AU2008201215B2 - Poxvirus containing formulations and process for preparing stable, poxvirus containing compositions - Google Patents
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Description
I Poxvirus containing formulations and process for preparing stable, poxvirus containing compositions The present invention relates to a formulation, in particular an aqueous formulation comprising (i) a poxvirus of one of the genera orthopoxvirus, avipoxvirus, parapoxvirus, capripoxvirus and suipoxvirus, (ii) a disaccharide, (iii) a pharmaceutical acceptable polymer and optionally (iv) a buffer. The aqueous formulation is particularly suitable for freeze-drying processes resulting in a stable, freeze-dried, poxvirus containing composition. The invention further concerns a method for preparing a freeze-dried, poxvirus containing composition and the thus obtained product. Background of the invention The reference to any prior art in this specification is not, and should not be taken as an acknowledgement or any form of suggestion that such art forms part of the common general knowledge in Australia. Throughout this specification and the claims, unless the context requires otherwise, the word "comprise" and its variations, such as "comprises" and "comprising," will be understood to imply the inclusion of a stated integer or step or group of integers or steps but not the exclusion of any other integer or step or group of integers or steps. The poxviridae comprise a large family of complex DNA viruses that replicate in the cytoplasm of vertebrate and invertebrate cells. In humans smallpox was by far the most important poxvirus infection. The causative agent of smallpox is the variola virus, a member of the genus Orthopoxvirus. Vaccinia virus, also a member of the genus Orthopoxvirus in the family of Poxviridae, was used as live vaccine to immunize against smallpox. Successful worldwide vaccination with Vaccinia virus culminated in the eradication of variola virus (The global eradication of smallpox. Final report of the global commission for the 2 certification of smallpox eradication; History of Public Health, No. 4, Geneva: World Health Organization, 1980). In the meantime, most of the stocks of infectious variola viruses have been destroyed. However, it can not be excluded that poxviruses inducing smallpox or smallpox-like diseases might again become a major health problem. Thus, it is necessary to be in a position to produce stable vaccines against poxvirus infections, in particular variola infections, such as vaccines based on vaccinia virus. In the past vaccinia viruses have also been used to engineer viral vectors for recombinant gene expression and for the potential use as recombinant live vaccines (Mackett, M. , Smith, G. L. and Moss, B. [1982] P. N. A, S. USA 79, 7415-7419; Smith, G. L., Mackett, M. and Moss, B. [1984] Biotechnology and Genetic Engineering Reviews 2, 383-407). This entails inter alia DNA sequences (genes), which code for foreign antigens being introduced into the genome of the Vaccinia viruses with the aid of DNA recombination techniques. If the gene is integrated at a site in the viral DNA which .is non-essential for the life cycle of the virus, it is possible for the newly produced recombinant Vaccinia virus to be infectious, i. e. the virus is able to infect foreign cells and thus to express the integrated DNA sequence (EP 83286 and EP 110385). The recombinant Vaccinia viruses prepared in this way can be used, on the one hand, as live vaccines for the prophylaxis of infectious diseases and on the other hand, for the preparation of heterologous proteins in eukaryotic cells. Other examples for recombinant vaccinia viruses are viruses harboring therapeutic genes such as suicide genes, ribozyme genes or antisense genes. Modified Vaccinia virus Ankara (MVA) is known to be exceptionally safe. MVA has been generated by long-term serial passages of the Ankara strain of Vaccinia virus (CVA) on chicken embryo fibroblasts (for review see Mayr, A., Hochstein-Mintzel, V. and Stickl, H. [1975] Infection 3,6-14 ; Swiss Patent No. 568,392). Examples for MVA virus strains deposited in compliance with the requirements of the Budapest Treaty are strains MVA 572 deposited at the European Collection of Animal Cell Cultures (ECACC), Salisbury (UK) with the deposition number ECACC V94012707, MVA 575 deposited under ECACC V00120707 and MVA-BN with the deposition number ECACC V00083008. MVA is distinguished by its great attenuation that is to say by diminished virulence or infectiosity while maintaining good immunogenicity. The MVA virus has been analyzed to determine alterations in the genome relative to the wild type CVA strain. Six major deletions of genomic DNA (deletion 1, 11, lit, IV, V, and VI) totaling 31,000 base pairs have been identified (Meyer, H., Sutter, G. and Mayr A. [1991] J. Gen. Virol. 72, 1031-1038). The resulting MVA virus became severely host cell restricted to avian cells. Furthermore, MVA is characterized by its extreme attenuation. When tested in a variety of animal models, MVA was proven to be virulent even in immunosuppressed animals. More importantly, the excellent properties of the MVA strain have been demonstrated in extensive clinical trials (Mayr et al., Zbl. Bakt, Hyg. 1, Abt. Org. B 167,375-390 [1987], Stickl et al., Dtsch. med. Wschr. 99, 2386-2392 [1974]). During these studies in over 120,000 humans, including high-risk patients, no side effects were associated with the use of MVA vaccine. Recombinant MVA useful as vaccines have already been constructed (see, e. g. , WO 97/. 02355) and are used in clinical trials. WO 98/13500 discloses a recombinant MVA containing and capable of expressing DNA sequences encoding dengue virus antigens. The foreign DNA sequences were recombined into the viral DNA at the site of a naturally occurring deletion in the MVA genome. An MVA strain showing an even stronger attenuation and enhanced safety characteristics is the strain MVA-BN, deposited at the European Collection of Animal Cell Cultures (ECACC), Salisbury, UK with the deposition number V00083008.
4 Besides vaccinia virus other poxviruses have been used as vectors to deliver genetic information into mammalian cells. In this context reference is made to avipox viruses such as fowlpoxvirus. Fowlpoxviruses containing HIV genes in the genome are disclosed in US 5,736, 368 and US 6,051, 410. Processes for preparing poxvirus containing compositions suitable as vaccines are known to the person skilled in the art (see for example Joklik W. K., Virology (1962), 18,9-18 ; Richter, K. H., Abhandlungen aus dem Bundesgesundheitsamt (1970), 9,53-57). The known purification results in aqueous, poxvirus containing solutions or in poxvirus containing sediments. The poxviruses in these solutions and sediments are not stable, i. e. the infectivity of the viruses rapidly decreases. However, it is necessary that a vaccine can be stored and distributed in a stabilized form, especially when the vaccines need to be transported in tropical regions with limited distribution infrastructure. A freeze-dried product can be stored at temperatures in the range from 4* C to 25* C. This is a clear advantage compared to the standard storage conditions for liquid formulations, which have to be stored below -20'C (Cryopreservation and freeze-drying protocols "Day J, McLellan M; Methods in Molecular Biology, 38,1995, Humana Press). Processes for the freeze-drying of poxviruses, in particular vaccinia virus, and virus containing compositions and solutions suitable for this purpose are known (Burke et al-, Critical Reviews in Therapeutic Drug Carrier Systems (1999), 16,1-83). In general terms freeze-drying of a vaccine involves freezing of the vaccine containing aqueous formulation suitable for freeze-drying, followed by removing water by sublimation under conditions of reduced pressure and low temperatures and further followed by removal of water by desorption under conditions of reduced pressure and higher temperatures.
