IE80851B1 - Helicobacter proteins and vaccines - Google Patents

Helicobacter proteins and vaccines

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Publication number
IE80851B1
IE80851B1 IE950496A IE950496A IE80851B1 IE 80851 B1 IE80851 B1 IE 80851B1 IE 950496 A IE950496 A IE 950496A IE 950496 A IE950496 A IE 950496A IE 80851 B1 IE80851 B1 IE 80851B1
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vaccine
protein
helicobacter pylori
kda
pylori
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IE950496A
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IE950496A1 (en
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Dermot Kelleher
Henry Windle
William Byrne
Ross Mcmanus
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Rican Limited
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Priority claimed from IE940538A external-priority patent/IE940538A1/en
Application filed by Rican Limited filed Critical Rican Limited
Priority to IE950496A priority Critical patent/IE80851B1/en
Publication of IE950496A1 publication Critical patent/IE950496A1/en
Publication of IE80851B1 publication Critical patent/IE80851B1/en

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Abstract

A vaccine includes at least one Helicobacter, especially Helicobacter pylori protein to which immunoreactivity is detected in H. pylori negative individuals. The Helicobacter proteins are preferably less than 30 kDa and the vaccine especially includes 24 to 25 kDa and/or 18 to 19 kDa proteins. The vaccine may include interleukin 12 as an adjuvant.

