CA1276552C - Conjugate vaccine against infections by gram-negative bacteria, method for its preparation and use - Google Patents
Conjugate vaccine against infections by gram-negative bacteria, method for its preparation and useInfo
- Publication number
- CA1276552C CA1276552C CA000517689A CA517689A CA1276552C CA 1276552 C CA1276552 C CA 1276552C CA 000517689 A CA000517689 A CA 000517689A CA 517689 A CA517689 A CA 517689A CA 1276552 C CA1276552 C CA 1276552C
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- CA
- Canada
- Prior art keywords
- conjugate
- vaccine
- polysaccharide
- preparation
- vaccines
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Expired - Lifetime
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Classifications
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K16/00—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies
- C07K16/12—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from bacteria
- C07K16/1203—Immunoglobulins [IGs], e.g. monoclonal or polyclonal antibodies against material from bacteria from Gram-negative bacteria
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
- A61K39/02—Bacterial antigens
- A61K39/025—Enterobacteriales, e.g. Enterobacter
- A61K39/0258—Escherichia
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
- A61K39/02—Bacterial antigens
- A61K39/104—Pseudomonadales, e.g. Pseudomonas
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
- A61K2039/60—Medicinal preparations containing antigens or antibodies characteristics by the carrier linked to the antigen
- A61K2039/6031—Proteins
- A61K2039/6037—Bacterial toxins, e.g. diphteria toxoid [DT], tetanus toxoid [TT]
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y02—TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
- Y02A—TECHNOLOGIES FOR ADAPTATION TO CLIMATE CHANGE
- Y02A50/00—TECHNOLOGIES FOR ADAPTATION TO CLIMATE CHANGE in human health protection, e.g. against extreme weather
- Y02A50/30—Against vector-borne diseases, e.g. mosquito-borne, fly-borne, tick-borne or waterborne diseases whose impact is exacerbated by climate change
Abstract
Abstract of the disclosure:
The invention relates to a non-toxic conjugate vaccine against infections by Gram-negative bacteria, composed of a species-specific polysaccharide and a protein which are covalently linked together, it being characteristic of the vaccine that the polysaccharide originates from the endotoxin of the bacterium and the protein is an exoprotein.
The vaccines according to the invention are, in particular, vaccines against infections by Pseudomonas aeruginosa or Escherichia coli.
The exoprotein is, in particular, an exotoxin or exotoxoid, preferably toxin A from Pseudomonas aeru-ginosa, but also a tetanus toxoid or diphtheria toxoid.
The process for the preparation of the new con-jugate vaccine against infections by Gram-negative bacteria comprises covalent linkage of an appropriate polysaccharide from the endotoxin of the bacterium with an exoprotein.
However, the invention also relates to a con-jugate vaccine composed of a mixture of 3-15 conjugates whose polysaccharide have (sic) been obtained from 3-15 different serotypes of the same species of bacteria.
The invention further relates to a polyvalent vaccine composed of a mixture of conjugate vaccines, each of whose individual components raises antibodies against a particular species of bacteria.
The invention further relates to the use of the new conjugate vaccines for the preparation of hyper-immune sera which in turn are used for the preparation of immunoglobulin which can be administered intra-venously or intramuscularly.
The invention relates to a non-toxic conjugate vaccine against infections by Gram-negative bacteria, composed of a species-specific polysaccharide and a protein which are covalently linked together, it being characteristic of the vaccine that the polysaccharide originates from the endotoxin of the bacterium and the protein is an exoprotein.
The vaccines according to the invention are, in particular, vaccines against infections by Pseudomonas aeruginosa or Escherichia coli.
The exoprotein is, in particular, an exotoxin or exotoxoid, preferably toxin A from Pseudomonas aeru-ginosa, but also a tetanus toxoid or diphtheria toxoid.
The process for the preparation of the new con-jugate vaccine against infections by Gram-negative bacteria comprises covalent linkage of an appropriate polysaccharide from the endotoxin of the bacterium with an exoprotein.
However, the invention also relates to a con-jugate vaccine composed of a mixture of 3-15 conjugates whose polysaccharide have (sic) been obtained from 3-15 different serotypes of the same species of bacteria.
The invention further relates to a polyvalent vaccine composed of a mixture of conjugate vaccines, each of whose individual components raises antibodies against a particular species of bacteria.
The invention further relates to the use of the new conjugate vaccines for the preparation of hyper-immune sera which in turn are used for the preparation of immunoglobulin which can be administered intra-venously or intramuscularly.
Description
6SS~
Conjugate vaccines against infections by Gram-negative b~cteria, process for their preparation and us~ thereof The invention relates to non-toxic conjugate vaccines against infections by Gram-negative bacteria, in particu-S lar against infections by Pseudomonas aeruginosa and Escherichia coli, to the process for the preparation of vaccines of this type, and to their use for the pre-paration of hyperimmune sera which in turn are used for the preparation of immunoglobulin.
Infections by Pseudomonas aeruginosa or Esche-richia coli occur particularLy in hospitalized patients, victims of burns and cancer patients who are treated with immunosuppressants. They are one of the main causes of life-threatening "nosocomial" infections in populations accommodated in a confined space (hospital pitalized).
H.Y. Reynolds et al. Pseudomonas aeruginosa infections:
Persisting problems and current research to find new therapies. Annals Internal Medic;ne 82:819-831 (1975).
The incidence of intections of this type has increased drastically in parallel with the widespread use of anti-biotics in the past 30 ye3rs.
Pseudomonas aeruginosa and Escherichia coli are also frequently the cause of urinary tract infections~
otitis, sinusitis and meningitis.
Antibodies against a number of somatic antigens of pseudomonas aerug;nosa (see, for example, H.E.
Gilleland et al: Use of Pseudomonas Aeruginosa as a protective vaccine in mice. Infection Immunity 44: 49-54 (1984)) and against extracellular protein (O.R.
Pavlovskis et al. Protection against experimental Pseu-domonas aeruginosa infection in mice by active immuniz-ation ~ith exotoxin A toxoids. Infection Immunity 32: 681-689 (1981)) have proved to be an effective pro-tection against infection in animal experiments.
Toxin A is the most toxic product of the meta-bolism of Pseudomonas aeruginosa (P.a.). It prevents eukaryotic /~rotein synthesis. Mutants of P.a. with specific toxin A deficiency are less virulent than ,;: .
- ~27655~
their parent strains (D.E. Ohman et al. Corneal intec-tions in mice with toxin A and elastase mutants of P.a.
J. lnfectious Diseases 142: 547-555 (1980)). Antitoxin A antibodies administered passively or raised by active v3ccination generate a clearly detectable protection against experimentally produced P.a. infections (compare O.R. Pavlovskis et al , loc. cit and Infection Immunity 18: 596-602 (1977)). Further investigations have shown a direct association between the content of antitoxin anti-body and the survival rate of patients suffering from P.a. bacteremia (M.S. Pollack et al. Protective activity of antibodies to exotoxin A and lipopolysaccharide at the onset of P.a. septicemia in man. J. Clinical Investi-gation 63: 276-286 (1979)).
The virulence of P.a. in mice traumati2ed by burns depends on the presence of a complete "smooth-type"
lipopolysaccharide molecule (S.J. Cryz et al., Infection Immunity 44: 50~-513 (1984)).
The protective effect of serotype-specific anti-lipopolysaccharide antibodies against experimental P.a.
infections is adequately documented. (Compare, for example, S.J. Cryz et al~, Infection Immunity 43:
795-799 (1984)).
! Increased anti-lipopolysaccharide antibody titers strikingly increase the survival time of patients suffer-; ing from P.a. septicemia (A.S. Cross et al., J. Infect-ious Diseases 142: 538-546 (1980)). Clinical trials with vaccines based on P.a. lipopolysaccharide produced I very promising results (J.W. Alexander et al., J.
, 30 Infectious Diseases 130 (Suppl.): 5152-S158 (1974).
I Although P.a. lipopolysaccharide (LPS) contains protec-tive serotype-specific antigenic determinants, it cannot be employed as a parenteral vaccine for practical use be-I cause its ~oxicity in humans is too high (J.E. Pennington, ¦ 35 J. Infectious Diseases 130 (Suppl.): S159 S162 (1974);
¦ M.D. Haghbin et al.~ Cancer 32: 761-762 (1973)).
¦ The serotype-specific antigenic determinants of P.a. are accommodated in the O~polysaccharide (PS) part of the LPS molecule~ The polysaccharide (PS) can be 12~7~S52 separated and isoLated from the toxic lipid A half of the ~ipopolysaccharide ~LPS). Although PS contains the antigenic determinants PS cannot be used as a vaccine sinte PS is non-immunogenic (G.~. Pier et al., Infect;on Immunity 22: 919-925 (1978)).
To date no effective vaccine for the prevention of P.a. infections and infections by similar Gram-negative bacteria such as, for examPle, Eschericia coLi tE.c~) exists. In v;ew of the relative frequency of infections by P.a. or E.c. and their ha~ardousness this is a considerable deficiency.
Apart from the necessity to make available an effective vaccine for active immunization against infect-ions of this type, there is a pressing need for immuno-globulins from specific hyperimmune sera which contain a high titer of antibodies against Gram-negative bacteria, especially P.a. and E.c. These types of sera or immuno-globulins may alone be life-savers in cases of bacteremia or septicemia.
Antibiotics often fail owing to resistance of the microbes.
The aim of the present invention is to close these serious gaps in the medical management of in-fectious diseases. This is obviously possible only ~ith a conjugate vaccine.
Conjugate vaccines, obtained in particular by covalent linkage of, for example, lipopolysaccharides ~ith human serum albumin, are disclosed in, for ex-ample, American Patent Specification 4,185,090.
Methods for the covalent linkage of species-specific polysaccharides ~ith species-specific proteins are well known and widespread.
European Published Specification 118,831 des-cribes immunizing compositions against Gram-negative 35. bacteria, which were obtained by covalent coupling of detoxified endoprotein with detoxified polysaccharide of the same species of bacteria.
The efficacy of kno~n conjugate vaccines is modest and has not undergone clinical testing.
~.~7655~:
It has now been found that non-toxic and, at the same time, h;ghly effective conjugate vaccines can be obtained when LPS isolated from P~a. is converted into PS
and covalently coupled with an exoprotein composed either S of a P.a. toxin A, of a tetanus toxoid or a diphtheria toxoid. The resulting PS-toxin A, PS-tetanus toxoid and PS-diphtheria toxoid conjugate vaccines have proved to be non-toxic and immunogenic. They produced an effective protection against experimental P.a. infections.
lt has also been found that the new principle of covalent coupling of PS to exoProteins can be generalized and thus used for the preparation of vaccines also against infections by other Gram-negative bacteria, especially Escherichia coli (E.c.) infections.
Accordingly, the invention relates to a non-toxic conjugate vaccine against infections by Gram-negative bacteria, composed of a species-specific polysaccharide and a protein which are covalently linked together, it being character;stic of the vaccine that the polysaccha-ride originates from the endotoxin of the bacterium and the protein is an exoprotein.
The vaccines according to the invention are, in particular, vaccines against infections by Pseudomonas aeruginosa or Escherichia coli.
The exoprotein is~ in particular, an exotoxin or exotoxoid, preferably toxin A from Pseudomonas aeruginosa, but also a tetanus toxoid or diphtheria toxoid The process for the preparation of the ne~ conju-gate vaccine against infections by Gram-negative bacteria compr-ses covalent linkage of an appropriate polysaccha-ride from the endotoxin of the bacterium with an exopro-tein.
Ho~ever, the invention also relates to a conju-gate vaccine composed of a mixture of 3-15 conjugates ~hose polysaccharide has been obtained from 3-15 different serotypes of the same sQecies of bacteria.
The ;nvention further relates to a polyvalent vaccine composed of a mixture of conju~ate vaccines~
each of whose inrJividual components raises antibodies ~ 27~i5~
against a particu~ar species of bacteria.