The known poxvirus-containing formulations for freeze-drying have important disadvantages. Many of the known vaccinia virus containing compositions for freeze-drying contain peptone or haemaccel, which are often of animal origin. However, there are concerns that animal diseases such as BSE could be transmitted from animal to man via animal products such as peptone, gelatine or haemaccel. Moreover, the poxviruses in the known virus containing formulations for freeze-drying have not been purified. Thus, the poxvirus containing compositions for freeze-drying known in the prior art contain inter alia large amounts of proteins derived from the cells of the cell or tissue culture system and from the bovine serum used during cell cultivation, respectively. The person skilled in the art also knows freeze-drying compositions that do not contain additional compounds of animal origin (which are e. g. peptone or haemaccel). In this case the compositions contain the following compounds alone or in certain combinations: sodium glutamate, sorbitol, lactose, salts, amino acids and glycerin. However, the product obtained after the freeze drying process is often rather unstable, i. e. the overall loss in virus titer is unacceptably high during storage. Moreover, it has been shown that the poxvirus tends to form aggregates in some of these formulations and that other compounds precipitate before or during freezing. US 3,577, 526 discloses a smallpox vaccine characterized by the fact that it is made up of a ground virus material of the vaccine dispersed in sucrose. The amount of sucrose is in the range of 20 to 40 %. The formulation may further comprise 5% dextran. The term ground virus refers to virus derived from pulps and pustules. Basically, the lymph is ground to break up lumps and separate the liquid from the dead hair and skin, Thus, the protein load of the vaccine preparation is very high and contributes to the stabilization of the virus.
6 Summary of the invention In one aspect the present invention provides a poxvirus containing formulation, in particular an aqueous poxvirus containing formulation, for freeze-drying which leads to a stable freeze-dried product, wherein the poxvirus is preferably a purified or at least partially purified virus. In a further aspect, the present invention provides an aqueous poxvirus containing formulation in which the poxviruses do not tend to aggregate and in which the components do not precipitate before or during freezing. In another further aspect, the present invention provides a poxvirus containing formulation, in particular an aqueous poxvirus containing formulation, comprising low amounts of non-poxvirus associated proteins. In yet a further aspect, the present invention provides a stable, freeze-dried, poxvirus containing composition and a method for obtaining said composition. Detailed description of the invention The present invention provides poxvirus containing formulation, in particular an aqueous poxvirus containing formulation. The formulation, in particular the aqueous formulation may be suitable for freeze-drying of said poxvirus. Furthermore, the invention provides the freeze-dried, poxvirus containing product. The formulation according to the present invention, in particular the aqueous formulation, comprises the poxvirus, a disaccharide, a pharmaceutical acceptable polymer and optionally further a buffer. Although the freeze-dried formulation according to the present invention neither contains stabilizing additives of animal origin such as peptone, gelatine, haemaccel nor high amounts of proteins derived from the system used to amplify the virus (such as cell culture systems), the virus in the formulation is surprisingly stable, i. e. the poxvirus in the freeze-dried WO 03/053463 PCT/EP02/13434 7 composition remains infectious for long periods of time, even at high storage temperatures such as room temperature or 37 *C. if not specified otherwise the term "room temperature" as used in the 5 present specification corresponds to a temperature of 20 to 25 0C. The poxviruses to be freeze-dried are any poxviruses selected from the group consisting of Orthopoxviruses, Parapoxviruses, Avipoxviruses, Capripoxviruses and Suipoxviruses. These viruses might be useful as a io vaccine for human beings or animals (Virology, 3 rd edition, 1995, ed.-in chief: Fields, B.N.). Particularly preferred poxviruses are viruses of the genera Orthopoxvirus or Avipoxvirus. Preferred examples of poxviruses belonging to the genus avipoxvirus are canarypoxvirus and fowlpoxvirus. Preferred examples belonging to the family Orthopoxvirus are cowpoxvirus 15 and vaccinia virus. The poxvirus contained in the formulation according to the present invention can be a naturally occurring poxvirus, an attenuated poxvirus or a recombinant poxvirus. 20 For vaccination of human beings against smallpox the poxvirus in the formulation is preferably a vaccinia virus strain. Examples for vaccinia virus strains suitable for this purpose are the strains Temple of Heaven, Copenhagen, Paris, Budapest, Dairen, Gam, MRIVP, Per, Tashkent, TBK, 25 Tom, Bern, Patwadangar, BIEM, B-15, Lister, EM-63, New York City Board of Health, Elstree, Ikeda and WR. The most preferred vaccinia virus strains are modified vaccinia virus strain Ankara (MVA) and its derivatives, in particular the strain that has been deposited at ECACC with the deposition number V00083008 and strain Elstree. 30 WO 03/053463 PCT/EP02/13434 8 The poxvirus in the formulation according to the present invention is preferably a poxvirus that is essentially apathogen in the animal or subject to be vaccinated. For this purpose it is preferred either to use attenuated virus strains or to use a poxvirus that naturally replicates in a host species 5 different from the species to be vaccinated and that is not pathogenic in the heterologous host. An "attenuated virus" is a virus originating from a pathogenic virus but that upon infection of the host organism leads to a lower mortality and/or 1o morbidity compared to the non-attenuated parent virus. Examples of attenuated poxviruses are known to the person skilled in the art. Most preferred is modified vaccinia virus Ankara (MVA). Typical MVA strains are MVA 575 and MVA 572 that have been deposited at the European Collection of Animal Cell Cultures under the deposition numbers ECACC V00120707 15 and ECACC V 94012707, respectively. Most preferred is MVA-BN or a derivative thereof, which has been described in WO 02/42480 (PCT/EPO1/13628). The content of this application is included in the present application by reference. MVA-BN has been deposited at the European Collection of Animal Cell Cultures with the deposition number 20 ECACC V00083008. Examples of poxviruses for which human beings are heterologous hosts and which are not pathogenic in human beings are fowlpoxvirus or canarypoxvirus. 25 The term "recombinant virus" refers to any virus having inserted into the viral genome a heterologous gene that is not naturally part of the viral genome. A heterologous gene can be a therapeutic gene, a gene coding for a peptide comprising at least one epitope to induce an immune response, an 3o antisense expression cassette or a ribozyme gene. Methods to construct WO 03/053463 PCT/EP02/13434 9 recombinant viruses are known to a person skilled in the art. The most preferred poxvirus vector is MVA, in particular MVA 575 and MVA-BN (see above) 5 It is known to the person skilled in the art how poxviruses can be amplified and recovered from infected cell cultures. Generally, in a first step eukaryotic cells are infected with the poxvirus that is intended to be part of the formulation according to the present invention. The eukaryotic cells are cells that are susceptible to infection with the respective poxvirus and allow 10 replication and production of infectious virus. Such cells are known to the person skilled in the art for all poxviruses. For MVA an example for this type of cells are chicken embryo fibroblasts (CEF) (Drexler I. et al., J. Gen. Virol. (1998), 79, 347-352). CEF cells can be cultivated under conditions known to the person skilled in the art. Preferably the CEF cells are cultivated in serum 15 free medium. The incubation time preferably is 48 to 96 hours at 370 C ± 2* C. For the infection poxviruses are used at a multiplicity of infection (MOI) of 0,05 to 1 TCID 50 (TCID= tissue culture infectious dose) and the incubation takes place 48 to 72 hours at the same temperature. 