ULTRAFILTRATION FOR PREPARING OUTER MEMBRANE VESICLES
All documents cited herein are incorporated by reference in their entirety.
TECHNICAL FIELD
This invention is in the field of vesicle preparation for immunisation purposes. BACKGROUND ART
One of the various approaches to immunising against N.meningitidis infection is to use outer membrane vesicles (OMVs). An efficacious OMV vaccine against serogroup B has been produced by the Norwegian National Institute of Public Health [e.g. ref. 1] but, although this vaccine is safe and prevents NmB disease, its efficacy is limited to the strain used to make the vaccine. The 'RINM' vaccine is based on vesicles containing six different PorA subtypes and has been shown to be immunogenic in children in phase II clinical trials [2].
References 3 & 4 disclose a vaccine against different pathogenic serotypes of serogroup meningococcus based on OMNs which retain a protein complex of 65-kDa. Reference 5 discloses a vaccine comprising OMNs from genetically-engineered meningococcal strains, with the OMNs comprising: at least one Class 1 outer-membrane protein (OMP) but not comprising a Class 2/3 OMP. Reference 6 discloses OMNs comprising OMPs which have mutations in their surface loops. Reference 7 discloses compositions comprising OMNs supplemented with transferrin binding proteins (e.g. TbpA and TbpB) and/or Cu,Zn-superoxide dismutase. Reference 8 discloses compositions comprising OMNs supplemented by various proteins. References 9 & 10 also describe OMN preparations from meningococcus.
Reference 11 discloses a process for preparing OMN-based vaccines, particularly for serogroup A meningococcus, comprising the following 10 steps: (a) cultivating bacterial cells; (b) concentrating the cultivated cells from step (a); (c) treating the cells with a bile acid salt detergent at a pH sufficiently high not to precipitate the detergent, for inactivating the bacteria, disrupting the outer membrane of the bacteria and forming vesicles of the outer membrane of the bacteria, said vesicles comprising outer membrane components mainly presented in their native form; (d) centrifuging the composition from step (c) at 10,000-20,000 x g for about 1 to 2 hours to separate the outer membrane vesicles from the treated cells and cell debris, and collecting the supernatant; (e) performing a high speed centrifugation of the supernatant from step (d) and collecting the outer membrane vesicles in a pellet; (f) re-dispersing the pellet from step (e) in a buffer by stirring at ambient temperature; (g) performing a second high speed centrifugation in accordance with step (e), collecting the outer membrane vesicles in a pellet; (h) re-dispersing the pellet from step (g) in an aqueous medium containing a stabilising agent by stirring at ambient temperature; (i) performing a step-wise sterile filtration through at least two filters of decreasing pore size of the re-dispersed composition from step (h), ending with a filter of pore-size of about OJμm; and (j) optionally including the composition from step (i) in a pharmaceutically acceptable carrier and/or adjuvant composition.
It is an object of the present invention to provide an improved process for preparing OMNs for use in vaccines, in particular a process which can prepare a greater quantity of OMNs in a shorter time, and particularly a process suitable for industrial-scale use.
DISCLOSURE OF THE INVENTION The invention is based on the finding that, compared to the centrifugation used in step (e) of the process of reference 11, ultrafiltration allows much larger amounts of OMV-containing supernatant to be processed in a much shorter time (typically >15 litres in 4 hours, compared to <1.5 litres in 10 hours). As well allowing step (e) to be performed more quickly, the use of ultrafiltration allows step (f) to be avoided because the OMVs remains in suspension. Thus the invention provides a process for preparing bacterial OMVs, comprising a step of ultrafiltration. The ultrafiltration step is performed on an aqueous suspension of OMVs after they have been prepared from bacteria and the OMVs remain in suspension after the ultrafiltration step.
The invention also provides, in a process for preparing OMVs from a bacterium, the improvement consisting of the use of ultrafiltration of an OMV suspension in place of a step of centrifugation. The invention also provides a process for purifying bacterial OMVs, wherein the process does not include a centrifugation step in which the OMNs are pelleted, particularly a centrifugation step performed on crude OMNs.
The ultrafiltration step
Ultrafiltration is a separation process whereby solvent is removed from a solution (including a colloidal solution) or a suspension by forcing it to flow through a membrane by the application of a hydraulic pressure. Components in the solution which are significantly larger than the solvent cannot pass through the membrane. Ultrafiltration therefore separates components based on size.
The ultrafiltration step preferably results in diafiltration of the solution. In diafiltration, solvent and/or microsolutes (e.g. salts) which are removed during ultrafiltration are replaced by new solvent and microsolutes. In general, removal and replacement occur at the same rate and the volume of the solution is thus kept constant. The overall effect of the process is therefore the replacement of original solvent/microsolutes with new solvent/microsolutes. The process of the invention may thus include a step of diafiltration.
The ultrafiltration is preferably cross-flow or tangential flow ultrafiltration, in which the solution flows substantially parallel to the membrane surface, rather than flowing perpendicular to the surface as in ordinary filtration.
Preferred membranes for use in the ultrafiltration step have a cut-off of about 300kDa.
The ultrafiltration step preferably last less than 10 hours e.g. between 2 and 6 hours, preferably between 3 and 5 hours e.g. between 3.5 and 4.5 hours. Membranes may be made from any suitable material e.g. polyethersulphone.