The invention further relates to the use of the new conjugate vaccines for the preparation of hyper-immune sera ~hich in turn are used for the preparation of immunoglobulin which can be administered intra-venously or intramuscularly.
Description of the production of the vaccine by the example of a Pseudomonas aeruginosa vaccine Production of the endotoxin (PS):
A very particular serotype of P.a. is used as the source for the production of the endotox;n for the pre~
; paration of the vaccine against P.a. according to the invention. The lipopolysaccharide (LPS) from the bac teria is obtained by, for example, phenol/water extract-ion by the method of 0. Westphal et al., Zeitschr.
Naturforschung: 148-155 (1952). The LPS obtained contains less than 1% by weight of protein and nucleic acids. The 0-polysaccharide (PS) is detached from the LPS by hydro-lysis with di;ute acetic acid at 100C. Method: I.R.
~ 20 Chester et al., J. General Microbiology 78: 305-318 ! (1973). The insoluble, toxic lipid A part is separated j by centrifugation. The supernatant is extracted with a chloroform/methanol solution in order to remove residues of lipid AD The aqueous phase, ~hich contains the PS, ;s concentrated in vacuo and then purified by chromato-graphy, polysaccharide (PS) with a molecular weight of 10,0ûO to 75,000 being collected and freeze-dried.
Oxidation of PS:
The resulting polysaccharide (PS) is oxidized in water by the addition of sodium periodate at room tempera-ture, this producing aldehyde groups capable of coupling.
After addition of ethylene glycol, the material is puri-fied by dialysis and then freeze-dried.
¦ Procluction of exoprotein (toxin A):
Toxin A ~ith a purity of more than 95% is obtained, by the method of S.J. Cryz et al., lnfection Inmuni~y 43:
795-799 (1q84), from a Pseudomonas aeruginosa strain ~hich provides an especially large amount of toxin A.
~Z~655~
Synthe s of toxin A-coupler:
An a~iphatic dicarboxylic acid dihydrazide and carbodiimide such as, for example, 1-ethyl-3(3-di-methylaminopropyl)carbodiimide is added to dilute toxin S A. This operation results in free carboxyl grûups of the toxin A being linked with the dicarboxylic acid di-hydrazide. The resulting product can be depicted by, for example, the following formula:
(Toxin A)-C0-NH-N~-CO(CH2)1 6-C0-NH-NH2 Synthesis of Pseudomonas polysaccharide/toxin A
con~ugate:
~ he resulting toxin A-coupler is linked ~ith the oxidized PS which has aldehyde groups by mixing equiva-lent amounts of toxin A-coupler and ùxidized PS and re-ducing the resulting Schiff's base (hydrazone) with analkali metal borohydride such as, for example, with NaBH4 or Na~H3CN.
This results in the formation of a stable con-jugate whose structure has not been elucidated but can be imagined to be approximately as sho~n in the follow;ng diagram, inter alia:
~Tox~n A)-C0-NH-NH-C0-(CH2)1 6-C0-NH-NH-(Po1ysaccharide.) The conjugate is purified by di3lysis, insoluble material is removed by centrifugation, and the res~lting mixture is separated by chromatography on an agarose column. Material with a molecular ~eight of more than 350,000, which markedly exceeds the molecular weight of PS and of toxin A and ~hich represents the PS-toxin A
conjugate, is removed and freeze-dried.
Synthesis of polysaccharide-tetanus toxoid conjugate Tetanus toxoid ; A tetanus toxoid specified for use in humans - for example TE Anatoxin(R) o~ the Schweiz. Serum- und Impf-institut is purified by ion exchange chromatography on cellulose and gel filtration on agarose in such a manner that it is composed of 90Z of tetanus toxoid.
~19Z765S~
cOupl ing Th;s is carried out in this instance by, for example, the general method of Jerker Porath, Methods in Enzymology Vol. 34, pages 21 et seq. Polysatcharide (PS) which has been obtained from LPS by hydrolysis is not oxidized ~or this coupling but is reacted in aqueous solution with cyanogen bromide in alkaline medium at room temperature in a manner known per se. This entails the cyanogen bromide ~BrCN) reacting with free -OH groups of the polysaccharide, formulated diagrammatically as (PS)-OH below. The activated polysaccharides thus obtained can be reacted with an alkylenedicarboxylic acid di-hydrazide tfor example H2NNHCO-(CH2)1_6-CONH-NH2) such as, for example, adipic acid dihydrazide (AD~). This entails the dihydrazide being covalently bonded to the polysaccharide. The reactions taking place during the linkage can be illustrated, inter alia, approximately as follows, for example:
(P5)-OH + BrCN ~ (PS)-O-C-N ~ H2N-NHCO-(CH2)l 6-CO-NH-NH2 (PS)-O-C(NH)-NH-NH-CO-(CH2)l_6-CO-NH-NH2 + H20 (PS)-O-CO-NH-NH-CQ-(CH2)1_6-CO-NH-NH2, The PS-dihydrazide conjugate obtained thereby is purified by thorough dialysis. The solution is made weakly acid by addi~ion of a dilute mineral acid, and an equivalent amount of tetanus toxoid and a carbodiimide are added, and the mixture is stirred at room temperature for some hours. The reaction with the toxoid (formulated diagram-matically as HOCO-ttoxoid)~ in the presence of carbodi-imide entails condensation of free carboxyl groups in the toxoid-with free hydrazide groups in the PS-di-j hydrazide conjugate and production of the desired PS-dihydrazidetoxoid conjugate, ~hose structure has not been elucidated but can be imagined to be approximately as shown in the following diagram:
O (CH2)l 6 CO NH NH CO (Toxoid3 The resulting mixture is dialy~ed against a phosphate buffer and chromatographed on an agarose column.
Material with a molecul2r weight of over 350,000, ~hich -` ~L2~7655i~
-- ~ o markedly exceeds the molecular weight of the starting components, is removed and freeze-dried. In the above synthesis it is also possible to replace the tetanus toxoid by diphtheria toxoid.
It is also possible in a manner analogous to that described above to produce vaccines against other Gram-negative bacteria such as, for example, against infections by Escherichia coli.
Determination of the safety and effi_cacy of the conjug-ate vaccines according to the invention Properties_of the Pseudomonas (PS-toxin_A?, (PS-tetanus toxoid) and (PS-diphtheria toxoid) , conjugates accord-ng to the invention:
It is evident from the data in Table 1 (page 12) that the conjugates have a molecular weight greater than 350,0aO and thus far exceed the molecular weight of the starting materials. The covalent bonding of the toxin A
results in this highly toxic agent being detoxified. This entails the lethal dose increasing by at least 1,000-fold~
from 0.2 ~ug~mouse to more than 200 ~g/mouse~ The pyrogeni-city of the conjugates has, compared with that of natural Pseudomonas aeruginosa PA 22~ LPS (0.7 ~g/ml/kg body weight), virtually disappeared.
The conjugates induce specific antibody responses both against the polysaccharide and against the protein carrier, that is to say against toxin A, against tetanus toxin or against diphtheria toxin. The covalent bonding of toxin A to the polysaccharide results in the toxin A
being completely detoxified without thereby losing its immunogenic activity~
It has been possible to demonstrate the ability of (PS-toxin A) conjugate = (PS-toxin A) conjugate vaccine to protect mice against l~thal poisoning ~ith purified toxin A as follows, for example:
Groups of mice recei~ed intramuscular adminis-trations, at the start of the test and on the 14th day of the test, of either 10 ~9 of protein in the form of corresponding amounts of (PS-toxin A) conjugate or a buffer (control group). On the 28th day of the test 7~ 2 ~, gradually increasing doses of toxin A were administered to the mice. The median lethal dose for the control ani-mals was 0.2 ~9, whereas the median lethal dose for the animals pretreated with (PS-toxin A~ conjugate was 4.7 ug/mouse.
Eff;cacy of (PS-tetanus toxoid) conjugate and of (PS-toxin A) conjugate as ~accine .. _ .... _ The ability of natural liPopolysaccharide (LPS
from Pseudomonas aeruginosa)" (PS-tetanus toxoid) con-jugate and of (PS-toxin A) conjugate to protect experi-mental animals against experimentally generated Pseudo-monas aeruginosa sePsis of burns is demonstrated by Table 2~ page 13.
The data demonstrate that the immunization with LPS, (PS-tetanus toxoid) conjugate and with (PS-toxin A) conjugate produces a protective effect of about the same strength against fatal P.a. sepsis. The lethal dose of P. aeruginosa PA Z20 is increased by S0,000-fold, com-pared ~ith the non-immunized control group, by this.
Safety and immunogenicity of (PS-tetanus toxoid) conju-.
gate vaccine in humans Healthy adult volunteers of both sexes and 16 to59 years of age received 1ûO ~9 of the conjugate vaccine in 0.5 ml administered subcutaneously in the upper arm at the start of the test and after 14 days.
All the reastions of the test subjects were re~
corded. Secondary reactions were rare, minor and tran-sient. Venous blood samples were taken at the start of the test and 14 and 28 days after the inoculation. The sera obtained from the blood samples were collected and stored at -20C. The immunoglob~lin G (IgG) antibody titers ~ere determined.
The immunization with tPS-tetanus toxoid) conjugate resulted in a significant rise, compared with the initial titer, in the mean anti-PA 2Z0 LPS IgG titer after 14 and 28 days from the innoculation. See Table 3, page 15.
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Table 2:
Protection against lethal sepsis of burns, caused by Pseudomonas aeruginosa PA 220, by immunization with LPS
of PA 220, (PS-tetanus toxoid) conjugate and with (PS-toxin A) conjugate Immunogen1) LDS~) None (controls) 20 PS-tetanus toxoid conjugate 106 PS-toxin A
conjugate 1û6 1) Mice rece;ved 1 ~9 i.m. before the start of the test and on the 14th day of the test. They ~ere then sub-jected to a burn injury (method: I~A. Holder et al., Infection Immunity 35. 276-Z80 (1982) and on the 28th day were exposed to increasing doses of P.
aeruginosa 220.
Conjugate vaccines against infections by Gram-negative b~cteria, process for their preparation and us~ thereof The invention relates to non-toxic conjugate vaccines against infections by Gram-negative bacteria, in particu-S lar against infections by Pseudomonas aeruginosa and Escherichia coli, to the process for the preparation of vaccines of this type, and to their use for the pre-paration of hyperimmune sera which in turn are used for the preparation of immunoglobulin.
Infections by Pseudomonas aeruginosa or Esche-richia coli occur particularLy in hospitalized patients, victims of burns and cancer patients who are treated with immunosuppressants. They are one of the main causes of life-threatening "nosocomial" infections in populations accommodated in a confined space (hospital pitalized).
H.Y. Reynolds et al. Pseudomonas aeruginosa infections:
Persisting problems and current research to find new therapies. Annals Internal Medic;ne 82:819-831 (1975).
The incidence of intections of this type has increased drastically in parallel with the widespread use of anti-biotics in the past 30 ye3rs.
Pseudomonas aeruginosa and Escherichia coli are also frequently the cause of urinary tract infections~
otitis, sinusitis and meningitis.
Antibodies against a number of somatic antigens of pseudomonas aerug;nosa (see, for example, H.E.
Gilleland et al: Use of Pseudomonas Aeruginosa as a protective vaccine in mice. Infection Immunity 44: 49-54 (1984)) and against extracellular protein (O.R.
Pavlovskis et al. Protection against experimental Pseu-domonas aeruginosa infection in mice by active immuniz-ation ~ith exotoxin A toxoids. Infection Immunity 32: 681-689 (1981)) have proved to be an effective pro-tection against infection in animal experiments.
Toxin A is the most toxic product of the meta-bolism of Pseudomonas aeruginosa (P.a.). It prevents eukaryotic /~rotein synthesis. Mutants of P.a. with specific toxin A deficiency are less virulent than ,;: .