20 Progress of infection can be observed by looking at cytopathic effects (CPE), typically a significant rounding of the infected cells. Poxviruses are known to exist in two different forms: poxvirus attached to cellular membranes in the cytoplasm of the infected cells (intracellular 25 mature virions (IMV)) and viruses that have been externalized (extracellular enveloped virions (EEV)) (Vanderplasschen A. et al., J. Gen. Virol. (1998), 79, 877-887). Both viral forms can be used in the formulations according to the present invention. The EEVs can simply be obtained from the supernatant by centrifugation and may be directly suspended in an aqueous 30 formulation including a disaccharide and a pharmaceutically acceptable WO 03/053463 PCT/EP02/13434 10 polymer. However, the virus-containing fractions may comprise cellular detritus and other contaminants. Especially for vaccination of human beings it is thus preferred that the virus is further purified before it is included into a formulation according to the present invention. Methods for the 5- purification of poxviruses are known to the person skilled in the art. The purification step can be e.g. batch centrifugation (e.g. using sucrose cushions) or continuous-flow ultracentrifugation (sucrose gradients), ultrafiltration (e.g. cross-flow filtration using a membrane with a pore size bigger than 500 kDa, but equal or smaller than 0,1 pm), column 10 chromatography (e.g. ion exchange, hydrophobic interaction, size exclusion or a combination) or a combination of some or all of the above (Masuda N. et al., J Bacteriol (1981) 147, 1095-1104). In order to obtain IMVs the cells have to be harvested in a first step and 15 disrupted in a second step. If the infected cells are cells that can be cultivated in suspension culture the infected cells can easily be harvested by centrifugation. If the infected cells are more or less intact adherent cells it is possible to harvest the cells, i.e. to remove the cells from the culture vial, before subjecting them to the disruption step. Harvesting methods are 20 known to the person skilled in the art. Useful techniques are mechanic methods (e.g. by using a rubber cell scraper), physical methods (e.g. freezing below -15* C and thawing the culture vessels above +15* C) or biochemical methods (treatment with enzymes, e.g. Trypsin, in order to detach the cells from the culture vessel). If enzymes are used for this 25 purpose the incubation time should be controlled, since the enzymes might also damage the virus after prolonged incubation times. Methods for the disruption of cells are also known to the person skilled in the art. The freezing-thawing method described above already results in a 30 partial disruption of the cells. Other known techniques for the disruption of WO 03/053463 PCT/EP02/13434 11 cells include the use of ultrasound. The ultrasound treatment of cells results in a virus containing homogenate. For vaccination of animals the poxvirus containing homogenate could be used inthe formulations according to the present invention. However, it is 5 again preferred to use poxviruses that have been purified at least partially. As outlined above such purification methods are known to the person skilled in the art. The poxviruses are contained in the formulation, in particular in the aqueous 10 formulation in a concentration range of 104 to 109 TCID 50 /ml, preferably in a concentration range of e.g. 105 to 5x10 8 TCID 50 /ml, most preferably in a concentration range of e.g. 106 to 108 TCID 50 /ml. The actual concentration depends on the amount of virus to be administered to the human being or animal, which in turn depends on the type of virus to be administered. For 15 the vaccinia virus strain Elstree a typical vaccination dose for humans comprises 2.5 x 10 5
TCID
50 . For the vaccinia virus strain MVA-BN a typical vaccination dose for humans comprises 1 x 108 TCID 50 . As pointed out above the poxvirus in the formulation according to the 20 present invention is preferably a purified or at least partially purified virus. The term "purified or at least partially purified virus" refers to the fact that the virus used in the formulation according to the present invention has a purity that is higher than that of the unpurified virus ("ground virus") as used in the vaccines used until the eradication of smallpox (such as 25 disclosed in US 3,577,526). Such a higher purity can be obtained e.g by one or more of the following methods: batch centrifugation (e.g. using sucrose cushions) or continuous-flow ultracentrifugation (sucrose gradients), ultrafiltration (e.g. cross-flow filtration using a membrane with a pore size bigger than 500 kDa, but equal or smaller than 0,1 pm), column 30 chromatography (e.g. ion exchange, hydrophobic interaction, size exclusion WO 03/053463 PCT/EP02/13434 12 or a combination). Particularly preferred is ultrafiltration and/or batch centrifugation by using sucrose cushions. In more general terms the term "purified or at least partially purified virus" refers to virus preparations (such as preparations comprising MVA or Elstree) having a titer of at least 106, 5 preferably of at least 107, more preferably of at least 108, even more preferably of at least 5 x 10 TlDo 50 per mg total protein. For strain Elstree typical preparations have a titer of 8 x 108 TCID 50 per mg total protein. Methods how to determine the titer of a poxvirus containing preparation are known to the person skilled in the art; one of these methods is outlined in io the example section. The total protein content is preferably determined according to the method of Kjeldahl (Lynch, J.M. and Barbano, D.M., Kjeldahl nitrogen analysis as a reference method for protein determination in dairy products. J AOAC Int. 1999 Nov-Dec; 82(6):1389-98. Review). It is to be noted that the total protein content is the sum of viral proteins and 15 cellular proteins. It was unexpected that a formulation comprising a purified or partially purified virus, a disaccharide and a pharmaceutically active polymer is stable, since it was believed that the large amounts of non-virus protein in 20 the unpurified virus preparations contributed to the stability of the prior art formulations. The formulation according to the present invention, in particular the aqueous formulation, comprises a disaccharide. In contrast to monosaccharides such 25 as glucose which give a good bioprotection during freeze-drying but which have a low collapse temperature and often freeze-dry with collapse, disaccharides have been shown to be effective freeze-drying protectants displaying higher collapse temperatures than monosaccharides.
WO 03/053463 PCT/EP02/13434 13 The disaccharides comprised in the formulations according to the present invention are pharmaceutically acceptable disaccharides having a collapse temperature (Tc) in a range of about -25 'C to -35 *C. Typical collapse temperatures are -31 *C for sucrose, - 28.5 0C for trehalose and -30.5 *C for 5 lactose. Typical collapse temperatures for the entire formulation according to the present invention are preferably in the range of - 50 'C to -20 *C. Preferred subranges are e.g. -37 *C to -30*C, -36 *C to -31 0C or -35.7 to 31.2 *C. 1o Preferably the disaccharide is selected from the group consisting of trehalose, lactose and sucrose. Most preferred is sucrose. The disaccharide, preferably sucrose, is contained in the formulation according to the present invention, in particular the aqueous formulation, preferably in a concentration range of 10-100 g/l, more preferably in a range of 20- 80 g/l, 15 most preferably in a range of 25-60 g/l. For sucrose a typical concentration is 45 g/l. The formulation according to the present invention, in particular the aqueous formulation, further comprises a pharmaceutically acceptable polymer. The 20 polymer is preferably selected from the group consisting of dextran and polyvinylpyrrolidon (PVP). The polymer used has to be soluble in the formulation according to the present invention. If dextran is used its molecular weight is preferably in the range of 20,000 to 100,000, more preferably in the range of 30,000 to 70,000, most preferably in the range of 25 36,000 to 44,000. The most preferred dextran has an average molecular weight of 40,000. The concentration of dextran is in the range of 1 to 50 g/l, preferably in a range of 2 to 40 g/l or 3 to 30 g/l. Particularly good results have been observed in the ranges of 5 to 50 g/l, 5. to 40 g/l or 5 to 30 g/l. Even more preferred is the range of 8 to 30 g/1l. The most preferred range is 30 10 to 27 g/l. An example for a preferred concentration is 18.9 g/l. The WO 03/053463 PCT/EP02/13434 14 preferred concentrations and concentration ranges of Dextran as shown above, in particular the range of 5 to 50 g/l and the corresponding subranges, have the particular advantage that the collapse temperature of the formulation is relatively high, which makes it possible to carry out the 5 process in an industrial scale. If PVP is used its molecular weight is preferably in the range of 50,000 to 400,000, more preferably in a range of 70,000 to 360,000. The concentration of PVP is in the range of 5 to 200 g/l, more preferably in a range of 5 to 100 g/l, most preferably in a range of 10 to 40 g/l. 10 The formulation according to the present invention, in particular the aqueous formulation, further may comprise a buffer. As pointed out above it was one of the objects of the present invention to provide an aqueous poxvirus containing formulation in which the poxviruses do not aggregate and in 15 which no precipitation occurs upon drying. It has been shown unexpectedly that such undesired effects are correlated with the presence of a buffer containing phosphate