Pre-ultrafiltration steps
Prior to the ultrafiltration step, the process of the invention will typically comprise an initial step of cultivating bacterial cells (e.g. in broth or in solid medium culture), optionally followed by a step of collecting and/or concentrating the cultivated cells (e.g. by filtration or by a low-speed centrifugation to pellet the cells). However, the invention may be performed on bacteria which have already been cultured and/or harvested separately. The bacterial culture preferably involves the use of neither blood products nor material contaminated with a transmissible spongiform encephalopathy agent.
The ultrafiltration step is performed on an aqueous suspension of OMNs after they have been prepared from bacteria. Prior to ultrafiltration, the process may therefore comprise a step of OMN preparation in which cells are treated to disrupt their outer membranes. The preparation of OMNs from meningococcus is well-known in the art. Methods for obtaining suitable preparations are disclosed in, for instance, references 1 to 25. Techniques for forming OMNs include treating bacteria with a bile acid salt detergent (e.g. salts of lithocholic acid, chenodeoxycholic acid, ursodeoxycholic acid, deoxycholic acid, cholic acid, ursocholic acid, etc., with sodium deoxycholate [26 & 27] being preferred for treating Neisseria) at a pH sufficiently high not to precipitate the detergent [11]. Other techniques may be performed substantially in the absence of detergent [28] using techniques such as sonication, homogenisation, microfluidisation, cavitation, osmotic shock, grinding, French press, blending, etc.
After OMN formation and prior to ultrafiltration, the OMNs are preferably separated from bacterial cells and cell debris. Separation can conveniently be achieved by centrifugation (e.g. at 10,000- 20,000 x g for about 1 to 2 hours). OMNs remain in the supernatant and can then be subjected to ultrafiltration according to the invention, rather than to ultracentrifugation as in the prior art. Other methods for separating outer membrane fractions from cytoplasmic molecules may involve filtration (e.g. cross flow filtration), differential precipitation or aggregation of outer membranes and/or OMVs, affinity separation methods using ligands that specifically recognize outer membrane molecules, etc. Use of a closed filtration system may be preferred to avoid open handling of infectious bacteria.
In order to preserve the native conformation of proteins and other labile outer membrane antigens, mild conditions will generally be selected for preparation of OMVs. Heat inactivation of bacteria (e.g. at 56°C or higher) is thus preferentially avoided, as is solvent denaturation.
Post-ultrafiltration steps
After the ultrafiltration step, the OMVs may be further treated.
For example, the OMVs may be sterilised. Sterilisation is preferably a final step before packaging as a pharmaceutical, and can conveniently be achieved by filter sterilisation. Although OMVs will pass through a standard 0J2μm filters, these can rapidly become clogged by other material, and so it is preferred to perform sequential steps of filter sterilisation through a series of filters of decreasing
pore size, finishing with a standard sterilisation filter (e.g. a 0J2μm filter). Examples of preceding filters would be those with pore size of 0.8μm, 0.45 μm, etc. Filter sterilisation advantageously occurs at ambient temperature or above, rather than at refrigeration temperatures. Vesicle flexibility is higher at ambient temperature and larger vesicles (~0Jμm) can thus pass through a 0J2μm filter more easily, giving less clogging of filters.
The OMVs may also be centrifuged (e.g. ultracentrifuged) after ultrafiltration takes place. Thus, in some embodiments, the invention does not completely replace the use of ultracentrifugation during OMV preparation, but removes at least one step of ultracentrifugation relative to ref. 11. A normal ultracentrifugation step requires about 13 hours for 1J litres of OMV suspension, and so a large volume of OMVs requires a large ultracentrifugation resource. Ultrafiltration according to the invention can be used to reduce the volume which has to be ultracentrifuged (by around 3-fold) and so can improve throughput even though ultracentrifugation is not wholly avoided.
The OMVs may be combined with pharmaceutical carriers and/or adjuvants and/or stabilisers. For example, pellet(s) from ultracentrifugation can be re-suspended (e.g. in a sucrose solution, preferably about 3% sucrose) and then subjected to filter sterilisation as described above.
OMVs may be sonicated. Sonication is particularly useful between re-suspension of centrifugation pellets and sterilisation.
After re-suspension, OMV preparations preferably contain between 500 and 2000 mg of protein per millilitre e.g. between 900 and 1800 mg/ml, or 1000+100 mg/ml. Overall process for preparing sterile OMVs
In general, therefore, the process of the invention will include the following steps: (1) cultivating bacterial cells; (2) collecting the cultivated cells; (3) OMV formation; (4) separation of OMV from cell debris, to give an aqueous suspension of OMV; (5) ultrafiltration; (6) centrifugation and re-suspension to collect purified OMV; and (7) sterilisation. pH may be adjusted at any stage as required. Similarly, dilution as appropriate can be used.
Step (5) in this process replaces steps (e) and (f) from reference 11.