- ~27655~
their parent strains (D.E. Ohman et al. Corneal intec-tions in mice with toxin A and elastase mutants of P.a.
J. lnfectious Diseases 142: 547-555 (1980)). Antitoxin A antibodies administered passively or raised by active v3ccination generate a clearly detectable protection against experimentally produced P.a. infections (compare O.R. Pavlovskis et al , loc. cit and Infection Immunity 18: 596-602 (1977)). Further investigations have shown a direct association between the content of antitoxin anti-body and the survival rate of patients suffering from P.a. bacteremia (M.S. Pollack et al. Protective activity of antibodies to exotoxin A and lipopolysaccharide at the onset of P.a. septicemia in man. J. Clinical Investi-gation 63: 276-286 (1979)).
The virulence of P.a. in mice traumati2ed by burns depends on the presence of a complete "smooth-type"
lipopolysaccharide molecule (S.J. Cryz et al., Infection Immunity 44: 50~-513 (1984)).
The protective effect of serotype-specific anti-lipopolysaccharide antibodies against experimental P.a.
infections is adequately documented. (Compare, for example, S.J. Cryz et al~, Infection Immunity 43:
795-799 (1984)).
! Increased anti-lipopolysaccharide antibody titers strikingly increase the survival time of patients suffer-; ing from P.a. septicemia (A.S. Cross et al., J. Infect-ious Diseases 142: 538-546 (1980)). Clinical trials with vaccines based on P.a. lipopolysaccharide produced I very promising results (J.W. Alexander et al., J.
, 30 Infectious Diseases 130 (Suppl.): 5152-S158 (1974).
I Although P.a. lipopolysaccharide (LPS) contains protec-tive serotype-specific antigenic determinants, it cannot be employed as a parenteral vaccine for practical use be-I cause its ~oxicity in humans is too high (J.E. Pennington, ¦ 35 J. Infectious Diseases 130 (Suppl.): S159 S162 (1974);
¦ M.D. Haghbin et al.~ Cancer 32: 761-762 (1973)).
¦ The serotype-specific antigenic determinants of P.a. are accommodated in the O~polysaccharide (PS) part of the LPS molecule~ The polysaccharide (PS) can be 12~7~S52 separated and isoLated from the toxic lipid A half of the ~ipopolysaccharide ~LPS). Although PS contains the antigenic determinants PS cannot be used as a vaccine sinte PS is non-immunogenic (G.~. Pier et al., Infect;on Immunity 22: 919-925 (1978)).
To date no effective vaccine for the prevention of P.a. infections and infections by similar Gram-negative bacteria such as, for examPle, Eschericia coLi tE.c~) exists. In v;ew of the relative frequency of infections by P.a. or E.c. and their ha~ardousness this is a considerable deficiency.
Apart from the necessity to make available an effective vaccine for active immunization against infect-ions of this type, there is a pressing need for immuno-globulins from specific hyperimmune sera which contain a high titer of antibodies against Gram-negative bacteria, especially P.a. and E.c. These types of sera or immuno-globulins may alone be life-savers in cases of bacteremia or septicemia.
Antibiotics often fail owing to resistance of the microbes.
The aim of the present invention is to close these serious gaps in the medical management of in-fectious diseases. This is obviously possible only ~ith a conjugate vaccine.
Conjugate vaccines, obtained in particular by covalent linkage of, for example, lipopolysaccharides ~ith human serum albumin, are disclosed in, for ex-ample, American Patent Specification 4,185,090.
Methods for the covalent linkage of species-specific polysaccharides ~ith species-specific proteins are well known and widespread.
European Published Specification 118,831 des-cribes immunizing compositions against Gram-negative 35. bacteria, which were obtained by covalent coupling of detoxified endoprotein with detoxified polysaccharide of the same species of bacteria.
The efficacy of kno~n conjugate vaccines is modest and has not undergone clinical testing.
~.~7655~:
It has now been found that non-toxic and, at the same time, h;ghly effective conjugate vaccines can be obtained when LPS isolated from P~a. is converted into PS
and covalently coupled with an exoprotein composed either S of a P.a. toxin A, of a tetanus toxoid or a diphtheria toxoid. The resulting PS-toxin A, PS-tetanus toxoid and PS-diphtheria toxoid conjugate vaccines have proved to be non-toxic and immunogenic. They produced an effective protection against experimental P.a. infections.
lt has also been found that the new principle of covalent coupling of PS to exoProteins can be generalized and thus used for the preparation of vaccines also against infections by other Gram-negative bacteria, especially Escherichia coli (E.c.) infections.
Accordingly, the invention relates to a non-toxic conjugate vaccine against infections by Gram-negative bacteria, composed of a species-specific polysaccharide and a protein which are covalently linked together, it being character;stic of the vaccine that the polysaccha-ride originates from the endotoxin of the bacterium and the protein is an exoprotein.
The vaccines according to the invention are, in particular, vaccines against infections by Pseudomonas aeruginosa or Escherichia coli.
The exoprotein is~ in particular, an exotoxin or exotoxoid, preferably toxin A from Pseudomonas aeruginosa, but also a tetanus toxoid or diphtheria toxoid The process for the preparation of the ne~ conju-gate vaccine against infections by Gram-negative bacteria compr-ses covalent linkage of an appropriate polysaccha-ride from the endotoxin of the bacterium with an exopro-tein.
Ho~ever, the invention also relates to a conju-gate vaccine composed of a mixture of 3-15 conjugates ~hose polysaccharide has been obtained from 3-15 different serotypes of the same sQecies of bacteria.
The ;nvention further relates to a polyvalent vaccine composed of a mixture of conju~ate vaccines~
each of whose inrJividual components raises antibodies ~ 27~i5~
against a particu~ar species of bacteria.
The invention further relates to the use of the new conjugate vaccines for the preparation of hyper-immune sera ~hich in turn are used for the preparation of immunoglobulin which can be administered intra-venously or intramuscularly.
Description of the production of the vaccine by the example of a Pseudomonas aeruginosa vaccine Production of the endotoxin (PS):
A very particular serotype of P.a. is used as the source for the production of the endotox;n for the pre~
; paration of the vaccine against P.a. according to the invention. The lipopolysaccharide (LPS) from the bac teria is obtained by, for example, phenol/water extract-ion by the method of 0. Westphal et al., Zeitschr.
Naturforschung: 148-155 (1952). The LPS obtained contains less than 1% by weight of protein and nucleic acids. The 0-polysaccharide (PS) is detached from the LPS by hydro-lysis with di;ute acetic acid at 100C. Method: I.R.
~ 20 Chester et al., J. General Microbiology 78: 305-318 ! (1973). The insoluble, toxic lipid A part is separated j by centrifugation. The supernatant is extracted with a chloroform/methanol solution in order to remove residues of lipid AD The aqueous phase, ~hich contains the PS, ;s concentrated in vacuo and then purified by chromato-graphy, polysaccharide (PS) with a molecular weight of 10,0ûO to 75,000 being collected and freeze-dried.
Oxidation of PS:
The resulting polysaccharide (PS) is oxidized in water by the addition of sodium periodate at room tempera-ture, this producing aldehyde groups capable of coupling.
After addition of ethylene glycol, the material is puri-fied by dialysis and then freeze-dried.
¦ Procluction of exoprotein (toxin A):
Toxin A ~ith a purity of more than 95% is obtained, by the method of S.J. Cryz et al., lnfection Inmuni~y 43:
795-799 (1q84), from a Pseudomonas aeruginosa strain ~hich provides an especially large amount of toxin A.
~Z~655~
Synthe s of toxin A-coupler:
An a~iphatic dicarboxylic acid dihydrazide and carbodiimide such as, for example, 1-ethyl-3(3-di-methylaminopropyl)carbodiimide is added to dilute toxin S A. This operation results in free carboxyl grûups of the toxin A being linked with the dicarboxylic acid di-hydrazide. The resulting product can be depicted by, for example, the following formula:
(Toxin A)-C0-NH-N~-CO(CH2)1 6-C0-NH-NH2 Synthesis of Pseudomonas polysaccharide/toxin A
con~ugate:
~ he resulting toxin A-coupler is linked ~ith the oxidized PS which has aldehyde groups by mixing equiva-lent amounts of toxin A-coupler and ùxidized PS and re-ducing the resulting Schiff's base (hydrazone) with analkali metal borohydride such as, for example, with NaBH4 or Na~H3CN.
This results in the formation of a stable con-jugate whose structure has not been elucidated but can be imagined to be approximately as sho~n in the follow;ng diagram, inter alia:
~Tox~n A)-C0-NH-NH-C0-(CH2)1 6-C0-NH-NH-(Po1ysaccharide.) The conjugate is purified by di3lysis, insoluble material is removed by centrifugation, and the res~lting mixture is separated by chromatography on an agarose column. Material with a molecular ~eight of more than 350,000, which markedly exceeds the molecular weight of PS and of toxin A and ~hich represents the PS-toxin A
conjugate, is removed and freeze-dried.
Synthesis of polysaccharide-tetanus toxoid conjugate Tetanus toxoid ; A tetanus toxoid specified for use in humans - for example TE Anatoxin(R) o~ the Schweiz. Serum- und Impf-institut is purified by ion exchange chromatography on cellulose and gel filtration on agarose in such a manner that it is composed of 90Z of tetanus toxoid.
~19Z765S~
cOupl ing Th;s is carried out in this instance by, for example, the general method of Jerker Porath, Methods in Enzymology Vol. 34, pages 21 et seq. Polysatcharide (PS) which has been obtained from LPS by hydrolysis is not oxidized ~or this coupling but is reacted in aqueous solution with cyanogen bromide in alkaline medium at room temperature in a manner known per se. This entails the cyanogen bromide ~BrCN) reacting with free -OH groups of the polysaccharide, formulated diagrammatically as (PS)-OH below. The activated polysaccharides thus obtained can be reacted with an alkylenedicarboxylic acid di-hydrazide tfor example H2NNHCO-(CH2)1_6-CONH-NH2) such as, for example, adipic acid dihydrazide (AD~). This entails the dihydrazide being covalently bonded to the polysaccharide. The reactions taking place during the linkage can be illustrated, inter alia, approximately as follows, for example:
(P5)-OH + BrCN ~ (PS)-O-C-N ~ H2N-NHCO-(CH2)l 6-CO-NH-NH2 (PS)-O-C(NH)-NH-NH-CO-(CH2)l_6-CO-NH-NH2 + H20 (PS)-O-CO-NH-NH-CQ-(CH2)1_6-CO-NH-NH2, The PS-dihydrazide conjugate obtained thereby is purified by thorough dialysis. The solution is made weakly acid by addi~ion of a dilute mineral acid, and an equivalent amount of tetanus toxoid and a carbodiimide are added, and the mixture is stirred at room temperature for some hours. The reaction with the toxoid (formulated diagram-matically as HOCO-ttoxoid)~ in the presence of carbodi-imide entails condensation of free carboxyl groups in the toxoid-with free hydrazide groups in the PS-di-j hydrazide conjugate and production of the desired PS-dihydrazidetoxoid conjugate, ~hose structure has not been elucidated but can be imagined to be approximately as shown in the following diagram:
O (CH2)l 6 CO NH NH CO (Toxoid3 The resulting mixture is dialy~ed against a phosphate buffer and chromatographed on an agarose column.
Material with a molecul2r weight of over 350,000, ~hich -` ~L2~7655i~
-- ~ o markedly exceeds the molecular weight of the starting components, is removed and freeze-dried. In the above synthesis it is also possible to replace the tetanus toxoid by diphtheria toxoid.
It is also possible in a manner analogous to that described above to produce vaccines against other Gram-negative bacteria such as, for example, against infections by Escherichia coli.