in the aqueous formulation. Examples for phosphate containing buffer are PBS (phosphate buffered saline) and phosphate buffer. Consequently, this particular object of the invention is solved by an aqueous 20 formulation for freeze-drying that does not contain a phosphate buffer. Thus, the buffer contained in the formulation according to the present invention is preferably selected from the group consisting of TRIS, TBS, MOPS, HEPES and (bi-)carbonate buffers. The most preferred buffers are TRIS and TBS. 25 The buffer is used in a concentration that is sufficient to exert the required buffer capacity. For TRIS buffers the preferred concentration range is 1-50 mM; the most preferred concentration is 10 mM. The pH is preferably adjusted to a value that on the one hand is pharmaceutically acceptable for administration in human beings or animals and that on the other hand is not WO 03/053463 PCT/EP02/13434 15 detrimental to the virus. Thus the pH should be in the range of 6.0 to 9.0, more preferably in the range of 7.2 to 7.8. The most preferred pH is 7.4. The unexpectedly good results by using a phosphate free buffer are obtained 5 irrespectively of whether the virus in the formulation is an unpurified, purified or partially purified virus. Purified or partially purified viruses are preferred. The formulation according to the present invention, in particular the aqueous 1o formulation may contain salts such as NaCl. Typical concentrations for NaCl are in the range of 10 to 200 mM. An example for a preferred NaCl concentration is 140mM. The formulation according to the present invention, in particular the aqueous 15 formulation further may comprise L-glutamic acid salts. The salt is preferably a monopotassium salt or a monosodium salt. The concentration of the L-glutamic acid salt is preferably in a range of 0.05 - 0.5 g/l, more preferably in a range of 0.1 - 0.15 g/l. 20 Some particularly preferred aqueous formulations according to the present application are listed in the following table 1. In all formulations listed in table 1 the buffer is 10 mM TRIS, pH 7.4, 140 mM NaCl. Table 1: Modified First Second Third Run in table 6 Vaccinia additive additive additive Virus [g/l] [gi/l] [g/l] Ankara
(MVA)
WO 03/053463 PCT/EP02/13434 16
[TCID
50 /ml] 5x10 8 25 10.5 0.06 (L- GT 8 (sucrose) (dextran) glutamic acid) 5x10 8 34.5 14.5 0.083 (L- GT 8 (sucrose) (dextran) glutamic acid) 5x10 8 45 18.9 0.108 (L- GT 9 (sucrose) (dextran) glutamic acid) 5x10 8 60 25.2 0.144 (L- GT 9 (sucrose) (dextran) glutamic acid) 1x10 8 45 18.9 0.108 (L (sucrose) (dextran) glutamic acid) 1x10 8 45 3.78 0.108(L (sucrose) (dextran) glutamic acid) The aqueous formulation according to the present invention is suitable for freeze-drying. For administration the freeze-dried product has to be reconstituted with an appropriate solvent. According to one embodiment 5 sterile water is added to the freeze-dried product in order to bring the compounds into solution. Preferably, the amount of added water corresponds more or less to the amount of water that has been eliminated during freeze-drying. Thus, according to this embodiment the composition of the reconstituted product is more or less identical to the initial aqueous 10 formulation. It is therefore within the scope of the present invention that the WO 03/053463 PCT/EP02/13434 17 aqueous formulation according to the present invention is used as a vaccine. According to an alternative embodiment the freeze-dried product may also be reconstituted in any other pharmaceutically acceptable diluent that may be used in appropriate amounts. By way of example the diluent may be 5 water comprising one or more of the compounds selected from phenol, glycerol and buffer. The concentration of phenol in the reconstituted product is e.g. 0.5%. As pointed out above, the buffer is preferably not a phosphate buffer. 10 In summary, this aspect of the invention concerns inter alia the following particularly preferred embodiments: (1) A formulation, in particular an aqueous formulation, comprising or even consisting of a purified or partially purified poxvirus selected from the group consisting of Orthopoxviruses, Parapoxviruses, Avipoxviruses, Capripoxviruses and Suipoxviruses, a 15 disaccharide, a pharmaceutically acceptable polymer and optionally a buffer, wherein the buffer is preferably not a phosphate buffer. Preferably the polymer is dextran, preferably in the amounts as specified above. (II) A formulation, in particular an aqueous formulation, comprising or even consisting of a poxvirus selected from the group consisting of 20 Orthopoxviruses, Parapoxviruses, Avipoxviruses, Capripoxviruses and Suipoxviruses, a disaccharide, a pharmaceutically acceptable polymer and a buffer, wherein the buffer is not a phosphate buffer and wherein the poxvirus is preferably a purified or partially purified virus. Preferably the polymer is dextran, preferably in the amounts as specified above. (111) A formulation, in 25 particular an aqueous formulation, comprising or even consisting of a poxvirus selected from the group consisting of Orthopoxviruses, Parapoxviruses, Avipoxviruses, Capripoxviruses and Suipoxviruses, a disaccharide, a pharmaceutically acceptable polymer and optionally a buffer, wherein polymer is dextran in the amounts as specified above, by way of 30 example preferably in the range of 5 to 40 g/l. Preferably the buffer is not a WO 03/053463 PCT/EP02/13434 18 phosphate buffer. Preferably the poxvirus is a purified or partially purified virus. The term "consisting" as used in the context of options (1), (11) and (Ill) 5 above, refers to formulations consisting of the above-mentioned compounds only and to formulations containing in addition one or more salts. Examples of salts that may be added to the formulations (1), (II) and (ll) consisting of the above defined compounds are KCI, NaCl, sodium-glutamate. Thus, the term "consisting" in the definition of the above defined formulations (1), (Il) 10 and (111) does not exclude the possibility to add one or more salts. By way of example a specific embodiment of the present invention comprises an aqueous formulation comprising a purified or partially purified poxvirus selected from the group consisting of Orthopoxviruses, Parapoxviruses, 15 Avipoxviruses, Capripoxviruses and Suipoxviruses, a disaccharide, a pharmaceutically acceptable polymer and a buffer, wherein the disaccharide is sucrose in the above specified amounts, wherein the polymer is dextran in the above specified amount and wherein the buffer is not a phosphate buffer. By way of example another specific embodiment of the present invention 20 comprises an aqueous formulation consisting of a poxvirus selected from the group consisting of Orthopoxviruses, Parapoxviruses, Avipoxviruses, Capripoxviruses and Suipoxviruses, a disaccharide, a pharmaceutically acceptable polymer and optionally a buffer. The poxvirus is preferably a purified or partially purified poxvirus. Preferred amounts and examples of 25 the disaccharide, the polymer and the buffer are outlined above. It is within the skills of the practitioner how such formulations, in particular an aqueous formulations containing poxviruses can be administered and which amounts of virus are used for vaccination. As pointed out above the 30 vaccines might be used to induce an immune response against the WO 03/053463 PCT/EP02/13434 19 poxviruses itself, in particular if attenuated or non-pathogenic, non recombinant poxviruses are used. If the poxviruses are recombinant poxviruses an immune response is additionally raised against the recombinant protein/peptide expressed by the poxvirus vector. 5 The term "formulation" as used above usually refers to liquid formulations, preferably to aqueous formulations, if not stated otherwise. If the concentrations or concentration ranges are defined in "mM", "g/l" and so on this is an indication that the respective formulation is a liquid or even 1o aqueous formulation . The term "aqueous formulation" relates to those formulations in which the diluent is water. However, the scope of the present invention also covers those dry formulations that can be obtained from a liquid or even aqueous formulation according to the present invention by removal of the liquid, irrespective of the method that is used for said 15 removal. Thus, the invention also covers those dry formulations that are obtained by methods other than freeze-drying. In particular, the present invention further relates to a method for preparing a stable, poxvirus containing composition characterized in that the 20 formulation according to the present invention, in particular the aqueous formulation is freeze-dried. In the present application the terms "stable, poxvirus-containing composition" and "freeze-dried poxvirus containing composition" are used interchangeably if not stated otherwise. The term "stable, poxvirus containing composition" is used in the present application 25 to define poxvirus-containing compositions in which the overall loss in virus titer at an incubation temperature of 37 OC during 28 days is less than 0.5 logs, preferably less than 0.4 logs. A detailed protocol to determine the virus titer and thus the overall, loss in virus titer is given in the example section. However, any other protocol to determine the viral titer can also be used. 30 WO 03/053463 PCT/EP02/13434 20 Methods of freeze-drying are generally known to the person skilled in the art (Day, J. and McLellan, M., Methods in Molecular Biology, Humana Press, (1995) vol. 38). A freeze-drying process usually consists of the following steps, which are 5 explained in more detail below: 1. Vaccine preparation; 2. Sample freezing; 3. Primary drying (sublimation); 4. Secondary drying (desorption); 10 5. Product stoppering and removal; 6. Vaccine storage; 7. Reconstitution. Vaccine preparation: The production and amplification of poxviruses to be 15 used as vaccines has been explained in detail above. The poxviruses are optionally purified. The formulation according to the present invention is obtained by adding the above defined disaccharides, polymers and, optionally, buffer, L-glutamic acid and optionally further additives to the poxvirus preparation. 