The bacterium
The bacterium from which OMVs are prepared may be Gram-positive, but it is preferably Gram- negative. The bacterium may be from any suitable genus, including Moraxella (e.g. M.catarrhalis [29,30]), Shigella (e.g. S.flexneri [31,32]), Pseudomonas (e.g. P.aeruginosa [31,32]), Treponema (e.g. T.pallidum [33]), Haemophilus (e.g. H.influenzae [9 & 10]), Porphyromonas (e.g. P.gingivalis [34]) or Helicobacter (e.g. H.pytori [35]), but it is preferably from the Neisseria genus. Preferred Neisseria species are N.meningitidis, N.lactamica [36] and N.gonorrhoeae [37 & 38]. Within N.meningitidis, any of serogroups A, C, W135 and Y may be used, but it is preferred to prepare vesicles from serogroup B.
Preferred strains within serogroup B are MC58, 2996, H4476, 394/98 and New Zealand strain 98/254. The best serotypes and strains to use, however, will depend on the strains prevalent in a particular geographical location. For example, the meningococcus can be of any serotype (e.g. X, 2a, 2b, 4, 14, 15, 16, etc.), of any serosubtype (P1J; P1.4; P1.5; Pl.5,2; Pl.7,16; P1.7,16b; P1.9; Pl.9,15; Pl.12,13; P1.13; P1.14; P1J5; Pl.21,16; Pl.22,14; etc.) and of any immunotype (e.g. LI; L3-3-7; L10; etc.), and preferred strains include: (a) B:4:P1.4; (b) B:4:P1J5; (c) B:15:P1.7,16; and (d) B:4:P1.7b,4. The meningococcus may be from any suitable lineage, including hyperinvasive and hypervirulent lineages e.g. any of the following seven hypervirulent lineages: subgroup I; subgroup III; subgroup IV- 1; ET-5 complex; ET-37 complex; A4 cluster; lineage 3. These lineages have been defined by multilocus enzyme electrophoresis (MLEE), but multilocus sequence typing (MLST) has also been used to classify meningococci [ref. 39] e.g. the ET-37 complex is the ST-11 complex by MLST, the ET-5 complex is ST-32 (ET-5), lineage 3 is ST-41/44, etc.
To reduce pyrogenic activity, it is preferred that the bacterium should have low endotoxin (LPS) levels. Suitable mutant bacteria are known e.g. mutant Neisseria [40] and mutant Helicobacter [41]. Processes for preparing LPS-depleted outer membranes from Gram-negative bacteria are disclosed in reference 42.
The bacterium may be a wild-type bacterium, or it may be a recombinant bacterium. Preferred recombinant bacteria over-express (relative to the corresponding wild-type strain) immunogens such as NspA, protein 287 [8], protein 741 [8], TbpA, TbpB, superoxide dismutase [7], etc. The bacterium may express more than one PorA class I outer membrane protein e.g. 2, 3, 4, 5 or 6 of PorA subtypes: Pl.7,16; Pl .5,2; Pl.19,15; PI.5c, 10; Pl.12,13; and P1.7h,4 [e.g. refs. 12 & 14].
Other recombinant bacteria that can be used with the invention have one or more mutations to decrease (or, preferably, to knockout) expression of particular gene products. Preferred genes for down-regulation and/or knockout include: (a) Cps, CtrA, CtrB, CtrC, CtrD, FrpB, GalE, HtrB/MsbB, LbpA, LbpB, LpxK, Opa, Ope, PilC, PorA, PorB, SiaA, SiaB, SiaC, SiaD, TbpA, and/or TbpB [9]; (b) CtrA, CtrB, CtrC, CtrD, FrpB, GalE, HtrB/MsbB, LbpA, LbpB, LpxK, Opa, Ope, PhoP, PilC, PmrE, PmrF, PorA, SiaA, SiaB, SiaC, SiaD, TbpA, and/or TbpB [10]; (c) lytic transglycosylase NMB0033 [43]; (d) ExbB, ExbD, rmpM, CtrA, CtrB, CtrD, GalE, LbpA, LpbB, Opa, Ope, PilC, PorA, PorB, SiaA, SiaB, SiaC, SiaD, TbpA, and/or TbpB [44]; and (e) CtrA, CtrB, CtrD, FrpB, OpA, OpC, PilC, PorA, PorB, SiaD, SynA, SynB, and/or SynC [45].
Pharmaceutical compositions
For human use, OMVs will generally be combined with a pharmaceutically acceptable carrier.
The term "pharmaceutically acceptable carrier" refers to a carrier for administration of a therapeutic agent, such as antibodies or a polypeptide, genes, and other therapeutic agents. The term refers to any pharmaceutical carrier that does not itself induce the production of antibodies harmful to the individual receiving the composition, and which can be administered without undue toxicity. Suitable
carriers can be large, slowly metabolized macromolecules such as proteins, polysaccharides, polylactic acids, polyglycolic acids, polymeric amino acids, amino acid copolymers, and inactive virus particles. Such carriers are well known to those of ordinary skill in the art. Pharmaceutically acceptable carriers in therapeutic compositions can include liquids such as water, saline, glycerol and ethanol. Auxiliary substances, such as wetting or emulsifying agents, pH buffering substances, and the like, can also be present in such vehicles. Typically, the therapeutic compositions are prepared as injectables, either as liquid solutions or suspensions; solid forms suitable for solution in, or suspension in, liquid vehicles prior to injection can also be prepared. Liposomes are included within the definition of a pharmaceutically acceptable earner. Pharmaceutically acceptable salts can also be present in the pharmaceutical composition, e.g. mineral acid salts such as hydrochlorides, hydrobromides, phosphates, sulfates, and the like; and the salts of organic acids such as acetates, propionates, malonates, benzoates, and the like. A thorough discussion of pharmaceutically acceptable excipients is available in reference 46. The composition will typically include saline.
