that two of the R groups are H, and

ii) a fatty acid with 6 to 24 carbon atoms, the acyl chain of the fatty acid being saturated or unsaturated,

iii) water,

wherein the concentration of i) is from 0.1 g to 50 g per 100 ml of water, and the concentration of ii) is from 1 g to 50 g per 100 ml of water, and wherein the administration of the adjuvant to a human or animal elicits an immune response in the human or animal to an antigen administered to the human or animal.

2. An adjuvant according to claim 1, wherein the vaccine contains an antigen component.

3. An adjuvant according to claim 1, wherein the purity of the monoglyceride i) is at least 90%.

4. An adjuvant according to claim 1, wherein the purity of the monoglyceride i) is at least 95%.

5. An adjuvant according to claim 1, wherein the acyl group of the monoglyceride i) contains from 8 to 20 carbon atoms.

6. An adjuvant according to claim 1, wherein the acyl group of the monoglyceride i) contains from 14 to 20 carbon atoms.

7. An adjuvant according to claim 1, wherein the acyl group of the fatty acid ii) contains from 8 to 20 carbon atoms.

8. An adjuvant according to claim 1, wherein the acyl group of the fatty acid ii) contains from 14 to 20 carbon atoms.

9. A vaccine composition comprising an adjuvant according to any of claims 1-8 and an immunogenic quantity of an antigen component.

10. A vaccine composition according to claim 9, wherein the antigen component is capable of causing the formation of an immune response in animals including humans and marine animals.

11. A vaccine composition according to claim 9 or 10, wherein the antigen component is selected from the group consisting of antigens from pathogenic and non-pathogenic bacteria, viruses, parasites and tumor cells.

12. A vaccine composition according to any of claims 9-11 containing, in 100 g of the final composition:

from 0.1 to 50 g of a monoglyceride i)

from 1 to 50 g of a fatty acid ii)

from 0.01 to 90 g of the antigen component

from 0.01 to 99 g of water

from 0.01 to 99 g of PBS or saline

13. A vaccine composition, according to any of claims 9-12, wherein the composition comprises additional pharmaceutical excipients selected from the group consisting of preservatives, osmotic pressure controlling agents, ph-controlling agents, organic solvents, enzyme inhibitors, water absorbing polymers, absorption promoters and anti-oxidative agents.

14. A vaccine composition according to any of claims 9-13, wherein the composition comprises additional adjuvants.

15. A vaccine composition according to any of claims 9-14, wherein the composition is in a form suitable for parenteral or mucosal administration.

16. A vaccine composition according to claim 15, wherein the composition is in a form suitable for administration to the mucosa of the nose, mouth, vagina, rectum or intestine.

17. A vaccine composition according to claim 15, wherein the composition is in a form suitable for administration to the mucosa of the nose.

18. A vaccine composition according to any of claims 9-17, wherein the antigen component is selected from the group consisting of diphteria toxoid, influenza virus, and rotavirus.

19. A vaccine composition according to any of claims 9-18, wherein the purity of the monoglyceride i) of the adjuvant is at least 90%.

20. A vaccine composition according to claim any of claims 9-19, wherein the purity of the monoglyceride i) of the adjuvant is at least 95%.

21. A vaccine composition according to any of claims 9-20, wherein the acyl group of the monoglyceride i) of the adjuvant contains from 8 to 20 carbon atoms.

22. A vaccine composition according to any of claims 9-21, wherein the acyl group of the monoglyceride i) of the adjuvant contains from 14 to 20 carbon atoms.

23. A vaccine composition according to any of claims 9-22, wherein the acyl group of the fatty acid ii) of the adjuvant contains from 8 to 20 carbon atoms.

24. A vaccine composition according to any of claims 9-23, wherein the acyl group of the fatty acid ii) of the adjuvant contains from 14 to 20 carbon atoms.

25. Use of an adjuvant according to any of claims 1-8 for the production of a pharmaceutical composition for enhancing an immune response to an antigen in an animal including a human.