20 Sample freezing: Freezing of the sample does immobilize the components in the solution, thereby preventing product foaming when the pressure is reduced. Freezing is a two-step process during which water initially nucleates, followed by 25 growth of ice crystals, resulting in a mixture of ice and solute concentrate. Ice nucleation is encouraged by reducing the temperatures and agitating the cooled suspension. In contrast to nucleation, ice growth is encouraged by increasing temperature, thereby decreasing suspension viscosity. Regardless of the precise freezing pattern, proliferation of ice throughout the medium 30 results in an increase of solute concentration. Biopolymers in solution or WO 03/053463 PCT/EP02/13434 21 suspension are damaged or inactivated by exposure to these increasing concentrations of solute. Rapid cooling minimizes exposure of the bioproduct to the concentrate. Above a critical temperature (the glass transition temperature) the mass viscosity may decrease sufficiently so that 5 the glass softens and distorts. It dries to form a structureless sticky residue within the vial. The temperature of the distortion is termed the collapse temperature. More specifically the collapse temperature is defined as the temperature at which the mobility of the water in the interstitial region of the matrix becomes significant. To avoid the distortion the freezing temperature 10 has to be below the collapse temperature of the aquous formulation. The collapse temperature can be determined according to methods known by the person skilled in the art, e.g. by differential thermal analysis (Jennings, T.A., "Lyophilization, Introduction and Basic Principles", Interpharm Press, Denver, CO, US, 1999, ISBN 1-57491-081-7, pages 132-134). 15 If the temperature is too low, water diffusion from the virus may be inhibited, and injury by intracellular ice might occur. Consequently, the person skilled in the art will empirically test several freezing temperatures which are all below the collapse temperature of the aqueous formulation and he will test 20 which temperature leads to a freeze-dried product having the highest titer of infectious poxviruses. Primary drying (sublimation): The primary drying is that part of the freeze-drying process that drives the 25 sublimation of the solvent (ice) from the frozen matrix. The primary drying process starts after the freeze-dryer attains the required condenser temperature and chamber pressure. The pressure in the chamber is usually lower than 1 mbar, preferably lower than 0.2 mbar. Typically the pressure is in the range of 0.04 to 0.12 mbar. Throughout this specification these 30 conditions are sometimes referred to as "low pressure".
WO 03/053463 PCT/EP02/13434 22 The shelf temperature is increased such that sublimation of the ice in the product matrix occurs and the product temperature is significantly lower than the collapse temperature of the formulation to ensure a completely frozen matrix throughout the entire primary drying process and to ensure 5 freeze-drying without collapse. The temperature may remain constant during the whole primary drying process. Alternatively the shelf temperature can be increased continuously during the primary drying. However, the temperature of the product has to be below the collapse temperature during the whole primary drying process. At the end of the primary drying the dried product io still can contain more than 5% moisture (w/w). In order to obtain a product with a moisture content that will not longer support biological growth or chemical reactions it is necessary to carry out a secondary drying step. Secondary drying (desorption): 15 During secondary drying water vapor is desorbed from the surface of the cake that is formend during primary drying. This is accomplished by increasing the temperature while the chamber is still at low pressures so that water is desorbed from the cake surface. The shelf temperatures for the secondary drying are determined by the 20 stability of the product and may be in the range of 0 *C to +30 *C. The product temperature is usually in the range of -5 0C to 30 'C. More preferred is a temperature in the range of 5 0C to 20 *C. The secondary drying can be made in two steps. In a first step the product temperature may be in the range of -5 'C to +15 *C, preferably in the range of 0 *C to 25 +10 'C, more preferably in the range of 2 *C to +7 *C. The second step is made at a higher temperature than the secondary drying in the first step. The temperature may be in the range from 0 *C to 30 *C, preferably in the range of +5 OC to +20 C. Also the residual moisture content of the formulation depends on the requirements of the product. Some products 30 need higher, some products lower moisture content.-to achieve best product WO 03/053463 PCT/EP02/13434 23 stability. The optimal residual moisture content as well as the time to reach this has to be determined empirically. The secondary drying process is continued until the desired moisture is achieved. Methods to determine the moisture of a product are known to the 5 person skilled in the art. In particular the coulometric Karl-Fischer titration can be used (Jennings, T.A., "Lyophilization, Introduction and Basic Principles", Interpharm Press, Denver, CO, US, 1999, ISBN 1-57491-081-7, pages 415-418). The residual moisture content is preferably lower tkan 5%, more preferably in a range of 0.5 to 4%, even more preferably in a range of 1 10 to 3%. Product stoppering and removal: All product-containing vials are sealed according to methods known to the person skilled in the art. The vials can be sealed under very low pressure 15 (e.g. 0.04 - 2.56 mbar) directly in the freeze dryer. It is also possible to seal the vials under more or less normal pressure by using a chemically inert gas such as nitrogen or helium. Typically the vials may be sealed in a nitrogen atmosphere at a pressure of 900 mbar. The vials are closed, preferably by using butyl rubber stoppers. Once the product is stoppered the system can 20 be returned to atmospheric pressure and the shelf can be unloaded. Afterwards, the vials further may be sealed with aluminum caps for long term storage. Vaccine storage: 25 The freeze-dried product can be stored at room temperature (25 OC) and remains stable for at least 18 weeks, preferably at least 20 weeks more preferably at least 22 weeks at this temperature. "Stable at a certain temperature for a certain period of time" means that the loss of viral titer at this temperature is less than 0.5 logs during this time period. However, if 30 cooling is available it is preferred that the freeze-dried product is stored at WO 03/053463 PCT/EP02/13434 24 lower temperatures such as 4 *C. Preferably the product is stored in the dark. If this is not possible it is preferred to use coloured glass for storage or any other vials, which avoid a detrimental exposure to light. 5 Reconstitution. For reconstitution of the freeze-dried product an appropriate amount of a solvent is added to the freeze-dried product resulting in a pharmaceutically acceptable formulation allowing the administration to human beings or animals. The solvent is preferably water. Usually the solvent is added to the 10 formulation in an amount that corresponds substantially to the amount of solvent lost during the freeze-drying process. The invention concerns also the freeze-dried product obtained by the process according to the present invention. 15 Thus, the freeze-dried product according to the present invention comprises (i) a poxvirus, preferably of the genera orthopoxvirus or avipoxvirus, (ii) a disaccharide, (iii) a pharmaceutically acceptable polymer and optionally (iv) a buffer, wherein the pox virus, the disaccharide, the polymer and the buffer 20 are defined as above. Typical compositions in the freeze-dried product are shown in the following table 2. In all formulations shown in table 2 the amount of virus is 5 x 108
TCID