Once formulated, compositions can be administered directly to a subject. Delivery will generally be accomplished by parenteral injection (e.g. subcutaneously, intraperitoneally, intravenously or intramuscularly, or to the interstitial space of a tissue) or by mucosal administration (e.g. oral, pulmonary, rectal, vaginal, intranasal [47,48]), etc.). Transdermal applications, needles, and gene guns or hyposprays may also be used. Intramuscular injection is the preferred manner of delivery.
The dose and the means of administration of the inventive pharmaceutical compositions are determined based on the specific qualities of the therapeutic composition, the condition, age, and weight of the patient, the progression of the disease, and other relevant factors.
Neisserial infections affect various areas of the body and so the compositions of the invention may be prepared in various forms. For example, the compositions may be prepared as injectables, either as liquid solutions or suspensions. Solid forms suitable for solution in, or suspension in, liquid vehicles prior to injection can also be prepared (e.g. a lyophilised composition). The composition may be prepared for topical administration e.g. as an ointment, cream or powder. The composition be prepared for oral administration e.g. as a tablet or capsule, or as a syrup (optionally flavoured). The composition may be prepared for pulmonary administration e.g. as an inhaler, using a fine powder or a spray. The composition may be prepared as a suppository or pessary. The composition may be prepared for nasal, aural or ocular administration e.g. as drops.
The OMVs of the invention may be combined with an adjuvant. Preferred adjuvants to enhance effectiveness of the composition include, but are not limited to: (A) MF59 (5% Squalene, 0.5% Tween 80, and 0.5% Span 85, formulated into submicron particles using a microfluidizer) [see Chapter 10 of ref. 49; see also ref. 50]; (B) microparticles (i.e. a particle of ~100nm to ~150μm in diameter, more preferably ~200nm to ~30μm in diameter, and most preferably ~500nm to ~10μm in diameter) formed from materials that are biodegradable and non-toxic (e.g. a poly(α-hydroxy acid), a polyhydroxybutyric acid, a polyorthoester, a polyanhydride, a polycaprolactone, etc.), with
poly(lactide-co-glycolide) being preferred, optionally treated to have a negatively-charged surface (e.g. with SDS) or a positively-charged surface (e.g. with a cationic detergent, such as CTAB) [51 & 52]); (C) liposomes [see Chapters 13 and 14 of ref. 49]; (D) ISCOMs [see Chapter 23 of ref. 49] , which may be devoid of additional detergent [53]; (E) SAF, containing 10% Squalane, 0.4% Tween 80, 5% pluronic-block polymer L121, and thr-MDP, either microfluidized into a submicron emulsion or vortexed to generate a larger particle size emulsion [see Chapter 12 of ref. 49]; (F) Ribi™ adjuvant system (RAS), (Ribi Immunochem) containing 2% Squalene, 0.2% Tween 80, and one or more bacterial cell wall components from the group consisting of monophosphorylipid A (MPL), trehalose dimycolate (TDM), and cell wall skeleton (CWS), preferably MPL + CWS (Detox™); (G) saponin adjuvants, such as QuilA or QS21 [see Chapter 22 of ref. 49], also known as Stimulon™; (H) chitosan [e.g. 54]; (I) complete Freund's adjuvant (CFA) and incomplete Freund's adjuvant (IF A); (J) cytokines, such as interleukins (e.g. IL-1, IL-2, IL-4, IL-5, IL-6, IL-7, IL-12, etc.), interferons (e.g. interferon-γ), macrophage colony stimulating factor, tumor necrosis factor, etc. [see Chapters 27 & 28 of ref. 49]; (K) a saponin (e.g. QS21) + 3dMPL + IL-12 (optionally + a sterol) [55]; (L) monophosphoryl lipid A (MPL) or 3-O-deacylated MPL (3dMPL) [e.g. chapter 21 of ref. 49]; (M) combinations of 3dMPL with, for example, QS21 and/or oil-in-water emulsions [56]; (N) oligonucleotides comprising CpG motifs [57] i.e. containing at least one CG dinucleotide; (O) a polyoxyethylene ether or a polyoxyethylene ester [58]; (P) a polyoxyethylene sorbitan ester surfactant in combination with an octoxynol [59] or a polyoxyethylene alkyl ether or ester surfactant in combination with at least one additional non-ionic surfactant such as an octoxynol [60]; (Q) an immunostimulatory oligonucleotide (e.g. a CpG oligonucleotide) and a saponin [61]; (R) an immunostimulant and a particle of metal salt [62]; (S) a saponin and an oil-in-water emulsion [63]; (T) E.coii heat-labile enterotoxin ("LT"), or detoxified mutants thereof, such as the K63 or R72 mutants [e.g. Chapter 5 of ref. 64]; (U) cholera toxin ("CT"), or detoxified mutants thereof [e.g. Chapter 5 of ref. 64]; (V) double-stranded RNA; (W) aluminium salts, such as aluminium hydroxides (including oxyhydroxides), aluminium phosphates (including hydroxyphosphates), aluminium sulfate, etc [Chapters 8 & 9 in ref.49]; (X) monophosphoryl lipid A mimics, such as aminoalkyl glucosaminide phosphate derivatives e.g. RC-529 [65]; (y) polyphosphazene (PCPP); (Z) a bioadhesive [66] such as esterified hyaluronic acid microspheres [67] or a mucoadhesive selected from the group consisting of cross-linked derivatives of poly(acrylic acid), polyvinyl alcohol, polyvinyl pyrollidone, polysaccharides and carboxymethylcellulose. Other substances that act as immunostimulating agents may also be used [e.g. see Chapter 7 of ref. 49].