Determination of the safety and effi_cacy of the conjug-ate vaccines according to the invention Properties_of the Pseudomonas (PS-toxin_A?, (PS-tetanus toxoid) and (PS-diphtheria toxoid) , conjugates accord-ng to the invention:
It is evident from the data in Table 1 (page 12) that the conjugates have a molecular weight greater than 350,0aO and thus far exceed the molecular weight of the starting materials. The covalent bonding of the toxin A
results in this highly toxic agent being detoxified. This entails the lethal dose increasing by at least 1,000-fold~
from 0.2 ~ug~mouse to more than 200 ~g/mouse~ The pyrogeni-city of the conjugates has, compared with that of natural Pseudomonas aeruginosa PA 22~ LPS (0.7 ~g/ml/kg body weight), virtually disappeared.
The conjugates induce specific antibody responses both against the polysaccharide and against the protein carrier, that is to say against toxin A, against tetanus toxin or against diphtheria toxin. The covalent bonding of toxin A to the polysaccharide results in the toxin A
being completely detoxified without thereby losing its immunogenic activity~
It has been possible to demonstrate the ability of (PS-toxin A) conjugate = (PS-toxin A) conjugate vaccine to protect mice against l~thal poisoning ~ith purified toxin A as follows, for example:
Groups of mice recei~ed intramuscular adminis-trations, at the start of the test and on the 14th day of the test, of either 10 ~9 of protein in the form of corresponding amounts of (PS-toxin A) conjugate or a buffer (control group). On the 28th day of the test 7~ 2 ~, gradually increasing doses of toxin A were administered to the mice. The median lethal dose for the control ani-mals was 0.2 ~9, whereas the median lethal dose for the animals pretreated with (PS-toxin A~ conjugate was 4.7 ug/mouse.
Eff;cacy of (PS-tetanus toxoid) conjugate and of (PS-toxin A) conjugate as ~accine .. _ .... _ The ability of natural liPopolysaccharide (LPS
from Pseudomonas aeruginosa)" (PS-tetanus toxoid) con-jugate and of (PS-toxin A) conjugate to protect experi-mental animals against experimentally generated Pseudo-monas aeruginosa sePsis of burns is demonstrated by Table 2~ page 13.
The data demonstrate that the immunization with LPS, (PS-tetanus toxoid) conjugate and with (PS-toxin A) conjugate produces a protective effect of about the same strength against fatal P.a. sepsis. The lethal dose of P. aeruginosa PA Z20 is increased by S0,000-fold, com-pared ~ith the non-immunized control group, by this.
Safety and immunogenicity of (PS-tetanus toxoid) conju-.
gate vaccine in humans Healthy adult volunteers of both sexes and 16 to59 years of age received 1ûO ~9 of the conjugate vaccine in 0.5 ml administered subcutaneously in the upper arm at the start of the test and after 14 days.
All the reastions of the test subjects were re~
corded. Secondary reactions were rare, minor and tran-sient. Venous blood samples were taken at the start of the test and 14 and 28 days after the inoculation. The sera obtained from the blood samples were collected and stored at -20C. The immunoglob~lin G (IgG) antibody titers ~ere determined.
The immunization with tPS-tetanus toxoid) conjugate resulted in a significant rise, compared with the initial titer, in the mean anti-PA 2Z0 LPS IgG titer after 14 and 28 days from the innoculation. See Table 3, page 15.
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Table 2:
Protection against lethal sepsis of burns, caused by Pseudomonas aeruginosa PA 220, by immunization with LPS
of PA 220, (PS-tetanus toxoid) conjugate and with (PS-toxin A) conjugate Immunogen1) LDS~) None (controls) 20 PS-tetanus toxoid conjugate 106 PS-toxin A
conjugate 1û6 1) Mice rece;ved 1 ~9 i.m. before the start of the test and on the 14th day of the test. They ~ere then sub-jected to a burn injury (method: I~A. Holder et al., Infection Immunity 35. 276-Z80 (1982) and on the 28th day were exposed to increasing doses of P.
aeruginosa 220.
2) LD50 = median lethal dose of P. aeruginosa PA 220 calculated by the method of L.J. Reed and H.A.
Muench, American J. Hygiene 27. 493-497 (1938).
'~,V~7~S5 More than 80X of the test subjects reacted with an antibody titer which was increased by four-fold or more.
The immunization ~ith this conjugate vaccine also resul-eed in an anti-tetanus antibody titer neutralizing tetanus toxin.
Serum pools were obtained by combining an eclui-valent amount of serum from each test subject at the start of the test (pre-immun~e pool) and after 28 days (immune pool). The pre-immune pool contained 2.7 international tetanus toxin-neutralizing units per ml, ~hereas the immune pool showed 6.2 units per ml.
Anti-PA Z20 LPS IgG antibodies which were pro-duced by inoculation of humans ~ith the (PS-tetanus toxoid) conjugate according to the invention proved to be highly effective against fatal sepsis caused experimen-tally by P. aeruginosa. Post-immune IgG administered by passive transfer was significantly more effective for preventing deaths than was pre-immune IgG administered by passive transfer. The measured protection correlates j 20 ~ith the anti-PA 220 LPS IgG titer of the IgG prepara-tions. Table 4 see page 16.
Accordingly, (PS-tetanus toxo;d) conjugate is a vaccine ~hich can be used without hazard in humans and produces a significantly raised anti-PA 220 LPS IgG titer ?S in more than 80X of those inoculated. The anti-PA 220 LPS
immunoglobulin raised in humans in this manner proved to be highly effectiYe against fatal P~ aeruginosa sepsis.
Analogous results are also achieved with the P.a. (PS)-toxin A, P~a. ~PS)-diphtheria toxoid, E.c. (PS)-toxin A, E.c. (PS)-tetanus toxo;d ~nd E.c. (PS)-diphtheria toxo;d conjugate vaccines accord-ing to the invention.
(PS-tetanus toxoid)~ (PS-diph.theria toxoid) and (PS-toxin A) conjugate vaccines These conjugates proved, in a large number of tests, to be non-tclxic, non-pyrogenic and highly :1~2765S~, L
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Table 4:
Ability of IgG administered by passive transfer to protect mice against fatal P. aeruginosa PA 220 sepsis of burns.
IgG trans- Anti-LPS LD50 ferred1 ) IgG ELISA t i ter ....
None2~ _ 1.3 x 10 Pre-immune3) 73 1.3 x 103 Post-immune4) 1065 6.7 x 105 1) Each mouse received about 160 lug of human IgG ;n 0.2 ml i.v. 24 hours before exposure to P. aeruginosa PA 220.
2) The controls received 0.2 ml of sterile saline solu-tion.
Muench, American J. Hygiene 27. 493-497 (1938).
'~,V~7~S5 More than 80X of the test subjects reacted with an antibody titer which was increased by four-fold or more.
The immunization ~ith this conjugate vaccine also resul-eed in an anti-tetanus antibody titer neutralizing tetanus toxin.
Serum pools were obtained by combining an eclui-valent amount of serum from each test subject at the start of the test (pre-immun~e pool) and after 28 days (immune pool). The pre-immune pool contained 2.7 international tetanus toxin-neutralizing units per ml, ~hereas the immune pool showed 6.2 units per ml.
Anti-PA Z20 LPS IgG antibodies which were pro-duced by inoculation of humans ~ith the (PS-tetanus toxoid) conjugate according to the invention proved to be highly effective against fatal sepsis caused experimen-tally by P. aeruginosa. Post-immune IgG administered by passive transfer was significantly more effective for preventing deaths than was pre-immune IgG administered by passive transfer. The measured protection correlates j 20 ~ith the anti-PA 220 LPS IgG titer of the IgG prepara-tions. Table 4 see page 16.
Accordingly, (PS-tetanus toxo;d) conjugate is a vaccine ~hich can be used without hazard in humans and produces a significantly raised anti-PA 220 LPS IgG titer ?S in more than 80X of those inoculated. The anti-PA 220 LPS
immunoglobulin raised in humans in this manner proved to be highly effectiYe against fatal P~ aeruginosa sepsis.
Analogous results are also achieved with the P.a. (PS)-toxin A, P~a. ~PS)-diphtheria toxoid, E.c. (PS)-toxin A, E.c. (PS)-tetanus toxo;d ~nd E.c. (PS)-diphtheria toxo;d conjugate vaccines accord-ing to the invention.
(PS-tetanus toxoid)~ (PS-diph.theria toxoid) and (PS-toxin A) conjugate vaccines These conjugates proved, in a large number of tests, to be non-tclxic, non-pyrogenic and highly :1~2765S~, L
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Table 4:
Ability of IgG administered by passive transfer to protect mice against fatal P. aeruginosa PA 220 sepsis of burns.
IgG trans- Anti-LPS LD50 ferred1 ) IgG ELISA t i ter ....
None2~ _ 1.3 x 10 Pre-immune3) 73 1.3 x 103 Post-immune4) 1065 6.7 x 105 1) Each mouse received about 160 lug of human IgG ;n 0.2 ml i.v. 24 hours before exposure to P. aeruginosa PA 220.
2) The controls received 0.2 ml of sterile saline solu-tion.
3) Prepared from aliquots of the sera from all the volunteer test subjects before the immuni~ation.
4) Prepared from aliquots of the sera from all volun- -teers 28 days after the immunization.
1~765~;~
e~fective vaccines. No vaccines of these types have hitherto been disclosed. For practical use, it is desirab(e to be able to o~fer a vaccine which displays a ~ide-ranging effect against infections by various serotypes of, for example, Pseudomonas aeruginosa. I~
has been found that this ~ide-ranging effect can be achieved when use is made of a composition of (PS-tetanus toxoid), (PS-diphtheria toxoid) or (PS-toxin A) conjugates whose PS (polysaccharide) part originates from several serotypes of Pseudomonas aeruginosa (P.a.) which principally occur in infections. For this pur-pose about 3 to 15 different serotypes of Pseudomonas aeruginosa are necessary.
The linkage of the polysaccharides (PS) of the various serotypes to give the PS-protein conjugate must take place individually in order to obtain utilizable preparations. This means that the individual LPS are isolated from each of 3 to 15 pure strains of P.a., and from these the PS and the individual PS are individu-ally linked covalentLy with the protein part ttoxin A,tetanus toxoid or diphtheria toxoid), the resulting conjugates are tested for their tolerability and effi-cacy and, finally, the 3 to 15 individual conjugates are mixed together ~o give the final combination pre ?5 paration.
The same procedure is also used for the prepar-ation of a combination vaccine against infections by other Gram-negative bacteria such as, for example, Escherichia coli.
Vaccines which_are effective against infections by various species of Gram-negative bacteria It ~ould be very desirable to be able to raise antibodies against a variety of species of Gram-negative bacteria by a single inoculation. This would be especially important where the antibodies are to be harvested and processed to give immunoglobulins speci-fically effective against infection by 6ram-negative bacteria. It has been found that this object can be achieved uhen the specific conjugate vaccine against a ~L2'765~
species of bacteria is mixed wieh one or more specific conjugate vaccines against other species of bacteria.
Use ot coniuqate vaccines according_to the pre-sent invention for_the preparation of soecific immunoglobulins lt has been demonstrated above that the conjug-ate vaccine5 according to the invention bring about the formation of spec;fic antiboclies against the relevant species of bacteria in humans. The antibody titer pro-duced in this manner in the serum of the inoculated volunteers is so high that these sera can be used as starting materials for the preparation of specific immunoglobulins. Hence, the physician has in his hands an agent with which he can successfully treat, and save the life of, non-inoculated patients suffering from a corresponding bacteremia.