50 /ml. 25 Table 2: Amount of DSG 20 30 40 [%] in the aqueous formulation WO 03/053463 PCT/EP02/13434 25 before freeze drying (DSG: 63 g/l dextran MW 36.000-44.000, 150 g/l sucrose, 0.36 g/l L glutamic acid monopotassioum salt monohydrate) Sucrose[%] in 54.7 (36 58.7 (54 mg) 58.4 (72 mg) freeze-dried mg) product Dextran [%] in 23 (15.12 24.7 (22.68 24.6 (30.24 freeze-dried mg) mg) mg) product L-Glutamic acid 0.13 0.14 0.14 Monopotassium (0.0864 mg) (0.1296 mg) (0.1728 mg) salt Monohydrate [%] in freeze dried product Mean value freeze 65.8 92 123.1 dried cake [mg] (at filling of 1.2 ml) WO 03/053463 PCT/EP02/13434 26 The freeze-dried product according to the present invention is used for the preparation of a vaccine. To this end the freeze-dried product is resolved/reconstituted as described above and administered to a human being or an animal according to methods known to the person skilled in the 5 art. Brief explanations to the figures Figure 1 shows the stability of MVA containing freeze-dried formulation at a 10 temperature of 31 *C. The tested formulation is GT23 (see example section, and table 6). The virus titer in the aqueous formulation according to the present invention is determined before freeze-drying. Freeze-drying was made as described for GT23 (see examples and table 6). After freeze-drying the formulation was stored at 31 *C. At the indicated time points the freeze 15 dried formulation was reconstituted and the viral titer was again determined. Figures 2 and 3 show the results of the same experiment as described in the legend to figure 1 with the exception that the incubation temperature was 37 *C in Figure 2 and 45 0C in Figure 3. 20 WO 03/053463 PCT/EP02/13434 27 Examples The following examples will further illustrate the present invention. It will be well understood by a person skilled in the art that the provided example(s) in 5 no way may be interpreted in a way that limits the applicability of the technology provided by the present invention to this example(s). Example 1: Freeze-drying of formulations containing Modified Vaccinia Virus Strain Ankara (MVA) 10 In this example formulations according to the present invention containing MVA were freeze-dried under different conditions. The freeze-dried product was stored at different temperatures. The stability of MVA in the preparation was analyzed by determing the titer of MVA after reconstitution of the freeze 15 dried product and comparing it with the MVA titer before freeze-drying. The influence of different storage times on the viral titer was determined. The protocol for the determination of the titer of a MVA containing formulation is given in example 2. 20 1. Experimental settings: Vaccine preparation/Formulations To test the freeze-drying process according to the present invention several MVA preparations were used. For the freeze-drying experiments (rows GT1 25 4, 6-10 and 13-15 in table 6) modified vaccinia virus strain Ankara (MVA) was used. The virus was purified by 36%- and 40%-sucrose cushions centrifugation followed by resuspension in 1mM Tris-buffer at pH 9.
WO 03/053463 PCT/EP02/13434 28 In freeze dryings experiments GT1-4 (table 6) no additives were used. The used buffer system was 10mM Tris with 140mM NaCI at pH 7.4. For the freeze dryings starting with number GT6 (table 6) different additives were used without changing the buffer system. 5 Two different formulations with different additives were chosen. The additives were given to the virus containing solutions by adding a dilution buffer. The composition of the-dilution buffers used is shown in the following tables 3 and 4. The addition of dilution buffer 1 (DSG) results in an aqueous formulation according to the present invention. The use of dilution buffer 2 10 (DGG) results in a formulation used for comparative analysis. Table 3: Dilution buffer 1 (DSG) Concentration i n stock solution [g/l] Dextran (MW 36000 - 44000) 63 Sucrose 150 L-Glutamic acid Monopotassium 0,36 salt Monohydrate Table 4: Dilution buffer 2(DGG) Concentration in stock solution [g/l] Dextran (MW 36000 - 44000) 63 Glucose 150 L-Glutamic acid Monopotassium j0,36 salt Monohydrate 15 These dilution buffers were used at different concentrations in the final formulation. Dilution buffer 1 (DSG) was used at 16.7%, 23%, 30% and 40% WO 03/053463 PCT/EP02/13434 29 (v/v), dilution buffer 2 (DGG) at 20% (v/v). The TCID 50 /ml of the final formulation was adjusted to 5 x 108 TCID 50 /ml with a physiological Tris buffer (10mM Tris-buffer; 140mM NaCl; pH 7.4). 5 Sample freezing The samples were frozen inside the freeze-dryer (Christ freeze dryer, Type Alpha 2-4). For the formulation with sucrose (DSG) the comparison of different freezing temperatures (- 3 0 C to - 450 C) showed that the suspension has to be frozen to - 400 C, which is below the collapse 10 temperature of the formulation, to get a perfect cake structure. When frozen inside the freeze dryer, - 40 C were reached within about 3.5 to 4.5 hours (starting at about 200 C). Primary drying 15 For the formulation with sucrose (DSG) a collapse temperature of about - 30 to - 370 C was assumed on account of the collapse temperature of sucrose (- 31* C). Therefore, the product temperature was adjusted to values in the range of - 37 to - 41* C, to ensure a completely frozen matrix. Pressures of 0.04 and 0.12 mbar (- 50* C and - 40 C in the phase diagram of water) 20 were used. The driving force of sublimation during primary drying is the pressure difference between the product and the condenser of the freeze dryer created by their temperature differential. A law of nature is that as the 25 temperature of water is decreased the pressure over that water also decreases. A specific temperature of water is always associated with a specific pressure. The condenser was set to temperatures in the range of 830 C to - 89* C. The pressure in the chamber and the shelf temperature WO 03/053463 PCT/EP02/13434 30 regulates the product temperature. This indicates that the length of the primary drying cannot be shortened very easily, because the condenser temperature is fixed. For increasing the product temperature, Tc of the formulation is the limiting factor. 5 Secondary drying The temperatures for the secondary drying are determined by the stability of the product. Also the residual moisture content of the formulation depends on the requirements of the product. Some need higher, some lower moisture 1o content to achieve best product stability. The optimal residual moisture content as well as the time to reach this has to be determined empirically. Since secondary drying starts when the product reaches a temperature above 0* C, secondary drying was done in two steps. In the first step shelf temperature was regulated for some hours (in the range of 4 to 7 hours) in 15 that way that the product temperature was above 0* C (in the range of 4 to 60 C). In that way all possibly existing ice that remained after primary drying was melted. By using such mild conditions to start the secondary drying damages to product will be minimised. Afterwards, the second step was initiated by increasing the product temperature to values in the range of 18 20 to 210 C for 20 - 30 hours. The time for the second step is strongly dependent on the wanted residual moisture of the freeze-dried product. To obtain different residual moisture contents different times were used. As assay to measure the residual moisture content of the freeze-dried material the coulometric Karl-Fischer titration was (Jennings, T.A., 25 "Lyophilization, Introduction and Basic Principles", Interpharm Press, Denver, CO, US, 1999, ISBN 1-57491-081-7, pages 415-418).
WO 03/053463 PCT/EP02/13434 31 Product stoppering and removal All products made during the process development were sealed under very low pressure (0.04 - 2.56 mbar) directly in the freeze dryer. The vials were closed using butyl rubber stoppers. Once the product was stoppered the 5 system was returned to atmospheric pressure and the shelf was unloaded. Afterwards, the vials were sealed with aluminum caps for long-term storage. Vaccine storage An important aspect of the formulation exercise is to produce a vaccine that io is shelf-stable. Factors influencing stability include residual moisture content, sealing atmosphere composition, and storage conditions, including temperature, humidity, and light. The different batches produced during the process development were all stored at 40 C and at room temperature. Furthermore, a few batches were 15 also stored at 31 *C, 370 C and 45 *C. All samples were stored in the dark. Reconstitution The freeze-dried samples were reconstituted with autoclaved Milli-Q water. 20 More specifically the water (1.2 ml) was added to the sample using a syringe. The suspension was mixed by gentle shaking. The reconstitution takes only a few seconds. The virus titer of the reconstituted product was determined and compared to the virus titer before freeze-drying. 25 Accelerated stability test The stability of the formulation GT23 (see table 6) was assessed at 31 *C, 37 'C and 45 *C. The viral titer was monitored regularly. The results are shown in figures 1 to 3.