Description

“HELICOBACTER PROTEINS AND VACCINES” Field of the Invention The invention relates to a vaccine or therapeutic composition for die treatment or prophylaxis of Helicobacter pylori associated disease and protein used in the vaccine.
Background Helicobacter pylori is a widely prevalent organism found on gastric biopsy in approximately 30% of die population less than 40 years old with increasing incidence thereafter. The organism is a causative agent of chronic gastritis in humans (e.g. Marshall & Warren 19841; Blaser, 19902). Epidemiological studies have shown that H pylori is most commonly found in association with gastritis. Serological investigations have demonstrated that evidence of a current or prior infection can be found in 30 - 50% of a randomly chosen population of blood donors. No direct causal relationship has been conclusively proven for duodenal ulcer disease. However, die organism is found in 95% of patients with duodenal ulcer. Furthermore, eradication of the organism results in rapid ulcer healing (e.g. Rauws & Tytgat, 19903). These data provide strong evidence that H pylori is a dominant factor in the development of duodenal ulcer. Additional evidence for the pathogenic involvement of H. pylori in these conditions has been provided by studies with gnotobiotic piglets (Lambert et al., 19874) and the fulfilment of Koch’s postulates with human volunteers (Marshall et al., 1985s; Morris & Nicholson, 19876).
In addition, there is now strong circumstantial evidence impheating H. pylori in foe pathogenesis of gastric carcinoma (e.g. Jiang et al., 19877; Lambert et al., 19868; Crabtree et al., 1992’; 199310; Forman et al., 199011, 199112; Nomura et al., 199113; Pajsonnet et al., 199114). Most recently, foe Eurogast Study Group, led by -2Forman (199315), demonstrated a significant relationship between H. pylori seropositivity and gastric cancer mortality and incidence. Indeed, there is now a convincing body of literature implying infection with H. pylori in a considerable proportion of upper gastrointestinal morbidity. A number of hypotheses have been suggested for die pathogenic mechanisms of H. pylon induced gastroduodenal disease, including die production of cytotoxins and mechanical disruption of the epithelium (e.g. Blaser, 199216). Interestingly, however, many infected persons remain asymptomatic despite the persistent presence of the pathogen (Taylor & Blaser, 199117).
Statements of Invention According to die invention there is provided a vaccine prepared for the treatment or prophylaxis of Helicobacter pylori infection or Helicobacter pylori associated disease, the vaccine comprising H. pylori protein or a derivative, or fragment or mutant thereof to which immunoreactivity is detected in H. pylori negative individuals, the protein including one or both of a H. pylori protein having a molecular weight of 18 to 19 kDa and/or a H. pylori protein having a molecular weight of 24 to 25 kDa. Preferably the immunoreactivity is antibody based.
In a particularly preferred embodiment of die invention, the vaccine indudes a H. pylori protein having a molecular weight of 24 to 25 kDa or a derivative or fragment or mutant thereof.
The 24 to 25 kDa protein has a N-terminal amino add sequence listed in Sequence Id. No. 1, or a portion thereof.
The 24 to 25 kDa protein has an internal amino acid sequence listed in Sequence Id. No. 4, or portion thereof. -3In a particularly preferred embodiment of the invention, the vaccine includes a H pylori protein having a molecular weight of 18 to 19 kDa protein, or a derivative, fragment or mutant thereof.
Most preferably the 18 to 19 kDa protein has a N-terminal amino acid sequence listed in Sequence Id. No. 2, or a portion thereof.
The 18 to 19 kDa protein also indudes an internal amino acid sequence listed in Sequence Id. No. 3, or a portion thereof.
In a particularly preferred embodiment of die invention, the 18 to 19 kDa protein has an N-terminal Sequence listed in Sequence Id. No. 6, or a portion thereof.
The vaccine may indude a pharmaceutically acceptable carrier.
The vaccine may be combined with a suitable adjuvant such as interleukin 12 or a heat shock protein or both.
The vaccine may indude at least one other pharmaceutical product such as an antibiotic and/or antibacterial agent such as bismuth salts. Typically the antibiotic is sdected from one or more of metronidazole, amoxycillin, tetracycline, erthromycin, clarithromycin or tinidazole.
The vaccine may be in a form for oral, intranasal, intravenous or intramuscular administration.
The vaccine may indude a peptide delivery system.
The vaccine is for the treatment or prophylaxis of Helicobacter pylori infection or Heliocabcterpylori associated disease(s).
According to another aspect of the invention there is provided die use of a Helicobacter pylori protein or derivative or fragment or mutant thereof to which immunoreactivity is detected in H pylori negative individuals, the protein -4including one or both of a Helicobacter pylori protein having a molecular weight of 18 to 19 kDa and/or a H pylori protein having a molecular weight of 24 to 25 kDa, in die preparation of a medicament for use in a method for the treatment or prophylaxis of H. pylori infection or H. pylori associated disease in a host. Preferably, the immunoreactivity is antibody based.
In a particularly preferred embodiment of the invention, the Helicobacter pylori protein has a molecular weight of 24 to 25 kDa or derivative or fragment or mutant thereof.
The 24 to 25 kDa has the N-terminal amino add sequence listed in Sequence Id. No. 1, or a portion thereof.
The 24 to 25 kDa Helicobacter pylori protein has an internal amino add sequence listed in Sequence Id. No. 4, or a portion thereof.
In another preferred embodiment of the invention, the Helicobacter pylori has a molecular weight of 18 to 19 kDa or a derivative or fragment or mutant thereof.
The 18 to 19 kDa Helicobacter pylori protein has the N-terminal amino add sequence listed in Sequence Id. No. 2, or a portion thereof.
The 18 to 19 kDa Helicobacter pylori protein has the internal amino add sequence listed in Sequence Id. No. 3, or a portion thereof.
The 18 to 19 kDa Helicobacter pylori is further characterised in that it indudes the N-terminal amino add sequence listed in Sequence No. 6.
The invention further provides monoclonal or polyclonal antibodies or fragments thereof, to H pylori protein or a derivative or fragment or mutant thereof, to which -5immunoreactivity is detected in H. pylori negative individuals, the protein including a H. pylori protein having a molecular weight of 18 to 19 kDa.
The invention also provides purified antibodies or serum obtained by immunisation of an animal with die vaccine according to the invention.
The invention also envisages the use of such serum and antibodies in the treatment or prophylaxis of Helicobacter associated disease(s) and in particular Helicobacter pylori associated disease(s).
The invention also includes the use of interleukin 12 in combination with the 18 to 19 kDa protein, the 24 to 25 kDa or any other H pylori subunit as an adjuvant therapy.