Aluminium salts are preferred adjuvants for parenteral immunisation. Mutant toxins are preferred mucosal adjuvants. The use of an aluminium hydroxide adjuvant is most preferred, particularly for intramuscular injection, and this adjuvant is preferably used with a histidine buffer [68].
The invention provides a process for preparing a pharmaceutical composition, comprising the steps of: (i) preparing OMVs according to the invention; and (ii) formulating the OMVs as a
pharmaceutical. Step (ii) may involve activities such as filtration, addition of adjuvants, addition of buffer, etc.
OMVs and OMV-based compositions
The invention provides OMNs obtained by a process of the invention. The invention also provides OMNs obtainable by a process of the invention, which generally comprise outer membrane components in essentially their native form.
The invention also provides a composition comprising such OMNs and a pharmaceutically acceptable carrier. The composition may also comprise an adjuvant.
Compositions of the invention are preferably immunogenic compositions, and are more preferably vaccine compositions. Such compositions can be used to raise immune responses (e.g. antibody responses) in a mammal (e.g. in a human, such as a child).
The pH of the composition is preferably between 6 and 8, preferably about 7. The pH may be maintained by the use of a buffer. The composition may be sterile and/or pyrogen-free. The composition may be isotonic with respect to humans. The composition may or may not include a preservative (e.g. thiomersal, 2-phenoxyethanol, etc.). Mercury-free compositions are preferred.
The composition is preferably free from blood-derived components. The composition is preferably free from transmissible spongiform encephalopathy agents (e.g. prions). The composition is preferably substantially free from whole bacteria, and in particular from living bacteria.
The composition may include residual material from vesicle preparation (e.g. detergent, preferably <0.4μg detergent per μg OMN protein). The composition may include soluble sugars e.g. disaccharides such as sucrose and/ trehalose. LPS content is preferably <0Jμg per μg OMN protein.
Compositions of the invention may be distributed in various containers e.g. vials or pre-filled syringes. The use of glass vials is preferred. These containers will generally be sterile and hermetically-sealed. Each container preferably includes a single dose e.g. 0.5ml of liquid. Containers may be packaged singly or in multiples e.g. a box of 10 vials. Once packaged, compositions of the invention are preferably stored at between 2°C and 8°C, but should not be frozen.
Vaccines of the invention may be prophylactic (i.e. to prevent disease) or therapeutic (i.e. to reduce or eliminate the symptoms of a disease).
Compositions for administration to patients will comprise an immunologically effective amount of the OMNs. An "immunologically effective amount" is an amount sufficient to effect an immune response in a patient, and more preferably a protective immune response in a patient. The precise amount for a patient will depend upon their size and health, the nature and extent of their condition, and the therapeutics or combination of therapeutics selected for administration. The effective amount for a given situation is determined by routine experimentation and is within the judgment of a physician. For purposes of the present invention, an immunologically effective amount will generally
be administered at a dosage of from about O.Olmg/kg to about 5 mg/kg, or about 0.01 mg/ kg to about 50 mg/kg or about 0.05 mg/kg to about 10 mg/kg of the composition of the invention in the individual to which it is administered. A typical composition will include 50μg/ml of protein.
In addition to OMN antigens, compositions of the invention may include one or more of the following additional antigens:
- a saccharide antigen from N.meningitidis serogroup A, C, W135 and/or Y, such as the oligosaccharide disclosed in ref. 142 from serogroup C [see also ref. 69] or the oligosaccharides of ref. 146.
- antigens from Helicobacter pylori such as CagA [70 to 73], NacA [74, 75], NAP [76, 77, 78], HopX [e.g. 79], HopY [e.g. 79] and/or urease.
- a saccharide antigen from Streptococcus pneumoniae [e.g. 80, 81, 82].
- an antigen from hepatitis A virus, such as inactivated virus [e.g. 83, 84].
- an antigen from hepatitis B virus, such as the surface and/or core antigens [e.g. 84, 85].
- an antigen from hepatitis C virus [e.g. 86]. - a diphtheria antigen, such as a diphtheria toxoid [e.g. chapter 3 of ref. 87].
- a tetanus antigen, such as a tetanus toxoid [e.g. chapter 4 of ref. 87].
- an antigen from Bordetella pertussis, such as pertussis holotoxin (PT) and filamentous haemagglutinin (FHA) from B.pertussis, optionally also in combination with pertactin and/or agglutinogens 2 and 3 [e.g. refs. 88 & 89]; whole-cell pertussis antigen may also be used. — a saccharide antigen from Haemophilus influenzae B [e.g. 69].
- polio antigen(s) [e.g. 90, 91] such as OPV or, preferably, IPV.
- an antigen from N.gonorrhoeae [e.g. 92, 93, 94, 95].
- an antigen from Chlamydia pneumoniae [e.g. refs. 96 to 102].