WO 03/053463 PCT/EP02/13434 32 2. Results and Conclusion: MVA was freeze-dried with and without using different additives. Formulations without additives were shown to be unstable (see table 6). In 5 this context samples were considered as stable when the titer did not drop more than 0.5 log. Thus, the term "stable at a certain temperature for a certain period of time" means that the loss of viral titer at this temperature is less than 0.5 logs during this time period. A formulation "fails" if the loss of virus titer during the indicated time period at the indicated temperature is 10 0.5 logs or more. Formulations comprising dextran and glucose showed a very low stability at room temperature. The formulations according to the present invention comprising different concentrations of sucrose and dextran proved to be stable. The stability of MVA in the formulations according to the present invention is at least 25 weeks at 4* C and room temperature. 15 Detailed information regarding individual experiments is given in table 6: In table 6 it is shown that the stability of the formulations without additives (table 6, GT1-4) was very poor. After only a few weeks they lost 0.5 logs of 20 their original starting titer, which is not acceptable. The formulation with 20% (v/v) DGG was not acceptable due to a collapse of the material during the freeze-drying process (data not shown). This collapse is explainable by the low Tc of glucose, which was not markedly increased by 25 the use of dextran, which has a high Tc (- 110 C). For primary drying the lowest possible temperature of the freeze-drying equipment (- 450 C) was used. Therefore, it was not possible to decrease temperatures below the Tc of glucose. The formulations with 30% (v/v) DGG did not collapse. This phenomenon is probably due to the higher overall amount of dextran, which 30 increases.-Tc to a value higher than the temperature used for primary drying.
WO 03/053463 PCT/EP02/13434 33 Although the material did not collapse the stability, especially at room temperature, was not satisfying, which might be due to the low solid state Tc of glucose (table 6, GT 10). 5 Dilution buffer 1 (DSG) was used in most of the experiments. The stabilization with this additive is very good. Due to the high Tc (- 310 C) of sucrose collapse was not a problem with this formulation. The stability of the freeze-dried material was always good (table 6). There were no big differences between the use of 16.7%, 20%, 23%, 28.6%, 30% and 40% 10 (v/v) DSG in the formulation. Stability at 4* C and room temperature is proven for all 6 formulations. The freeze-dried products with 30% and 40% DSG had a slightly better stability. One of the formulations (process GT 23, see table 6) was analyzed in detail 15 in an accelerated stability test. The results are shown in figures 1 to 3 and summarized in the following table 5. Table 5: Temperature [0 Loss of titer Loss of 0.5 logs after C] (experimental data) [days] (calculated) 31 0.245 logs in 29 59 days 37 0.321 logs in 35 54 days 45 0.332 logs in 29 44 days 20 At 310 C the vaccine has been stored for about 1 month and still met specifications (loss in virus titer is less than half a log). But even at higher WO 03/053463 PCT/EP02/13434 34 temperatures it would be possible to store the vaccine for more than a month, which might be interesting especially for tropical regions. For the old smallpox vaccines the WHO recommended a method for 5 estimation of stability. If the vaccine lost less than 1 log within 4 weeks at 370 C, it was assumed to be stable for at least one year when stored at 4* C (acceptance criterion for use of the old vaccine was loss of less than 1 log). As shown the formulation GT23 according to the present invention fulfills this criterion. 10 Example 2: Titration of Modified Vaccinia Virus Ankara (MVA) The titration of Modified Vaccinia virus Ankara (MVA) is performed in a
TCID
50 -based assay using 10-fold dilutions in a 96-well format. 15 At the endpoint of the assay, infected cells are visualised using an anti vaccinia virus antibody and an appropriate staining solution. 2-3 day old primary CEF (chicken embryo fibroblasts) cells are diluted to 1 x 105 cells/ml in 7% RPMI. 10 fold dilutions are done with 8 replicates per 20 dilution. Following dilution, 100 pl are seeded per well of 96-well plates. Cells are then incubated over night at 37'C and 5% C02. Dilutions of the virus containing solutions are made in 10-fold steps (10- to 10-12 as appropriate) using RPMI without foetal calf serum. Then, 100 RI of 25 every virus sample is added to the cell containing wells. The 96-well-plates are incubated at 370C with 5% C02 for 5 days to allow infection and viral replication. Cells are stained 5 days after infection with a vaccinia virus specific 30 antibody. For the detection of the specific antibody, a horseradish WO 03/053463 PCT/EP02/13434 35 peroxidase (HRP) coupled secondary antibody is used. The MVA specific antibody is an anti-vaccinia virus antibody, rabbit polyclonal, IgG fraction (Quartett, Berlin, Germany #9503-2057). The secondary antibody is anti rabbit IgG antibody, HRP coupled goat polyclonal (Promega, Mannheim, 5 Germany, # W401 1). The colour reaction.is carried out according to known techniques. Every well with cells that are positive in the colour reaction is marked as positive for the calculation of the TCID 50 . 10 The titre is calculated by using the formula of Spearman [1] and Kaerber [2]. Because all assay parameters are kept constant, the following simplified formula is used: a+1,5+x +x +x Virus titre [TCID 5 0 /mI] = 101"888 a = dilution factor of last column, in which all eight wells are positive 15 xa= number of positive wells in column a+1 Xb= number of positive wells in column a+2 xc= number of positive wells in column a+3 20 WO 03/053463 PCT/EP02/13434 36 -c U) E 0 o C 5-0 0 0 .- 0 5 0 4- (1) 4 ci) ?) e C?)en U CI (1) (y )Cci '-V) 4? 5 o -. 4N N c) ,V -~~~~ 0n~ nO nE ) 0i 0 41 41 L.. s- ) o -> W3 .: 23% 0 23M0 2 - 5o 5r- 5-Q E~~ E~ C?? E2~2 ? u a-o 0 co (D o i 4 - - 55 IN C? 0l (1)3 4- 4- *I3 0'- 230 2 '-2 en -'-- ~ (n 235 en('' n Z3 '- n 2 m C ) 0 0 Qi) 00 PI 0 0 0 0 C- L- 0 (1 ~ c) 0 5- 5- C? -5- 5 CO ) O 00 0- o - n4 o L a, NY) ~ N -0 Z3 -(i -Ci 5-(i c) 4. 3.a) L6a a)cci C5 E = CL 6I E~ N 0l E~~-0 ~ 0) E 4- 0.4-' ~ 5- ) 0 5- 4. 4 - .. ' ''5 "5 4 ) ..- 4- 230 111 23a;3 4 2 en ~en o 0en J 0U) :3 ~ 0:(/ V) fi) ci) ) oci 0 0 in) 0 ( O) CN CL 0- 5 - - 5- 5) Q >~ C. CON C)a 0.a ~ a ~ a 0 0 000 X 0 0 0 0 0 LO '4- ? o 0 0 0 0 0 0 4- 4-C/ 0 00 0.