Examples Example 1 Pseudomonas aeruginosa vaccine: PS-toxin A conjugate A. Isolation of the LPS (IT-5 = Habs 10) 500 ml of 3~ trypticase soy broth (TSB) (Becton, Dickinson and Company, USA) containing 1% glycerol are inoculated with a free~e-dried culture of Pseudomonas aeruginosa (IT-5 = Habs 10) and incubated at 37C and 150 rpm. 50 lt of 3% TS~ medium containing 1X glycerol are inocu~ated ~ith this preculture and incubated in a fermenter at 37C for 16 hours. The cells are har-vested using a continuous-flo~ centrifuge (for example from ~estfalia) and washed triçe with tris/NaCl buffer pH 9. The cells are then suspended in tris/NaCl buffer pH 9 and mechanically disrupted, for example using glass beads (Dyno-Mill, ~.A. 8achhofer AG, ~asel~ Switzerland).
The cells walLs are removed from the cytoplasm, which is discarded, by centrifugation. The cell walls are sus-pended once more in tris/NaCl buffer and sedimentedusing a refrigerated centrifuge ~t 23,500 9 for 30 min.
The cell ~alls are then suspended in 1,000 ml of water, and 128Q ml of 80% phenol are added. Method~ estphal, Z. Naturforsch. 7: 148-155. The mixture is heated ~o * Trade Mark ~ ~7655~
_ ~8-70C and stirred at this tem-perature for 5 min. The extract;on mixture is then coo~ed to 4-10C in an ice bath and subsequently centrituged in a refrigerated centrifuge at 23,500 9 for 15 min to separate the phases. The upper S phase corresponds to the aqueous phase and contains the - lipopoly-saccharides tLPS)= It is carefully removed from the phenol phase, to wh;ch a further 1 liter o~ distilled ~ater is added, and the mixture is once more stirred at 68-70C for 5 min. It is again cooled to 4-10C in an ice bath, and the phases are separated as above. The a~ueous phases are combined and dialyzed against water until they are free of water. The phenol phases are discarded. The aqueous phases are then centrifuged in an ultracentrifuge at 100,00û 9 for three hours to sediment the LPS. The sediment is dissolved in 0.05 m tris buf-fer, p~ 7.2, containing O.OS M NaCl, and is treated with RNAse, DNAse and pronase (9Oehringer, Mannheim, West Germany) as follows. RNAse is added to a final concen-tration of 20 ~g/ml, and the mixture is incubated at 37C
for three hours. Then DNAse is added to a final concen-tration of 20 ~g/ml, and MgS04 is added to a final concen-trat;on of 0.1 M, and the mixture is again incubated at 37C for three hours. Subsequently pronase is added to a concentration of 200 ~ug/ml, and the mixture is incu-bated at 37C for 2-3 hours and subsequently dialyzed agains~ ~ater at 4C overnight. The LPS are further purified by ultracentrifugation t~ice and subsequently freeze-dried. The LPS thus purified contain less than 1Z nucleic acids and protein as contaminant.
~. Isolation of the serotype-sPecific polysaccharide The purified LPS are suspended at a concentration of 3 mg/ml of 1~ acetic acid and hydrolyzed at 100C for 90 min. Method: G. Schmidt et al., Eur. J~
~iochem. 10: 501-510 (1969). With this treatment the Polysaccharide part is separated from the toxic lipid part (lipid A). Lipid A is insolubLe and is removed from the solubLe polysaccharide by centrifugation. The aqueous polysaccharide solution is extracted three times uith the same volume of chloroform/methanol (3:1) to .... .
lZ~765~'~
remove traces of lipid A~ and is concentrated under wa~er ; pump vacuum. The concentrated PS solution is chromato-graphed on an zgarose gel, for example ACA 3~ gel (LK~-irodukter A~ ~romma, Sweden). (Column 5 cm x 40 c~, flo~ rate 1.7 ml/min, fraction size 17 ml.) Poly-saccharide i3 determined in the ind;vidual fract;ons.
The fractions ~h;ch contain the PS with a molecular ~eight of 1û,000 to 75,000 are pooled and freeze-dried.
; C. Oxidat;on of the PS
j 10 The freeze-dried PS are dissolved in distilled water in a concentration of 5 mg/ml. To this is added NaI04 (sodium periodate) to a concentration of 0.1 M. The solution is left to stand in the dark at room tempera-ture for two hours. E~cess oxidizing agent is inactivated by addition of ethylene glycol to a concen-tration of 0.2 M. The oxidized PS are exhaustively dialyzed against water and free~e-dried.
D. Toxin A
Toxin A is isolated from the suPernatant of P.
¦ 20 aeruginosa strain PA 103 tobtained from Dr. ~. Wret-¦ lind, Karolinska Institute, Stockholm, Sweden) by the j follobing kno~n method: ultrafiltration, DEAE-cellulose chromatography, hydroxyapatite chromatography (des-cribed by Cryz _ al. in Infect. Immun. 39: 1072-1079~
1983). The purity of the toxin A thus isolated is more than 95%.
E. Preparation of toxin A-ADH (ADH = adipic acid di-= . . .. _ . .. .. ___ ..
hydrazide) As a "spacer" molecule and for the introduction of reactive amino groups, ADH is covalently linked withtoxin A as follows: pure toxin h is adjusted to S mg/ml in 0.05 N Na phosphate buffer, pH 7.2. To this are added ADH (adipic acid dihydra2ide) and 1-ethyl~3-(3-dimethylaminopropyl)carbodiimide in the solid form to a concentration of 10 m~/ml each. The pH is adjusted to 4.8 with dilute hydrochloric acid. The solution is cautiously stirred at 22C for two hours, and the pH is maintained constant at 4.8 by addition of further 1N hydrochloric acid. After the reaction is ~ ~76~5~
complete, the mixture is exhaustively dialyzed against O.OS M Na phosphate buffer pH 8.0 at 4C. Insoluble mater;ol is removed by centrifugation. The to~in A-ADH
solution is adjusted to a concentration of S mg/ml.
F. Preparation of polysaccharide-toxin A conjugate The tox;n A-ADH solution is dialyzed against 0.5 M
Na phosphate buffer at room temperature for t~o hours, and the to~in A-ADH solution is adjusted to 5 mg/ml.
To this solution is added an equal volume of a solution of 5 mg/ml oxidized PS, likewise dissolved in 0.5 M Na phosphate buffer pH 8Ø The solution is left to stand at room temperature for six hours~ and then Na~H3CN
from a ten-fold concentrated (0.5 M) solueion is added to a concentration of 0.05 M. The mixture is then left to stand at room temperature for 5-7 days~ It is sub-seque~tly exhaustively dialyzed against phosphate buffer ~PBS) of pH 7.4, containing O.û2% Merthiolate.
Insoluble material is removed by centrifugation, and the dissolved reaction mixture is chromatographed on an agarose gel, for example AcA 34 gel. The absûrption of I the fractions at 280 and 220 nm is measured. Material ! uhich is eluted ~ith the bed volume (vo), and accord-ingly has a molecular ~eight above 350,000, ~hich is far above the molecular weights of the reactants, is collected and sterilized by filtration. The material is diluted so that 0.5 ml corresponds to a dose for humans, and so that the final solution contains 5% lac-~ tose in 50% strength PBS and Q.01Z Merthiolate, and ;s ! then freeze-dried.
'~ 30 The following tests are carried out with the vaccine:
12~76~iS~
.
Test Method Polysaccharide content Phenol/sulfuric acid1 using pure starting PS as stan-dard.
1~765~;~
e~fective vaccines. No vaccines of these types have hitherto been disclosed. For practical use, it is desirab(e to be able to o~fer a vaccine which displays a ~ide-ranging effect against infections by various serotypes of, for example, Pseudomonas aeruginosa. I~
has been found that this ~ide-ranging effect can be achieved when use is made of a composition of (PS-tetanus toxoid), (PS-diphtheria toxoid) or (PS-toxin A) conjugates whose PS (polysaccharide) part originates from several serotypes of Pseudomonas aeruginosa (P.a.) which principally occur in infections. For this pur-pose about 3 to 15 different serotypes of Pseudomonas aeruginosa are necessary.
The linkage of the polysaccharides (PS) of the various serotypes to give the PS-protein conjugate must take place individually in order to obtain utilizable preparations. This means that the individual LPS are isolated from each of 3 to 15 pure strains of P.a., and from these the PS and the individual PS are individu-ally linked covalentLy with the protein part ttoxin A,tetanus toxoid or diphtheria toxoid), the resulting conjugates are tested for their tolerability and effi-cacy and, finally, the 3 to 15 individual conjugates are mixed together ~o give the final combination pre ?5 paration.
The same procedure is also used for the prepar-ation of a combination vaccine against infections by other Gram-negative bacteria such as, for example, Escherichia coli.
Vaccines which_are effective against infections by various species of Gram-negative bacteria It ~ould be very desirable to be able to raise antibodies against a variety of species of Gram-negative bacteria by a single inoculation. This would be especially important where the antibodies are to be harvested and processed to give immunoglobulins speci-fically effective against infection by 6ram-negative bacteria. It has been found that this object can be achieved uhen the specific conjugate vaccine against a ~L2'765~
species of bacteria is mixed wieh one or more specific conjugate vaccines against other species of bacteria.
Use ot coniuqate vaccines according_to the pre-sent invention for_the preparation of soecific immunoglobulins lt has been demonstrated above that the conjug-ate vaccine5 according to the invention bring about the formation of spec;fic antiboclies against the relevant species of bacteria in humans. The antibody titer pro-duced in this manner in the serum of the inoculated volunteers is so high that these sera can be used as starting materials for the preparation of specific immunoglobulins. Hence, the physician has in his hands an agent with which he can successfully treat, and save the life of, non-inoculated patients suffering from a corresponding bacteremia.
Examples Example 1 Pseudomonas aeruginosa vaccine: PS-toxin A conjugate A. Isolation of the LPS (IT-5 = Habs 10) 500 ml of 3~ trypticase soy broth (TSB) (Becton, Dickinson and Company, USA) containing 1% glycerol are inoculated with a free~e-dried culture of Pseudomonas aeruginosa (IT-5 = Habs 10) and incubated at 37C and 150 rpm. 50 lt of 3% TS~ medium containing 1X glycerol are inocu~ated ~ith this preculture and incubated in a fermenter at 37C for 16 hours. The cells are har-vested using a continuous-flo~ centrifuge (for example from ~estfalia) and washed triçe with tris/NaCl buffer pH 9. The cells are then suspended in tris/NaCl buffer pH 9 and mechanically disrupted, for example using glass beads (Dyno-Mill, ~.A. 8achhofer AG, ~asel~ Switzerland).
The cells walLs are removed from the cytoplasm, which is discarded, by centrifugation. The cell walls are sus-pended once more in tris/NaCl buffer and sedimentedusing a refrigerated centrifuge ~t 23,500 9 for 30 min.
The cell ~alls are then suspended in 1,000 ml of water, and 128Q ml of 80% phenol are added. Method~ estphal, Z. Naturforsch. 7: 148-155. The mixture is heated ~o * Trade Mark ~ ~7655~
_ ~8-70C and stirred at this tem-perature for 5 min. The extract;on mixture is then coo~ed to 4-10C in an ice bath and subsequently centrituged in a refrigerated centrifuge at 23,500 9 for 15 min to separate the phases. The upper S phase corresponds to the aqueous phase and contains the - lipopoly-saccharides tLPS)= It is carefully removed from the phenol phase, to wh;ch a further 1 liter o~ distilled ~ater is added, and the mixture is once more stirred at 68-70C for 5 min. It is again cooled to 4-10C in an ice bath, and the phases are separated as above. The a~ueous phases are combined and dialyzed against water until they are free of water. The phenol phases are discarded. The aqueous phases are then centrifuged in an ultracentrifuge at 100,00û 9 for three hours to sediment the LPS. The sediment is dissolved in 0.05 m tris buf-fer, p~ 7.2, containing O.OS M NaCl, and is treated with RNAse, DNAse and pronase (9Oehringer, Mannheim, West Germany) as follows. RNAse is added to a final concen-tration of 20 ~g/ml, and the mixture is incubated at 37C
for three hours. Then DNAse is added to a final concen-tration of 20 ~g/ml, and MgS04 is added to a final concen-trat;on of 0.1 M, and the mixture is again incubated at 37C for three hours. Subsequently pronase is added to a concentration of 200 ~ug/ml, and the mixture is incu-bated at 37C for 2-3 hours and subsequently dialyzed agains~ ~ater at 4C overnight. The LPS are further purified by ultracentrifugation t~ice and subsequently freeze-dried. The LPS thus purified contain less than 1Z nucleic acids and protein as contaminant.