- an antigen from Porphyromonas gingivalis [e.g. 103]. — rabies antigen(s) [e.g. 104] such as lyophilised inactivated virus [e.g. 105, RabAvert™].
- measles, mumps and/or rubella antigens [e.g. chapters 9, 10 & 11 of ref. 87].
- influenza antigen(s) [e.g. chapter 19 of ref. 87], such as the haemagglutinin and/or neuraminidase surface proteins.
- antigen(s) from a paramyxo virus such as respiratory syncytial virus (RSV [106, 107]) and/or parainfluenza virus (PIN3 [108]).
- an antigen from Moraxella catarrhalis [e.g. 109].
- an antigen from Streptococcus pyogenes (group A streptococcus) [e.g. 110, 111, 112].
- an antigen from Staphylococcus aureus [e.g. 113].
- an antigen from Bacillus anthracis [e.g. 114, 115, 116]. - an antigen from a virus in the flaviviridae family (genus flavivirus), such as from yellow fever virus, Japanese encephalitis virus, four serotypes of Dengue viruses, tick-borne encephalitis virus, West Nile virus.
- a pestivirus antigen, such as from classical porcine fever virus, bovine viral diarrhoea virus, and/or border disease virus.
- a parvovirus antigen e.g. from parvovirus B 19.
- a prion protein (e.g. the CJD prion protein)
- an amyloid protein, such as a beta peptide [117]
- a cancer antigen, such as those listed in Table 1 of ref. 118 or in tables 3 & 4 of ref. 119. The inclusion of further N.meningitidis antigens is preferred. In particular, the composition may include a saccharide antigen from one or more (i.e. 1, 2, 3 or 4) of meningococcal serogroups A, C, W135 and/or Y. Where fewer than 4 of these additional serogroups are included, it is preferred to include at least serogroup C e.g. C+A+W135, C+A+Y, C+W135+Y.
Where a saccharide or carbohydrate antigen is used, it is preferably conjugated to a carrier protein in order to enhance immunogenicity [e.g. refs. 120 to 129]. Preferred carrier proteins are bacterial toxins or toxoids, such as diphtheria or tetanus toxoids. The CRMι 7 diphtheria toxin mutant is particularly preferred [130]. Other carrier polypeptides include the N.meningitidis outer membrane protein [131], synthetic peptides [132, 133], heat shock proteins [134, 135], pertussis proteins [136, 137], protein D from H.influenzae [138], cytokines [139], lymphokines [139], hormones [139], growth factors [139], toxin A or B from C. difficile [140], iron-uptake proteins [141], etc. Different saccharides can be conjugated to the same or different type of carrier protein. Any suitable conjugation reaction can be used, with any suitable linker where necessary. For meningococcal conjugates [142-148], preferred carriers are diphtheria toxoid, CRM197 and H.influenzae protein D.
Toxic protein antigens may be detoxified where necessary e.g. detoxification of pertussis toxin by chemical and/or genetic means [89].
Where a diphtheria antigen is included in the composition it is preferred also to include tetanus antigen and pertussis antigens. Similarly, where a tetanus antigen is included it is preferred also to include diphtheria and pertussis antigens. Similarly, where a pertussis antigen is included it is preferred also to include diphtheria and tetanus antigens. DTP combinations are thus preferred. Antigens in the composition will typically be present at a concentration of at least Iμg/ml each. In general, the concentration of any given antigen will be sufficient to elicit an immune response against that antigen.
As an alternative to using protein antigens in the composition of the invention, nucleic acid encoding the antigen may be used [e.g. refs. 149 to 157]. Protein components of the compositions of the invention may thus be replaced by nucleic acid (preferably DNA e.g. in the form of a plasmid) that encodes the protein.
Methods of treatment
The invention provides a method for raising an immune response in a patient, comprising administering an immunogenic dose of OMNs of the invention to the patient. The immune response is preferably protective and preferably involves antibodies and/or cell-mediated immunity. The method may raise a booster response.
The patient is preferably a human. Where the vaccine is for prophylactic use, the human is preferably a child (e.g. a toddler or infant) or a teenager; where the vaccine is for therapeutic use, the human is preferably a teenager or an adult. A vaccine intended for children may also be administered to adults e.g. to assess safety, dosage, immunogenicity, etc. The patient is preferably less than 20 years old e.g. 13-19 years old, 8-12 years old, 16-24 months old, 6-8 months old, 6 weeks-5 months old.
Vaccines of the invention are preferably administered by intramuscular injection. Typical sites for injection include the upper thigh and the upper arm.
The invention also provides OMVs of the invention for use in medicine.
The invention also provides the use of OMVs of the invention in the manufacture of a medicament for treating and/or preventing meningococcal infection and/or bacterial meningitis.
The invention may be used to elicit systemic and/or mucosal immunity.
Dosage treatment can be a single dose schedule or a multiple dose schedule. Multiple doses may be used in a primary immunisation schedule and/or in a booster immunisation schedule e.g. a primary immunisation schedule may involve three injections, with an interval of about 6 weeks between each injection. A typical volume for a single intramuscular liquid dose is 0.5ml.