26. Use of a vaccine composition according to any of the claims 9-24 for the production of a pharmaceutical composition for immunizing a human or an animal.

Ansprüche

1. Hilfsmittel zur Verwendung in einem Impfstoff, wobei das Hilfsmittel das Folgende enthält:

i) ein Monoglycerid einer Reinheit von wenigstens 80 Gew.-%, wobei das Monoglycerid die folgende Formel hat:

in der R aus H und einer Acylgruppe mit 6 bis 24 Kohlenstoffatomen ausgewählt ist, mit der Maßgabe, dass zwei der R-Gruppen H sind, und

ii) eine Fettsäure mit 6 bis 24 Kohlenstoffatomen, wobei die Acylkette der Fettsäure gesättigt oder ungesättigt ist,

iii) Wasser,

wobei die Konzentration von i) 0,1 g bis 50 g pro 100 ml Wasser ist, und die Konzentration von ii) 1 g bis 50 g pro 100 ml Wasser ist, und wobei die Verabreichung des Hilfsmittels an einen Menschen oder ein Tier eine Immunreaktion in dem Mensch oder Tier gegenüber einem Antigen hervorruft, das dem Menschen oder Tier, verabreicht wurde.

2. Hilfsmittel gemäß Anspruch 1, wobei der Impfstoff eine Antigen-Komponente enthält.

3. Hilfsmittel gemäß Anspruch 1, wobei die Reinheit des Monoglycerids i) wenigstens 90 % ist.

4. Hilfsmittel gemäß Anspruch 1, wobei die Reinheit des Monoglycerids i) wenigstens 95 % ist.

5. Hilfsmittel gemäß Anspruch 1, wobei die Acylgruppe des Monoglycerids i) 8 bis 20 Kohlenstoffatome enthält.

6. Hilfsmittel gemäß Anspruch 1, wobei die Acylgruppe des Monoglycerids i) 14 bis 20 Kohlenstoffatome enthält.

7. Hilfsmittel gemäß Anspruch 1, wobei die Acylgruppe der Fettsäure ii) 8 bis 20 Kohlenstoffatome enthält.

8. Hilfsmittel gemäß Anspruch 1, wobei die Acylgruppe der Fettsäure ii) 14 bis 20 Kohlenstoffatome enthält.

9. Impfstoff-Zusammensetzung, umfassend ein Hilfsmittel gemäß irgendeinem der Ansprüche 1 bis 8 und eine immunogene Menge einer Antigen-Komponente.

10. Impfstoff-Zusammensetzung gemäß Anspruch 9, wobei die Antigen-Komponente befähigt ist, die Bildung einer Immunreaktion in Tieren, einschließlich Menschen und Meerestieren, zu bewirken.

11. Impfstoff-Zusammensetzung gemäß den Ansprüchen 9 oder 10, wobei die Antigen-Komponente aus der Gruppe ausgewählt ist, die aus Antigenen von pathogenen und nicht-pathogenen Bakterien, Viren, Parasiten und Tumorzellen besteht.

12. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 11, die in 100 g der fertigen Zusammensetzung Folgendes enthält:

0,1 g bis 50 g eines Monoglycerids i)

1 g bis 50 g einer Fettsäure ii)

0,01 g bis 90 g der Antigen-Komponente

0,01 g bis 99 g Wasser

0,01 g bis 99 g PBS oder Salzlösung.

13. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 12, wobei die Zusammensetzung zusätzliche pharmazeutische Trägerstoffe umfasst, die aus der Gruppe ausgewählt sind, bestehend aus Konservierungsmitteln, Mitteln zur Steuerung des osmotischen Drucks, Mitteln zur Steuerung des pH-Werts, organischen Lösungsmitteln, Enzym-Inhibitoren, wasserabsorbierenden Polymeren, Absorptionsbeschleunigern und Antioxidationsmitteln.

14. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 13, wobei die Zusammensetzung zusätzliche Hilfsmittel umfasst.

15. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 14, wobei die Zusammensetzung in einer Form vorliegt, die zur parenteralen oder mucosalen Verabreichung geeignet ist.

16. Impfstoff-Zusammensetzung gemäß Anspruch 15, wobei die Zusammensetzung in einer Form vorliegt, die geeignet ist, um der Schleimhaut von Nase, Mund, Vagina, Rektum oder Darm verabreicht zu werden.

17. Impfstoff-Zusammensetzung gemäß Anspruch 15, wobei die Zusammensetzung in einer Form vorliegt, die geeignet ist, um der Nasenschleimhaut verabreicht zu werden.

18. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 17, wobei die Antigen-Komponente aus der Gruppe ausgewählt ist, die aus Diphtherie-Toxoid, Grippevirus und Rotavirus besteht.

19. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 18, wobei die Reinheit des Monoglycerids i) des Hilfsmittels wenigstens 90 % ist.

20. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 19, wobei die Reinheit des Monoglycerids i) des Hilfsmittels wenigstens 95 % ist.

21. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 20, wobei die Acylgruppe des Monoglycerids i) des Hilfsmittels 8 bis 20 Kohlenstoffatome enthält.

22. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 21, wobei die Acylgruppe des Monoglycerids i) des Hilfsmittels 14 bis 20 Kohlenstoffatome enthält.

23. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 22, wobei die Acylgruppe der Fettsäure ii) des Hilfsmittels 8 bis 20 Kohlenstoffatome enthält.

24. Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 23, wobei die Acylgruppe der Fettsäure ii) des Hilfsmittels 14 bis 20 Kohlenstoffatome enthält.

25. Verwendung eines Hilfsmittels gemäß irgendeinem der Ansprüche 1 bis 8 zur Herstellung einer pharmazeutischen Zusammensetzung, um die Immunreaktion gegenüber einem Antigen in einem Tier, einschließlich eines Menschen, zu verstärken.

26. Verwendung einer Impfstoff-Zusammensetzung gemäß irgendeinem der Ansprüche 9 bis 24 zur Herstellung einer pharmazeutischen Zusammensetzung, um einen Menschen oder ein Tier zu immunisieren.

Revendications

1. Adjuvant à utiliser dans un vaccin, l'adjuvant contenant

i) un monoglycéride ayant une pureté d'au moins 80% p/p, le monoglycéride ayant la formule

dans laquelle R est choisi parmi H et un groupe acyle contenant de 6 à 24 atomes de carbone à la condition que deux des groupes R soient H, et

ii) un acide gras avec 6 à 24 atomes de carbone, la chaîne acyle de l'acide gras étant saturée ou insaturée,

iii) de l'eau,

dans lequel la concentration de i) est de 0,1 g à 50 g pour 100 ml d'eau et la concentration de ii) est de 1 g à 50 g pour 100 ml d'eau, et dans lequel l'administration de l'adjuvant à un humain ou à un animal provoque une réponse immunitaire chez l'humain ou l'animal contre un antigène administré à l'humain ou à l'animal.

2. Adjuvant selon la revendication 1, dans lequel le vaccin contient un composant d'antigène.

3. Adjuvant selon la revendication 1, dans lequel la pureté du monoglycéride i) est d'au moins 90 %.

4. Adjuvant selon la revendication 1, dans lequel la pureté du monoglycéride i) est d'au moins 95 %.

5. Adjuvant selon la revendication 1, dans lequel le groupe acyle du monoglycéride i) contient de 8 à 20 atomes de carbone.

6. Adjuvant selon la revendication 1, dans lequel le groupe acyle du monoglycéride i) contient de 14 à 20 atomes de carbone.

7. Adjuvant selon la revendication 1, dans lequel le groupe acyle de l'acide gras ii) contient de 8 à 20 atomes de carbone.