~. Isolation of the serotype-sPecific polysaccharide The purified LPS are suspended at a concentration of 3 mg/ml of 1~ acetic acid and hydrolyzed at 100C for 90 min. Method: G. Schmidt et al., Eur. J~
~iochem. 10: 501-510 (1969). With this treatment the Polysaccharide part is separated from the toxic lipid part (lipid A). Lipid A is insolubLe and is removed from the solubLe polysaccharide by centrifugation. The aqueous polysaccharide solution is extracted three times uith the same volume of chloroform/methanol (3:1) to .... .
lZ~765~'~
remove traces of lipid A~ and is concentrated under wa~er ; pump vacuum. The concentrated PS solution is chromato-graphed on an zgarose gel, for example ACA 3~ gel (LK~-irodukter A~ ~romma, Sweden). (Column 5 cm x 40 c~, flo~ rate 1.7 ml/min, fraction size 17 ml.) Poly-saccharide i3 determined in the ind;vidual fract;ons.
The fractions ~h;ch contain the PS with a molecular ~eight of 1û,000 to 75,000 are pooled and freeze-dried.
; C. Oxidat;on of the PS
j 10 The freeze-dried PS are dissolved in distilled water in a concentration of 5 mg/ml. To this is added NaI04 (sodium periodate) to a concentration of 0.1 M. The solution is left to stand in the dark at room tempera-ture for two hours. E~cess oxidizing agent is inactivated by addition of ethylene glycol to a concen-tration of 0.2 M. The oxidized PS are exhaustively dialyzed against water and free~e-dried.
D. Toxin A
Toxin A is isolated from the suPernatant of P.
¦ 20 aeruginosa strain PA 103 tobtained from Dr. ~. Wret-¦ lind, Karolinska Institute, Stockholm, Sweden) by the j follobing kno~n method: ultrafiltration, DEAE-cellulose chromatography, hydroxyapatite chromatography (des-cribed by Cryz _ al. in Infect. Immun. 39: 1072-1079~
1983). The purity of the toxin A thus isolated is more than 95%.
E. Preparation of toxin A-ADH (ADH = adipic acid di-= . . .. _ . .. .. ___ ..
hydrazide) As a "spacer" molecule and for the introduction of reactive amino groups, ADH is covalently linked withtoxin A as follows: pure toxin h is adjusted to S mg/ml in 0.05 N Na phosphate buffer, pH 7.2. To this are added ADH (adipic acid dihydra2ide) and 1-ethyl~3-(3-dimethylaminopropyl)carbodiimide in the solid form to a concentration of 10 m~/ml each. The pH is adjusted to 4.8 with dilute hydrochloric acid. The solution is cautiously stirred at 22C for two hours, and the pH is maintained constant at 4.8 by addition of further 1N hydrochloric acid. After the reaction is ~ ~76~5~
complete, the mixture is exhaustively dialyzed against O.OS M Na phosphate buffer pH 8.0 at 4C. Insoluble mater;ol is removed by centrifugation. The to~in A-ADH
solution is adjusted to a concentration of S mg/ml.
F. Preparation of polysaccharide-toxin A conjugate The tox;n A-ADH solution is dialyzed against 0.5 M
Na phosphate buffer at room temperature for t~o hours, and the to~in A-ADH solution is adjusted to 5 mg/ml.
To this solution is added an equal volume of a solution of 5 mg/ml oxidized PS, likewise dissolved in 0.5 M Na phosphate buffer pH 8Ø The solution is left to stand at room temperature for six hours~ and then Na~H3CN
from a ten-fold concentrated (0.5 M) solueion is added to a concentration of 0.05 M. The mixture is then left to stand at room temperature for 5-7 days~ It is sub-seque~tly exhaustively dialyzed against phosphate buffer ~PBS) of pH 7.4, containing O.û2% Merthiolate.
Insoluble material is removed by centrifugation, and the dissolved reaction mixture is chromatographed on an agarose gel, for example AcA 34 gel. The absûrption of I the fractions at 280 and 220 nm is measured. Material ! uhich is eluted ~ith the bed volume (vo), and accord-ingly has a molecular ~eight above 350,000, ~hich is far above the molecular weights of the reactants, is collected and sterilized by filtration. The material is diluted so that 0.5 ml corresponds to a dose for humans, and so that the final solution contains 5% lac-~ tose in 50% strength PBS and Q.01Z Merthiolate, and ;s ! then freeze-dried.
'~ 30 The following tests are carried out with the vaccine:
12~76~iS~
.
Test Method Polysaccharide content Phenol/sulfuric acid1 using pure starting PS as stan-dard.
5 Protein content Lo~ry et al.Z using bovine serum albumin as standard.
Sterility Pyrogenicity Rabbits Tolerabili~y Two human doses intraperi-i 10 toneally to each of two guinea pigs, and one human dose to each of five mice.
Toxicity 20û ~9 (protein) 1n 0.5 ml intraperitoneally in six mice.
For re~ults, see Table 1.
1) M. Dubois et al. Colorimetric method for determin-- ation of sugars and related substances. Anal. Chem.
28: 350-356.
20 2) O.H. Lowry et al. Protein measurement ~ith the Folin-phenol reagent. J. ~iol. Chem. 193: 265-275 (1951).
Example 2 Pseudomonas aeruginosa vaccine. PS-tetanus toxoid con-25 iuqate 10û mg of PS~ prepared as in Example 1A/~, are dissolved in 9.2 ml of distilled water. To this is cautiously added û.44 ml of a solution of cyanogen bromide. The pH
is ma;ntainecd at pH 10.5 for 6 min. using 1 H NaOH. The 3û pH is then reduced to 8.6 by addition of solid NaHC03.
0.4 9 of adipic acid dihydra~ide (ADH) is added~ and the sOlue;on is left at 4~C for 16 hours, stirring cautiously.
~ After exhaustive dialysis against ~ater, 100 mg of con-J centrated or free~e-dried tetanus toxoid ~hich has been 35 pur;fied by, for example, ion exchanger and gel chromato-graphy, and 3.3 ml of 1-ethyl-3~-3-dimethylaminoproPYl)-1,~ 7~iSrj2 carbodiimide solution (20 mg/ml) are added. Th2 pH is adjusted to 4.8 with 0.1 N hydrochloric acid, and is - maintained constant at room temperature for 4 hours, stirring gently. The reaction mixture is then exhaus-tively dialyzed against PBS/Merthiolate 0.02X. There-after the mixture is chromatographed on an agarose gel (column 5 cm ~ ~0 cm, flow rate 1.1 ml per minute) using PBS/Merthiolate buffer. 11 ml fractions are col-lected, and the contents of protein and PS are deter-mined. Material which has eluted with the bed ~olume,and accordingly has a molecular weight above 350,000, is pooled and freeze-dried as in Example 1. PS-tetanus conjugate is tested in analogy to the PS-toxin A con-jugate (see Example 1).
Example 3 Pseudomonas aeruginosa vaccine: PS-diphtheria toxoid coniugate _ The polysaccharide which contains the serotyPe-sPecific determinants is covalently bonded to a purified Z0 and concentrated or freeze-dried diphtheria toxoid as described in Example 2.
The resulting vaccine is non-toxic and raises serotype-specific antibodies against Pseudomonas aeru-ginosa and antitoxic antibodies against diphtheria toxoid.
Example 4 Escherichia coli PS-toxin A conjugate vac_cine The polysaccharide which contains the serotype-specific determinants is isolated from the endotoxin from E. coli fermenter cultures in a manner analogous to -that described in Example 1. The polysaccharide is oxidized with Na periodate and covalently bonded to toxin A using the "spacer" molecule adipic acid dihyd-razide, as described in Example 1. The conjugate vaccine is freeze-dried and tested. I~ is non-toxic, ~ell ~olerated and induces the formation of serotype-specific antibodies against E. coli.
~276S~
Example 5 Escherichia coli - PS-tetanus toxoid conjugate vaccine coli polysaccharide cont~ining the serotype-specific determinants is activated with cyanogen bromide and covalently bonded, in analogy to Example 2~ with the spacer molecule adipic acid dihydra2ide (ADH). The polysaccharide-ADH is covalently bonded to the carboxyl groups of the tetanus toxoid using a ~ater-soluble carbodiimide.
The resulting vaccine is non-to~ic, well toler-ated and induces the formation of serotype-specific antibodies against E. coli and of antitoxic antibodies against tetanus toxoid.
Examples 6-8 Polyvalent Pseudomonas aeruginosa coniugate vaccines 6. 9-valent P. aeruginosa-P.a. toxin A vaccine 50-100 ~ug of each of nine serotype-sPecific indivi-dual conjugates per dose are combined by mixing to give the polyvalent Pseudomonæs aeruginosa conjugate vac-cine.
Procedure: the polysaccharide components of the conjugates are first isolated individually from ehe endotoxin of the follo~ing 9 Pseudomonas aeruginosa stra;ns:
25 PA 220 (Habs serotype 6d~; 8505 (Habs serotype 3);
~511 tHabs serotype 4), IT-2 (Habs serotype 11);
E 576 ~Habs serotype 2ab); PA 53 (Habs serotype 1);
18 (Habs serotyPe 10~; IT 2 (Habs serotype 11);
IT 6 (Habs serotype 8). (sic) The 9 different PS are then individually co-valently linked as in Example 1 with the prot~in part of exotoxin A of Pseudomonas aeruginosa, and the 9 conju-gates are final~y mixed to give the 9-valent vaccine.
The resulting 9-valent vaccine has the fol-lowing properties:
1) It is non-toxic for animals and non-pyrogenic for rabbits.
2) Its molecular weight is greater than 350,000.
3) The vaccine protects against a ~ide spectrum of ~'~765~;2 P. aeruginosa infections.
Sterility Pyrogenicity Rabbits Tolerabili~y Two human doses intraperi-i 10 toneally to each of two guinea pigs, and one human dose to each of five mice.
Toxicity 20û ~9 (protein) 1n 0.5 ml intraperitoneally in six mice.
For re~ults, see Table 1.
1) M. Dubois et al. Colorimetric method for determin-- ation of sugars and related substances. Anal. Chem.
28: 350-356.
20 2) O.H. Lowry et al. Protein measurement ~ith the Folin-phenol reagent. J. ~iol. Chem. 193: 265-275 (1951).
Example 2 Pseudomonas aeruginosa vaccine. PS-tetanus toxoid con-25 iuqate 10û mg of PS~ prepared as in Example 1A/~, are dissolved in 9.2 ml of distilled water. To this is cautiously added û.44 ml of a solution of cyanogen bromide. The pH
is ma;ntainecd at pH 10.5 for 6 min. using 1 H NaOH. The 3û pH is then reduced to 8.6 by addition of solid NaHC03.
0.4 9 of adipic acid dihydra~ide (ADH) is added~ and the sOlue;on is left at 4~C for 16 hours, stirring cautiously.