WO 03/053463 PCT/EP02/13434 37 U) o~3 ou -Cc - ) I- a) /) '4- / '-0 (D Q)LC (D 0t 0m a) 4-) 4 0a ini E ( a cE ci) 4-1 '44 414 4))a w 0 cQ) a-H. a) r E~ L E .2 C)E.0' o 1 C U) 0- cc LL- m 40Cl - -U) ( n z n n El N L.J El 00 N.c) 1 QO 0 i) Q.. 0 c ) 0 0 ) _ j L n~4 S- 0 4~ 0 ) (n '-C U ) Z5 ' C) Ln Z3 C Ln 0 () 0 U) - 0 (n Cl 0 0 0- () 0 0 -) 0 0 CV) r- N . -. . LC) C)- O ~ 0 a t 0- 0~ c a cu C E E a) ) - i 0 - ac' 0 4 i 0 0~f O 0 ~4-~O Un -a ) -C3 0 U) -0 0 (1 c) o N ci() 000 ON 0 [ C) C0 C) 0 0~ 0 0 (Y) t.0 () 0 0 N~ ("(y) N K Ica WO 03/053463 PCT/EP02/13434 38 a) V oD C D 4'-I 0 0n
U))
2r qt 0 (D 0 0 C A- - 0) - C0 ) a) M- a -) 4- IZ m - 0 m -i-' -1- 0 _1. 4) CD 4- m 4D CO in C!a Cn V-U C ) in C 4-) (n U) V - r- E C DC 0 0 CD 0 0 a) 0 a) CD U) - .2 - p CP 0 01- 4- ,D CO :3 a) = 0 = CD 5 LO) 0 n. 75 :3 LO o o N" 0 o - 0 0 ±. D 0 0~ 4-1 LL'tU. CU LO L < I.L LL < -It a)- CO L O L0 -C LO .0 0 - L6 .0 fl 0 - O 0 0- L E4 LO e-, lt DL ~J C ) - I) ~ D E . cq E -,CN c E 2 N6 E Lo N 6 o a) 0D a ) 0 0 ) -1Q 0 U) . " 0 00 CD &- 0D 0C o 41O oI Q L ) . 4 - ~ H Q Cn -0 (0 o-C .CO~ O~ 0 o )0 o .)0 o ()0 o .0 L- a - - L- S. "N IO 00 0J- GC- -- 0- 0- LO C~ nt o 4C0 -0 a3 _0 0 = 0D Z3) 0 =-i 0- - 00 0 -r- 0 ED CD E- CDJ E- mD . E- N a ) a) a) " a) . 0 " U) 0 4- 0 4- . 0 U). 0 0 U) . 0 0 C) :L3 C) w 3 C) C- :3 C)C 0) 0) 00 0f 00oi o 0 o V 0 () 0() a 0 00 a 0 0 0 0- I- a C)- o? C-- ") 0C0 C) C) 0 0 0 0 0 0 0 000 03 MN 03 00 el .9 CD9 0. . KY N KY K K) WO 03/053463 PCT/EP02/13434 39 00 4- ~ -I-' U U_ '4- U) 410 0 CU c 4-, 4 l) D C-l _ 00 C-) + 0. ) ~U ~0 n3 L) v) :3 0) 0.0 U '' i 0 L n Cl) C L) Q 0 U) 0 ) 0 0. 1 . 0 N Cl ) U) (Y') U 0 : f EDITORIAL CASE NOTE: "2008201215" This specification does not contains page numbered 40-42.
Claims (25)
1. A formulation comprising (i) a purified or partially purified poxvirus selected from the group consisting of Orthopoxviruses, Parapoxviruses, Avipoxviruses, Capripoxviruses and Suipoxviruses, (ii) a disaccharide, (iii) a pharmaceutically acceptable polymer and (iv) a buffer, wherein phosphate buffer is excluded.
2. Formulation according to claim 1, wherein the buffer is selected form the group consisting of TRIS, TBS, MOPS, HEPES, and bicarbonate buffers.
3. Formulation according to any one of claims 1 to 2, characterized in that the poxvirus is a vaccinia virus.
4. Formulation according to claim 3, wherein the vaccinia virus is selected from strain Elstree and modified vaccinia virus strain Ankara (MVA).
5. Formulation according to any one of claims 1 to 4, characterized in that the poxvirus is a recombinant poxvirus.
6. Formulation according to any one of claims 1 to 5, characterized in that the disaccharide is selected from the group consisting of sucrose, lactose and trehalose.
7. Formulation according to any one of claims 1 to 6, characterized in that the concentration of the disaccharide is in a range of 10 to 100 g/l. 44
8. Formulation according to any one of claims 1 to 7, characterized in that the pharmaceutically acceptable polymer is selected from dextran and polyvinylpyrrolidone (PVP).
9. Formulation according to claim 8, characterized in that the dextran has a molecular weight in the range of 30,000 to 70,000 and has a concentration of 1 to 50 g1l.
10. Formulation according to any one of claims 1 to 9, characterized in that the formulation further comprises glutamic acid.
11. Formulation according to any one of claims 1 to 10, characterized in that the collapse temperature of the formulation is in the range of -37 *C to -30 "C.
12. Formulation according to any one of claims 1 to 11, characterized in that the poxvirus is an MVA strain or strain Elstree and the dissaccharide is sucrose.
13. Formulation according to any one of claims 1 to 12, wherein the poxvirus is a virus having a titer of at least 106 TCID 5 o per mg total protein.
14. Formulation according to any one of claims 1 to 13 for use as vaccine. 45
15.Use of the formulation according to any one of claims 1 to 13 for the preparation of a vaccine.
16. Method of preparing a stable, poxvirus containing composition comprising the step of freeze-drying the formulation of any one of claims 1-13.
17. Method of claim 16 comprising the following steps: (i) freezing the formulation as defined in any one of claims 1-13 to a temperature lower than the collapse temperature of the formulation to obtain a frozen product matrix; (ii) primarily drying the frozen formulation under low pressure and at a product temperature allowing sublimation of the ice in the product matrix, wherein the product temperature is lower than the collapse temperature of the formulation; and (iii) secondarily drying at low pressure and at a product temperature in the range of 0 0C to 30 *C until the residual moisture of the product is lower than 5%.
18. Freeze-dried product obtainable by the method of any one of claims 16 to 17.
19.Freeze-dried product comprising the formulation according to any one of claims I to 14.
20. Freeze-dried product according to any one of claims 18 to 19, characterized in that the residual moisture content is in a range of 1 to 3 %. 46
21. Use of the freeze-dried product according to any one of claims 18 to 20 for the preparation of a vaccine.
22. Method for the reconstitution of the freeze-dried product according to any one of claims 18 to 20, characterized in that the product is dissolved in an appropriate amount of a pharmaceutically acceptable solvent.
23.A poxvirus containing vaccine comprising the formulation according to any one of claims 1 to 13.
24, The vaccine according to claim 23 in freeze-dried form.
25. Method for the vaccination of an animal or a human being in need thereof with the formulation according to any one of claims 1 to 13, the vaccine according to any one of claims 23 to 24 or the reconstituted product obtained by the method according to claim 22.
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AU2008201215A AU2008201215B2 (en) | 2001-12-10 | 2008-03-14 | Poxvirus containing formulations and process for preparing stable, poxvirus containing compositions |
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DKPA200101831 | 2001-12-10 | ||
AU2002361962A AU2002361962A1 (en) | 2001-12-10 | 2002-11-28 | Poxvirus-containing compositions and process for their preparation |
AU2008201215A AU2008201215B2 (en) | 2001-12-10 | 2008-03-14 | Poxvirus containing formulations and process for preparing stable, poxvirus containing compositions |
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AU2002361962A Division AU2002361962A1 (en) | 2001-12-10 | 2002-11-28 | Poxvirus-containing compositions and process for their preparation |
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AU2008201215B2 true AU2008201215B2 (en) | 2010-11-18 |
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Citations (3)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
FR7773M (en) * | 1968-06-14 | 1970-03-23 | ||
US3577526A (en) * | 1969-06-13 | 1971-05-04 | Merieux Inst | Stabilized smallpox vaccine |
US6258362B1 (en) * | 1998-04-24 | 2001-07-10 | Cantab Pharmaceuticals Research Ltd | Stabilization of herpes virus preparations |
-
2008
- 2008-03-14 AU AU2008201215A patent/AU2008201215B2/en not_active Ceased
Patent Citations (3)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
FR7773M (en) * | 1968-06-14 | 1970-03-23 | ||
US3577526A (en) * | 1969-06-13 | 1971-05-04 | Merieux Inst | Stabilized smallpox vaccine |
US6258362B1 (en) * | 1998-04-24 | 2001-07-10 | Cantab Pharmaceuticals Research Ltd | Stabilization of herpes virus preparations |
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AU2008201215A1 (en) | 2008-04-10 |
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