8. Adjuvant selon la revendication 1, dans lequel le groupe acyle de l'acide gras ii) contient de 14 à 20 atomes de carbone.

9. Composition de vaccin comprenant un adjuvant selon l'une quelconque des revendications 1 à 8 et une quantité immunogénique d'un composant d'antigène.

10. Composition de vaccin selon la revendication 9, dans laquelle le composant d'antigène est capable d'entraîner la formation d'une réponse immunitaire chez des animaux, incluant des humains et des animaux marins.

11. Composition de vaccin selon la revendication 9 ou 10, dans laquelle le composant d'antigène est choisi dans le groupe consistant en des antigènes de bactéries, de virus, de parasites et de cellules tumorales pathogéniques ou non pathogéniques.

12. Composition de vaccin selon l'une quelconque des revendications 9 à 11 contenant, pour 100 g de la composition finale :

de 0,1 à 50 g d'un monoglycéride i)

de 1 à 50 g d'un acide gras ii)

de 0,01 à 90 g du composant d'antigène

de 0,01 à 99 g d'eau

de 0,01 à 99 g de solution PBS ou de solution saline.

13. Composition de vaccin selon l'une quelconque des revendications 9 à 12, dans laquelle la composition comprend des excipients pharmaceutiques supplémentaires choisis dans le groupe consistant en des conservateurs, des agents de contrôle de la pression osmotique, des agents de contrôle du pH, des solvants organiques, des inhibiteurs enzymatiques, des polymères absorbant l'eau, des promoteurs d'absorption et des agents anti-oxydants.

14. Composition de vaccin selon l'une quelconque des revendications 9 à 13, dans laquelle la composition comprend des adjuvants supplémentaires.

15. Composition de vaccin selon l'une quelconque des revendications 9 à 14, dans laquelle la composition est sous une forme adaptée à l'administration parentérale ou muqueuse.

16. Composition de vaccin selon la revendication 15, dans laquelle la composition est sous une forme adaptée à l'administration sur la muqueuse du nez, de la bouche, du vagin, du rectum ou de l'intestin.

17. Composition de vaccin selon la revendication 15, dans laquelle la composition est sous une forme adaptée pour administration sur la muqueuse du nez.

18. Composition de vaccin selon l'une quelconque des revendications 9 à 17, dans laquelle le composant d'antigène est choisi dans le groupe consistant en l'anatoxine diphtérique, le virus influenza et un rotavirus.

19. Composition de vaccin selon l'une quelconque des revendications 9 à 18, dans laquelle la pureté du monoglycéride i) de l'adjuvant est d'au moins 90 %.

20. Composition de vaccin selon l'une quelconque des revendications 9 à 19, dans laquelle la pureté du monoglycéride i) de l'adjuvant est d'au moins 95 %.

21. Composition de vaccin selon l'une quelconque des revendications 9 à 20, dans laquelle le groupe acyle du monoglycéride i) de l'adjuvant contient de 8 à 20 atomes de carbone.

22. Composition de vaccin selon l'une quelconque des revendications 9 à 21, dans laquelle le groupe acyle du monoglycéride i) de l'adjuvant contient de 14 à 20 atomes de carbone.

23. Composition de vaccin selon l'une quelconque des revendications 9 à 22, dans laquelle le groupe acyle de l'acide gras ii) de l'adjuvant contient de 8 à 20 atomes de carbone.

24. Composition de vaccin selon l'une quelconque des revendications 9 à 23, dans laquelle le groupe acyle de l'acide gras ii) de l'adjuvant contient de 14 à 20 atomes de carbone.

25. Utilisation d'un adjuvant selon l'une quelconque des revendications 1 à 8 pour la production d'une composition pharmaceutique pour stimuler une réponse immunitaire à un antigène chez un animal, y compris un humain.

26. Utilisation d'une composition de vaccin selon l'une quelconque des revendications 9 à 24 pour la production d'une composition pharmaceutique pour immuniser un humain ou un animal.