Definitions
The term "OMV" as used herein includes any proteoliposomic vesicle obtained by disrupting a bacterial outer membrane to form vesicles of the outer membrane which include protein components of the outer membrane. OMVs are prepared artificially from bacteria (e.g. by detergent treatment) and are thus distinct from microvesicles (MVs [158]) and 'native OMVs' ('NOMVs' [48]), both of which are naturally-occurring membrane vesicles that form spontaneously during bacterial growth and are released into culture medium. MVs can be obtained by culturing Neisseria in broth culture medium, separating whole cells from the smaller blebs in the broth culture medium, and then collecting the MVs from the cell-depleted medium. Strains for use in production of MVs can generally be selected on the basis of the amount of MVs produced in culture e.g. refs. 159 & 160 describe Neisseria with high MV production.
The term "comprising" can mean "including" as well as "consisting" e.g. a composition "comprising" X may consist exclusively of X or may include something additional e.g. X + Y.
The term "about" in relation to a numerical value x means, for example, x+10%. The word "substantially" does not exclude "completely" e.g. a composition which is "substantially free" from Y may be completely free from Y. Where necessary, the word "substantially" may be omitted from the definition of the invention.
BRIEF DESCRIPTION OF DRAWINGS
Figure 1 shows a process including two ultracentrifugation steps without ultrafiltration. Figure 2 shows a process in which one ultracentrifugation step has been replaced by an ultrafiltration step.
MODES FOR CARRYING OUT THE INVENTION
Example 1 — OMVs from meningococcal serogroup B (Norwegian strain)
N.meningitidis serogroup B (strain 44/76, from Norway) was cultured on eight "selective medium for Meningococci" plates at 35°C in 5% CO2/air atmosphere for 24 hours. Cell were harvested into 2 tubes with 12 ml Frantz' medium. Contents of tubes were added to 2x500ml flasks containing Frantz' medium (150ml) and grown with shaking for 12 hours to obtain the correct growth for transferring into 2x5000ml flasks containing Frantz' medium (1500ml). The flasks were grown with shaking for a further 12 hours to yield the inoculum. One flask was added to a Chemap fermentor with 300L capacity, containing 110L of pre-sterilised Frantz' medium and sterile-filtered dialysed yeast extract. The pH after inoculation was 7J, maintained at 7.0 with 3N NaOH. A surface aeration fermentation was performed, controlling the amount of air O2 and stirrer applied, and cultivating for 10 hours at 35°C. Growth was terminated at an OD59onm of 7J0, the fermentor was cooled under 15°C, the air supply was reduced and stirring continued at 100 rpm overnight.
Transfer of the bacterial suspension from the fermentor was done by pressure to a Millipore CUF cross flow filtration unit equipped with valves, pumps and a filter module with 4 Pellicon P2B300V05 polyethersulphone filters (300kD cutoff). Initial transfer of 30L bacterial suspension was followed with a constant volume concentration until the fermentor was emptied, and then a further concentration was performed to give a volume of 5.5L.
Concentrating the suspension was performed in the CFF unit by circulating the suspension to be passing by the filters, with a transmembrane pressure being continuously monitored and kept less then 0.5 bar (observed: 0.5 bar at the end of concentration).
Adjustment of pH of the concentrated bacterial suspension from pH 7.0 to 8J was done by adding, via a tubing system, 5L of 0J M Tris-HCl buffer of pH 9 with 10 mM EDTA, followed by 15 min stirring in the CFF unit to secure uniform conditions. Inactivation/extraction of outer membrane (OM) material was initiated by adding, via tubing, 500 ml of an 0JM Tris-HCl buffer (pH 9) containing 10% deoxycholate (DOC), to give a final concentration of 0.5%. Subsequently the suspension was circulated in the CFF unit for 30 min, and the extracted suspension (9.5L), checked to be completely without living bacteria, was drained off by pumping into a 25L bottle. In a first experiment (experiment A; Figure 1), crude OMVs were prepared by distributing the inactivated suspension to centrifuge tubes of 500ml, and centrifuging in a Beckman centrifuge at 9000 rpm (16650 x g) for 1 hour at 4°C, collecting 8.5L of supernatant. 1J5L of crude OMVs was purified by two subsequent ultracentrifugations at 19000 rpm, 4°C, for 13.6 hours and 6.8 hours respectively, collecting the pellet. The pellet was suspended in 660ml of 3% sucrose with magnetic stirring at room temperature until homogeneous, obtaining a concentration of the purified material of 1.52g/L of total protein.
In a second experiment (experiment B; Figure 2), 3L of crude OMNs were prepared from bacterial suspension using a CUF cross flow filtration unit equipped with valves, pumps and a filter module with 1 Pellicon P2B300V05 polyethersulphone filters (300kD cutoff). Initial transfer of IL crude OMVs was followed with a constant volume concentration until the 3L was finished, and then diafiltered by adding 5L of 0.05 M Tris-HCl buffer of pH 8.6 with 2 mM EDTA, 1% of DOC and 20% sucrose. The retentate obtained was purified by ultracentrifugation at 19000rpm, 4°C, for 6,8 hours, collecting the pellet. The pellet was suspended in IL of 3% sucrose with magnetic stirring at room temperature until homogeneous, obtaining a concentration of 0.85g/L total protein in the purified material.