~ After exhaustive dialysis against ~ater, 100 mg of con-J centrated or free~e-dried tetanus toxoid ~hich has been 35 pur;fied by, for example, ion exchanger and gel chromato-graphy, and 3.3 ml of 1-ethyl-3~-3-dimethylaminoproPYl)-1,~ 7~iSrj2 carbodiimide solution (20 mg/ml) are added. Th2 pH is adjusted to 4.8 with 0.1 N hydrochloric acid, and is - maintained constant at room temperature for 4 hours, stirring gently. The reaction mixture is then exhaus-tively dialyzed against PBS/Merthiolate 0.02X. There-after the mixture is chromatographed on an agarose gel (column 5 cm ~ ~0 cm, flow rate 1.1 ml per minute) using PBS/Merthiolate buffer. 11 ml fractions are col-lected, and the contents of protein and PS are deter-mined. Material which has eluted with the bed ~olume,and accordingly has a molecular weight above 350,000, is pooled and freeze-dried as in Example 1. PS-tetanus conjugate is tested in analogy to the PS-toxin A con-jugate (see Example 1).
Example 3 Pseudomonas aeruginosa vaccine: PS-diphtheria toxoid coniugate _ The polysaccharide which contains the serotyPe-sPecific determinants is covalently bonded to a purified Z0 and concentrated or freeze-dried diphtheria toxoid as described in Example 2.
The resulting vaccine is non-toxic and raises serotype-specific antibodies against Pseudomonas aeru-ginosa and antitoxic antibodies against diphtheria toxoid.
Example 4 Escherichia coli PS-toxin A conjugate vac_cine The polysaccharide which contains the serotype-specific determinants is isolated from the endotoxin from E. coli fermenter cultures in a manner analogous to -that described in Example 1. The polysaccharide is oxidized with Na periodate and covalently bonded to toxin A using the "spacer" molecule adipic acid dihyd-razide, as described in Example 1. The conjugate vaccine is freeze-dried and tested. I~ is non-toxic, ~ell ~olerated and induces the formation of serotype-specific antibodies against E. coli.
~276S~
Example 5 Escherichia coli - PS-tetanus toxoid conjugate vaccine coli polysaccharide cont~ining the serotype-specific determinants is activated with cyanogen bromide and covalently bonded, in analogy to Example 2~ with the spacer molecule adipic acid dihydra2ide (ADH). The polysaccharide-ADH is covalently bonded to the carboxyl groups of the tetanus toxoid using a ~ater-soluble carbodiimide.
The resulting vaccine is non-to~ic, well toler-ated and induces the formation of serotype-specific antibodies against E. coli and of antitoxic antibodies against tetanus toxoid.
Examples 6-8 Polyvalent Pseudomonas aeruginosa coniugate vaccines 6. 9-valent P. aeruginosa-P.a. toxin A vaccine 50-100 ~ug of each of nine serotype-sPecific indivi-dual conjugates per dose are combined by mixing to give the polyvalent Pseudomonæs aeruginosa conjugate vac-cine.
Procedure: the polysaccharide components of the conjugates are first isolated individually from ehe endotoxin of the follo~ing 9 Pseudomonas aeruginosa stra;ns:
25 PA 220 (Habs serotype 6d~; 8505 (Habs serotype 3);
~511 tHabs serotype 4), IT-2 (Habs serotype 11);
E 576 ~Habs serotype 2ab); PA 53 (Habs serotype 1);
18 (Habs serotyPe 10~; IT 2 (Habs serotype 11);
IT 6 (Habs serotype 8). (sic) The 9 different PS are then individually co-valently linked as in Example 1 with the prot~in part of exotoxin A of Pseudomonas aeruginosa, and the 9 conju-gates are final~y mixed to give the 9-valent vaccine.
The resulting 9-valent vaccine has the fol-lowing properties:
1) It is non-toxic for animals and non-pyrogenic for rabbits.
2) Its molecular weight is greater than 350,000.
3) The vaccine protects against a ~ide spectrum of ~'~765~;2 P. aeruginosa infections.
7. 9-valent PO aeru~inosa-tetanus toxoid vaccine The preparation is carried out in analogy to Example 6.
The nine different PS are individually covalently linked to human tetanus toxo;d as in Example 2, and are then mixed to give the Polyvalent vaccine.
The resulting vaccine induces the formation of serotype-specific antibodies against P. aeruginosa and of antitoxic antibodies against te~anus toxin.
The nine different PS are individually covalently linked to human tetanus toxo;d as in Example 2, and are then mixed to give the Polyvalent vaccine.
The resulting vaccine induces the formation of serotype-specific antibodies against P. aeruginosa and of antitoxic antibodies against te~anus toxin.
8. Nine-valent P. aeruginosa-diphtheria toxoid vacrine . _ .
The 9 PS specified in Example 6 are individually covalently linked to diphtheria toxoid as in Example 3, and are then mixed to give the polyvalent vaccine.
The resulting vaccine induces the formation of serotype-specific antibodies against P. aeruginosa and of antitoxic antibodies against diphtheria toxin.
Example~ 9-13.
Polyvalent Escherichia coli conjugate vaccines 9. 14-valent E. coli-P.a. toxin vaccine .
50-100 ~9 of each of 14 individual conjugates ~hose polysaccharide part originates from the endotoxin of sero-types 1, 2, 4, 6, 7, 8, 11, 16, 18, 22, 25, 62 and 75 of E. coli and whose protein part originates from exo-to~in A of Pseudomonas aeruginosa (P.a.) are mixed.
The resulting vaccine induces the formation of serotype-specific antibodies against Escherichia coli and of antitoxic antiboclies against P~a. toxin.
The 9 PS specified in Example 6 are individually covalently linked to diphtheria toxoid as in Example 3, and are then mixed to give the polyvalent vaccine.
The resulting vaccine induces the formation of serotype-specific antibodies against P. aeruginosa and of antitoxic antibodies against diphtheria toxin.
Example~ 9-13.
Polyvalent Escherichia coli conjugate vaccines 9. 14-valent E. coli-P.a. toxin vaccine .
50-100 ~9 of each of 14 individual conjugates ~hose polysaccharide part originates from the endotoxin of sero-types 1, 2, 4, 6, 7, 8, 11, 16, 18, 22, 25, 62 and 75 of E. coli and whose protein part originates from exo-to~in A of Pseudomonas aeruginosa (P.a.) are mixed.
The resulting vaccine induces the formation of serotype-specific antibodies against Escherichia coli and of antitoxic antiboclies against P~a. toxin.
10. 14-valen~ E. coli-tetanus toxoid vaccine _ . ~
14 individual conjugates of the PS of E. coli men-~ioned in EKample 9 and human tetanus toxoid are pre-pared in analogy to Examples 1-3 and mixed in analogy to Examples 6/7~ The resuleing vaccine induces the formation of specific antibodies against E. coli and antitoxic antibodies against tetanus toxin.
14 individual conjugates of the PS of E. coli men-~ioned in EKample 9 and human tetanus toxoid are pre-pared in analogy to Examples 1-3 and mixed in analogy to Examples 6/7~ The resuleing vaccine induces the formation of specific antibodies against E. coli and antitoxic antibodies against tetanus toxin.
11. 14-valen~ E. coli-d;phtheria toxoid conjugat_ vaccine 14 individual conjugates of the PS of E. coli men-tioned in Example !~ and diphtheria toxoid are ~L~76~Z
prepared in analogy to Examples 1-3 and mixed in analogy to Examples 6/7. The resulting vaccine induces the formation of specific antibodies against E. coli and antitoxic antibodies against diphtheria toxin.
prepared in analogy to Examples 1-3 and mixed in analogy to Examples 6/7. The resulting vaccine induces the formation of specific antibodies against E. coli and antitoxic antibodies against diphtheria toxin.
12. 10-va(ent E. coli coniuga~e vaccine For each dose, 50-100 ~9 of each of 10 individual conjugates whose polysaccharide part originates from the endotoxin of 0-serotypes 1, 2, 4, 6~ 7, 8, 18, 22, 25 and 75 and whose protein part originates from exotoxin A of P. aeruginosa or from a human tetanus toxoid are .
mixed.
mixed.
13 3-valent E. coli coniugate vaccine For each dose, 50-100 ~9 o~ each of 3 individual conjugates whose polysaccharide part originates from the endotoxin of 0-serotypes a) 1, b) 2 and c) 4 and whose protein part originates a) from exotoxin A of P.
aeruginosa, b) from human tetanus toxoid and c) from diphtheria toxoid, respectively, are mixed.
Example 14 Polyvalent con]ugate vac _ne against infections by P.
aeruginosa and E. col i ~ . ~
This vaccine is obtained by mixing 9 individual con-jugates (50-100 ~9) whose polysaccharide part originates from Pseudomonas aeruginosa endotoxin, and 14 individual conjugates whose polysaccharide part originates from the endotoxin of E. coli. The protein part of the individual conjugates originates in each case either from exotox;n A
of P. aeruqinssa or from a human tetanus toxoid. The resulting vaccine is able to induce serotyPe-specific antibodies against P. aeruginosa and against E. coli.
Furthermore, this vaccine also induces antitoxic anti-bodies directed against exotoxin A and against tetanus toxin.
Example 15 Use of the polyvalent conjugate vaccine_for the prepar-, ~ .
ation of specific immunoglobulin _ _ _ Volunteers zlre immunized in the deltoid muscle with thepolyvalent vaccine accordlng to Example 14. Four weeks thereafter a booster inoculation ~ith the same vaccine ~27~i552 and dosage is administered in the deltoid muscle. One ~eek later a blood sample is taken from a brachial vein of the volunteers, and the titers of antibodies against the serotypes contained in the vaccine (of P. aeruginosa and E. coli) and against exotoxin A and tetanus toxin -are determined. If the increase in the titer against all the said antigens is 4 times or more as a result of the inoculations, then those inoculated donate about 240 ml of blood. The sera are pooled, and a gamma-globulin preparation for intravenous administration(IYIG) is prepared by the following known steps, for example by the process of European Patent Application 85,747: fractionated alcohol precipitation by the Cohn method, ion exchange chromatography, ultrafiltration ~5 and diafiltration. The protein content is adjusted to 5%, and freeze-drying is carried out in a stabilizing medium.
aeruginosa, b) from human tetanus toxoid and c) from diphtheria toxoid, respectively, are mixed.
Example 14 Polyvalent con]ugate vac _ne against infections by P.
aeruginosa and E. col i ~ . ~
This vaccine is obtained by mixing 9 individual con-jugates (50-100 ~9) whose polysaccharide part originates from Pseudomonas aeruginosa endotoxin, and 14 individual conjugates whose polysaccharide part originates from the endotoxin of E. coli. The protein part of the individual conjugates originates in each case either from exotox;n A
of P. aeruqinssa or from a human tetanus toxoid. The resulting vaccine is able to induce serotyPe-specific antibodies against P. aeruginosa and against E. coli.
Furthermore, this vaccine also induces antitoxic anti-bodies directed against exotoxin A and against tetanus toxin.
Example 15 Use of the polyvalent conjugate vaccine_for the prepar-, ~ .
ation of specific immunoglobulin _ _ _ Volunteers zlre immunized in the deltoid muscle with thepolyvalent vaccine accordlng to Example 14. Four weeks thereafter a booster inoculation ~ith the same vaccine ~27~i552 and dosage is administered in the deltoid muscle. One ~eek later a blood sample is taken from a brachial vein of the volunteers, and the titers of antibodies against the serotypes contained in the vaccine (of P. aeruginosa and E. coli) and against exotoxin A and tetanus toxin -are determined. If the increase in the titer against all the said antigens is 4 times or more as a result of the inoculations, then those inoculated donate about 240 ml of blood. The sera are pooled, and a gamma-globulin preparation for intravenous administration(IYIG) is prepared by the following known steps, for example by the process of European Patent Application 85,747: fractionated alcohol precipitation by the Cohn method, ion exchange chromatography, ultrafiltration ~5 and diafiltration. The protein content is adjusted to 5%, and freeze-drying is carried out in a stabilizing medium.
Claims (21)
1. A non-toxic conjugate vaccine against infections by Gram-negative bacteria comprising a species-specific polysaccharide and a protein which are covalently linked together wherein the polysaccharide originates from endotoxin of the bacteria and the protein is an exoprotein.