Final purifications of OMV obtained by both experiment A and B, after a dilution with 3% sucrose around 1 Jg/L of total protein, were both performed at 20°C by filtering through 3 capsule filters (Gelman Science Suporlife DCF) in sequence, first pre filters of 0.8μm and 0.45μm, respectively, then the final sterile filtration (0J2μm), testing 836ml of purified material for experiment A, with an initial protein concentration of 1.1 mg/ml, and IL for experiment B. The OMV protein concentrations after the filtration were 0J2 mg/ml and 0.59 mg/ml respectively.
OMVs were characterised as follows:
Thus the OMVs prepared using ultrafiltration have a similar composition to those obtained by ultracentrifugation. In comparison to the prior art method, however, the method of the invention is much simpler and quicker.
Example 2 — OMVs from meningococcal serogroup B (New Zealand strain)
N.meningitidis serogroup B (strain ΝZ 98/254, from New Zealand) was cultured as before, except that: (a) Catlin medium was used in place of Frantz' medium; (b) the initial 150ml cultures were grown to a level ready for transferring into a Chemap fermentor with 300L capacity, containing 120L
of pre-sterilized medium; (c) growth in the Chemap fermentor was for 12 hours; (d) growth was terminated at OD590nm of 5.90.
Transfer from the fermentor was as before, except that concentration was performed until 5L volume.
Concentration was performed as before. pH was adjusted as before, except that: (a) the final pH was 8.6; (b) the amount of 0J M Tris-HCl buffer added was 6L.
Inactivation/extraction was as before, except: (a) 600 ml of the Tris-HCl buffer was added; (b) the volume of extracted suspension was 19.5L.
Preparation of crude OMVs was as before, except: (a) centrifuge tubes were 1000ml volume; (b) centrifugation was at 8000 rpm (16650 x g), to give 17.5L of supernatant.
Cross-flow filtration for purifying OMVs (in place of centrifugation) was as in experiment B above, except: (a) using 17.5L crude OMVs; (b) using two P2B300V05 polyethersulphone filters (300kD cutoff); (c) using an initial transfer of 4L crude OMVs; (d) diafiltration with 30L Tris-HCl buffer; (e) pellet was resuspended in 1JL of 3% sucrose; (f) the homogenous material was further sonicated, and gave a final concentration of purified material of 1.5g/L total protein.
Final purification was as before, except: (a) filtration was through two capsule filters (Sartoclean CA, Sartobran P) in sequence, first pre-filters of 0.8+0.65 μm, then a final sterile filtration 0.45+0.22 μm. The OMV protein concentration after the filtration was 1.0 g/L.
OMVs were characterised as follows:
Thus the production method provided OMVs with a native antigen mosaic and a strongly reduced level of LPS. In comparison to the prior art method where two ultracentrifugation steps are used, however, the invention is much simpler and quicker.
Example 3 — OMVs from meningococcal serogroup B (New Zealand strain) Crude OMNs were prepared from the 98/254 strain as described above. The pH was adjusted to between 7.5 and 9.0 (typically between 8J and 8.5) with buffer, and then concentrated up to 20 litres by ultrafiltration for between 3.5 and 4.5 hours using Polysulphone Millipore Pellicon 2 cassettes with a surface area of 3m2. The concentrate material was diafiltered against 7 volumes of a solution containing Tris-EDTA, 1% DOC and 20% sucrose ('buffer B'), and then with 3 volumes of 'buffer Bl' (same as 'buffer B' but with only 0.5% DOC). The retentate was concentrated again up to 4 litres and collected. The ultrafiltration system was washed with buffer Bl. The retentate was then washed, and OMVs (retentate + washes) were stored at 2-8°C. The bioburden in the final material was zero, and endotoxin content was <0.05 Ul/ml. The process showed excellent lot-to-lot consistency. The stored material was centrifuged in a Beckman Coulter Optima XL 100K ultracentrifuge using a type 19 rotor and 250ml Beckman bottles (220+10ml material per bottle), 19000rpm for 408 minutes at 2-8°C. Pellets were washed in 10ml of a 3% sucrose solution, and were then re-suspended in 3% sucrose (60ml volume added) using a 700rpm magnetic agitator (2.5cm bar) in 250ml Beckman bottles. Re-suspended material was sonicated for 300 minutes at <20°C. If necessary, the sonicated material was diluted with 3% sucrose solution to give a final protein concentration of lJmg/ml. The bioburden in the final material was zero, and the process showed excellent lot-to-lot consistency.
The OMVs were subjected to a final filtration step, first through 0.8-0.65μm filters and then through 0J2μm filters. The sonicated OMVs were passed into a sterile glass container with Sartoclean CA 0.8-0.65μm OJm2 pre-filters. This pre-filtration was performed for 5-6 minutes with a peristaltic pump using only one set of filters. The filtrate was then passed into a second sterile glass container with Sartobran P 0.45-0J2μm 0.4m2 filters. This filtration lasted 7-10 minutes, again with peristaltic pumps. The pre-filters were first rinsed with 500-600ml of 3% sucrose, and the 0J2μm filters were washed with 200ml of 5% sucrose after filtration. Final OMV material was stored at 2-8°C, and contained <0J6μg LPS per μg of protein and <0.4μg DOC per μg of protein. Bioburden was zero. Protein content in the OMNs was between 800μg/ml and lOOOμg/ml.
It will be understood that the invention has been described by way of example only and modifications may be made whilst remaining within the scope and spirit of the invention.
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