2. A conjugate vaccines as claimed in claim 1, wherein the Gram-negative bacterium is Pseudomonas aeruginosa.
3. A conjugate vaccine as claimed in claim 1, wherein the Gram-negative bacterium is Escherishia coli.
4. A conjugate vaccine as claimed in claim 1, wherein the exoprotein is an exotoxin or exotoxoid.
5. A conjugate vaccine as claimed in claim 1, wherein the exotoxin is toxin A from Pseudomonas aeruginosa.
6. A conjugate vaccine as claimed in claim 1, wherein the exotoxoid is tetanus toxoid or diptheria toxoid.
7. A process for the preparation of a conjugate vaccine as claimed in any of claims 1, 2 or 3 comprising covalent linkage of an appropriate polysaccharide from the endotoxin of the bacterium with an exoprotein.
8. A process for the preparation of a conjugate vaccine as claimed in any of claims 4, 5 or 6 comprising covalent linkage of an appropriate polysaccharide from the endotoxin of the bacterium with an exoprotein.
9. A mixture of 3 to 15 conjugate vaccines, each of said conjugate vaccines comprising a non-toxic conjugate vaccine as defined in claim 1, wherein for each of said conjugate vaccines the polysaccharide originates from a different serotype of the same species of bacterium.
10. A polyvalent vaccine comprising a mixture of conjugate vaccines as defined in claim 1 wherein each of the conjugate vaccines raises antibodies against a parti-cular species of bacteria.
11. A conjugate vaccine as claimed in any of claims 1, 2 or 3 when used for the preparation of hyperimmune sera which in turn are used for the preparation of immunoglobulin which can be administered intravenously or intra-muscularly.
12. A conjugate vaccine as claimed in any of claims 4, 5 or 6 when used for the preparation of hyperimmune sera which in turn are used for the preparation of immunoglobulin which can be administered intravenously or intra-muscularly.
13. A conjugate vaccine as claimed in any of claims 9 or 10 when used for the preparation of hyperimmune sera which in turn are used for the preparation of immunoglobulin which can be administered intravenously or intra-muscularly.
14. An immunogenic conjugate, comprising (i) a P.
aeruginosa polysaccharide covalently linked through at least one of a hydroxyl or carboxyl group of said polysaccharide, said polysaccharide being essentially free of lipid A to (ii) a tetanus toxoid carrier protein.
aeruginosa polysaccharide covalently linked through at least one of a hydroxyl or carboxyl group of said polysaccharide, said polysaccharide being essentially free of lipid A to (ii) a tetanus toxoid carrier protein.
15. An immunogenic conjugate, comprising (i) a P.
aeruginosa polysaccharide covalently linked through at least one of a hydroxyl or carboxyl group of said polysaccharide, said polysaccharide being essentially free of lipid A, to (ii) a toxin A carrier protein.
aeruginosa polysaccharide covalently linked through at least one of a hydroxyl or carboxyl group of said polysaccharide, said polysaccharide being essentially free of lipid A, to (ii) a toxin A carrier protein.
16. The conjugate according to claim 14 or 15 wherein said conjugate has a molecular weight greater than 350,000.
17. The immunogenic conjugate according to claim 14 or 15 further comprising a spacer molecule, wherein said polysaccharide is covalently linked to said carrier protein through said spacer molecule.
18. The immunogenic conjugate according to claim 17 wherein said spacer molecule is water soluable adipic acid dihydrazide.
19. A P. aeruginosa immunogenic vaccine comprising said conjugate according to claim 14 or 15 and a pharmaceutically acceptable carrier, wherein said conjugate is present in an amount sufficient to elicit an immunogenic effect.
20. The vaccine according to claim 19 wherein said vaccine is nontoxic and nonpyrogenic.
21. The vaccine according to claim 19 wherein said vaccine is capable of inducing antibodies to both said polysaccharide and said carrier protein of said conjugate.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CH04199/85-0 | 1985-09-27 | ||
| CH419985 | 1985-09-27 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA1276552C true CA1276552C (en) | 1990-11-20 |
Family
ID=4271640
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA000517689A Expired - Lifetime CA1276552C (en) | 1985-09-27 | 1986-09-08 | Conjugate vaccine against infections by gram-negative bacteria, method for its preparation and use |
Country Status (11)
| Country | Link |
|---|---|
| US (1) | US4771127A (en) |
| EP (1) | EP0220387B1 (en) |
| JP (1) | JPH0662434B2 (en) |
| AT (1) | ATE56615T1 (en) |
| AU (1) | AU587865B2 (en) |
| CA (1) | CA1276552C (en) |
| DE (1) | DE3674328D1 (en) |
| DK (1) | DK163176C (en) |
| ES (1) | ES2000140A6 (en) |
| PT (1) | PT83096B (en) |
| ZA (1) | ZA866564B (en) |
Families Citing this family (21)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5360897A (en) * | 1981-08-31 | 1994-11-01 | The University Of Rochester | Immunogenic conjugates of streptococcus pneumonial capsular polymer and toxin or in toxiad |
| US5057301A (en) * | 1988-04-06 | 1991-10-15 | Neorx Corporation | Modified cellular substrates used as linkers for increased cell retention of diagnostic and therapeutic agents |
| JP2639416B2 (en) * | 1988-04-23 | 1997-08-13 | 財団法人化学及血清療法研究所 | Bivalve blood cell activating preparation for pearl production and method for producing pearl using the preparation |
| NZ239643A (en) * | 1990-09-17 | 1996-05-28 | North American Vaccine Inc | Vaccine containing bacterial polysaccharide protein conjugate and adjuvant (c-nd-che-a-co-b-r) with a long chain alkyl group. |
| US6139843A (en) * | 1991-04-02 | 2000-10-31 | Albert Einstein College Of Medicine Of Yeshiva University | Peptide compositions for the treatment of HIV |
| US5370872A (en) * | 1991-08-12 | 1994-12-06 | Swiss Serum And Vaccine Institute Berne | Escherichia coliO-polysaccharide-protein conjugate vaccine |
| US5554730A (en) * | 1993-03-09 | 1996-09-10 | Middlesex Sciences, Inc. | Method and kit for making a polysaccharide-protein conjugate |
| US5866132A (en) * | 1995-06-07 | 1999-02-02 | Alberta Research Council | Immunogenic oligosaccharide compositions |
| US5695768A (en) * | 1995-06-07 | 1997-12-09 | Alberta Research Council | Immunostimulating activity of Streptococcus pneumoniae serotype 8 oligosaccharides |
| US6749831B1 (en) * | 1997-05-16 | 2004-06-15 | Medical Defense Technology, Llc | Vaccine against lipopolysaccharide core |
| DE69830326T2 (en) * | 1997-10-03 | 2006-02-02 | Galenica Pharmaceuticals, Inc. | IMINING POLYSACCHARIDES, THEIR PREPARATION AND USE AS ADDITIVES AND IMMUNOSTIMULATING AGENTS |
| EP1073667A2 (en) | 1998-04-28 | 2001-02-07 | Galenica Pharmaceuticals, Inc. | Polysaccharide-antigen conjugates |
| JP2004515450A (en) * | 2000-04-18 | 2004-05-27 | エンドバイオロジックス, インコーポレイテッド | Lipopolysaccharide conjugate vaccine for the treatment of sepsis |
| US7749511B2 (en) | 2000-04-18 | 2010-07-06 | Endobiologics, Incorporated | Anti-sepsis conjugate vaccine |
| EP1651261B1 (en) * | 2003-08-06 | 2014-10-08 | THE GOVERNMENT OF THE UNITED STATES OF AMERICA, as represented by THE SECRETARY, DEPARTMENT OF HEALTH AND HUMAN SERVICES | Polysaccharide-protein conjugate vaccines |
| US8048432B2 (en) | 2003-08-06 | 2011-11-01 | The United States Of America As Represented By The Secretary Of The Department Of Health And Human Services | Polysaccharide-protein conjugate vaccines |
| AU2005249571B9 (en) * | 2004-06-04 | 2011-01-20 | The Government Of The United States Of America As Represented By The Secretary Of The Department Of Health And Human Services | Methods for preparing immunogenic conjugates |
| US7625736B2 (en) * | 2004-06-04 | 2009-12-01 | The United States Of America As Represented By The Department Of Health And Human Services | Methods for preparing immunogenic conjugates |
| EP2342217B1 (en) * | 2008-10-21 | 2015-12-23 | International Vaccine Institute | Novel shigella frotein antigens and methods |
| CN101912609B (en) * | 2009-08-20 | 2012-02-01 | 成都蓉生药业有限责任公司 | Composition for preventing and controlling pseudomonas aeruginosa infection and preparation method thereof |
| US9416173B2 (en) | 2011-04-21 | 2016-08-16 | Board Of Supervisors Of Louisiana State University And Agricultural And Mechanical College | Peptide and conjugate vaccines for fungal infections |
Family Cites Families (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4356170A (en) * | 1981-05-27 | 1982-10-26 | Canadian Patents & Development Ltd. | Immunogenic polysaccharide-protein conjugates |
| US4619828A (en) * | 1982-07-06 | 1986-10-28 | Connaught Laboratories, Inc. | Polysaccharide exotoxoid conjugate vaccines |
| US4663160A (en) * | 1983-03-14 | 1987-05-05 | Miles Laboratories, Inc. | Vaccines for gram-negative bacteria |
| US4693891A (en) * | 1985-09-09 | 1987-09-15 | Miles Laboratories, Inc. | Vaccine for Pseudomonas aeruginosa |
| US4707543A (en) * | 1985-09-17 | 1987-11-17 | The United States Of America As Represented By The Secretary Of The Army | Process for the preparation of detoxified polysaccharide-outer membrane protein complexes, and their use as antibacterial vaccines |
-
1986
- 1986-07-04 DK DK320786A patent/DK163176C/en not_active IP Right Cessation
- 1986-07-23 AT AT86110114T patent/ATE56615T1/en not_active IP Right Cessation
- 1986-07-23 DE DE8686110114T patent/DE3674328D1/en not_active Expired - Lifetime
- 1986-07-23 EP EP86110114A patent/EP0220387B1/en not_active Expired - Lifetime
- 1986-07-29 PT PT83096A patent/PT83096B/en not_active IP Right Cessation
- 1986-08-01 JP JP61180233A patent/JPH0662434B2/en not_active Expired - Fee Related
- 1986-08-04 US US06/892,846 patent/US4771127A/en not_active Expired - Lifetime
- 1986-08-11 ES ES8601006A patent/ES2000140A6/en not_active Expired
- 1986-08-29 ZA ZA866564A patent/ZA866564B/en unknown
- 1986-09-08 CA CA000517689A patent/CA1276552C/en not_active Expired - Lifetime
- 1986-09-29 AU AU63229/86A patent/AU587865B2/en not_active Ceased
Also Published As
| Publication number | Publication date |
|---|---|
| EP0220387A2 (en) | 1987-05-06 |
| ATE56615T1 (en) | 1990-10-15 |
| EP0220387A3 (en) | 1989-03-22 |
| AU587865B2 (en) | 1989-08-31 |
| ES2000140A6 (en) | 1987-12-16 |
| PT83096A (en) | 1986-08-01 |
| JPS6289632A (en) | 1987-04-24 |
| AU6322986A (en) | 1987-04-02 |
| JPH0662434B2 (en) | 1994-08-17 |
| US4771127A (en) | 1988-09-13 |
| PT83096B (en) | 1988-07-01 |
| DK163176C (en) | 1992-06-22 |
| DE3674328D1 (en) | 1990-10-25 |
| EP0220387B1 (en) | 1990-09-19 |
| DK320786A (en) | 1987-03-28 |
| DK320786D0 (en) | 1986-07-04 |
| DK163176B (en) | 1992-02-03 |
| ZA866564B (en) | 1987-05-27 |
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Legal Events
| Date | Code | Title | Description |
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| MKLA | Lapsed |