Therefore, in another aspect, the invention provides a vaccine against H. pylori comprising an immunogenically effective amount of a Helicobacter or a subunit, fragment, derivative, precursor or mutant thereof in combination with interleukin 12 as an adjuvant. Preferably the Helicobacteris Helicobacterpylori.
In one embodiment of the invention the vaccine indudes an antibiotic and may alternatively or additionally indude an antibacterial agent.
Description of Drawings Fig. 1: Adult sera (CLO negative) screened for the presence of anti-#. pylori IgG antibodies. The figure shows a Western blot of H pylori probed with serum obtained from CLO negative individuals. All sera were diluted 1:100 in PBS containing fat-free dried skimmed milk (5%, w/v). Proteins were transferred from SDS-PAGE gels to PVDF membrane. The antigen-antibody complexes were detected -6Fig.2: Fig.3: Fig. 4: Fig.5: Fig. 6: on washed membranes using an enhanced chemiluminescent detection system. Each track represents a different serum sample.
Absorbed sera : Sera from two individuals negative for H Pylori were absorbed with either whole C. jejuni (track A), H.pylori (track B), or E. coli (track C).
Partial purification of 18 and 25 kDa proteins: Both proteins were purified from whole Helicobacter pylori on the basis of molecular weight using preparative continuous-elution SDS-PAGE on a Model 491 Prep-Cell (Bio-Rad).
Sera obtained from CLO negative children screened for the presence of anti-#. pylori IgG antibodies. The figure shows a Western blot of H. pylori probed with serum obtained from CLO negative children. All sera were diluted 1:50 in PBS containing fatfree dried skimmed milk (5%, w/v). Each track represents a different serum sample.
Antigens recognised on C. jejuni and E. coli by anti-#, pylori antiserum. The figure shows a Western blot of H. pylori (track A), C. jejuni (track B) and E. coli (track C) probed with rabbit anti-#. pylori antiserum. Each bacterium (5 pg) was subjected to SDSPAGE followed by immunoblotting.
Western blot of purified 25 kDa protein developed with serum from an individual negative for #. pylori. Purified 25 kDa protein was subjected to SDS-PAGE and Western blotting. The blot was probed with serum obtained from a subject uninfected with #. pylori. -7Fig. 7: Biotinylation of proteins located on the surface of Helicobacter pylori.
Agar-grown H pylori were harvested in phosphate buffered saline (pH 7.3) and washed twice in this buffer prior to biotinylation of surface exposed proteins. Bacteria (2 nig ml'1) were resuspended in PBS (1 ml) and prewarmed to 37°G. Thereafter, biotin-X-NHS (Sulfosuccinimidyl-6(biotinamido) - hexanoate; Calbiochem) was added to the final concentration of ImM and was prepared immediately before use. After mixing to 10 min at 37°C, the labelling reaction was terminated by the addition of 1.5 M Tris-Cl (pH 8) to a final concentration of lOmM. The suspension was washed three times by centrifugation (10,000 g, 1 min) in ice-cold PBS. Examination of the bacteria by light microscopy after the labelling and washing procedures demonstrated that the cells were still intact and motile. Biotinylated H. pylori was subjected to analytical SDS-PAGE, followed by Western blotting, to identify the biotinylated proteins. The Western blots were developed with Extravidin-peroxidase (Sigma).
Fig. 8: Illustrates thymidine incorporation of lymphocytes in response to H pylori in the presence and absence of interleukin 12.
Fig. 9: Illustrates thymidine incorporation of peripheral blood mononuclear cells in the presence or absence of H. pylori with or without anti-interleukin 10 or recombinant interleukin 12.
Detailed Description of the Invention We have studied the prevalence of immuno-reactivity to H. pylori in both infected and un-infected individuals and found that un-infected individuals have a high response to H. pylori both in their B-cell and T-cell systems. Specifically, the Tcell immune response to H. pylori seems to be stronger in individuals who are -8negative for the organism. In this regard we have examined the secretion of the cytokine y-interferon which is extremely important for the killing of microorganism by macrophages. Secretion of if-interferon by T-cells of patients infected with H. pylori was considerably less than secretion by un-infected individuals when their T-cells were exposed to the organism (Fan et al., 199318). Hence, these data suggest that individuals who are H. pylori negative have been exposed to the organism and may potentially have cleared the organism. Furthermore, the response to the organism is considerably more potent in this group of individuals than it is in die H. pylori positive patients.
The term “H. pylori negative. individuals” means individuals with immunoreactivity to H. pylori who do not have evidence of H. pylori gastric colonisation as determined by techniques such as one or more of rapid urease testing, histological or culture of gastric biopsies.
A second component relates to die antibody response to H. pylori in H. pylori . negative individuals. Briefly, we have demonstrated using a sensitive detection system that the majority of H. pylori negative individuals have detectable antibodies to two H. pylori proteins. Specifically, these proteins are of MW 18 20 19 and 25- 26 kDa. It is thus proposed that a potent immune response to these antigens results in protective immunity to the organism. Furthermore, we have partially sequenced these proteins.
In many cases antibodies to H pylori are detected by ELISA.
An inherent constraint in the design of ELISA based detection systems is that of establishing a cut off point such that all samples below this threshold are considered negative. Clearly, many seropositive cases will remain undetected in this situation and a true estimate of the incident of prior contact with the organism will thereby be underestimated. In this approach we use Western blotting to investigate antigen specificity of systemic responses to H. pylori in both healthy -9and H. pylori-mfected individuals and have shown that the incidence of seropositivity in H. pylori negative individuals is much greater than has previously been demonstrated. Furthermore, we have demonstrated that antibodies to a 24 td 25 kDa protein are detectable in the majority of H. pylori negative individuals. These were detected using a technique which we have modified called Enhanced Chemiluminescence. Enhanced Chemiluminescence on Western blot analysis reveals that the majority of uninfected individuals have antibodies which are specific for H. pylori and recognise antigens which are not present on other micro organisms. Of these antigens the most common one recognised is a 24 to 25 kDa protein which appears to be specific to H pylori. Hence, these data suggest that immmunisation with the 24 to 25 kDa protein or sub-unit thereof could have the potential to confer protective immunity on individuals who are either un-infected with the organism or individuals in whom the organism has been cleared by antibacterial treatment. A second protein was also identified at 18 to 19 kDa in a large subgroup of H. pylori negative individuals. Similarly, immunization with this protein or subunit thereof could also confer protective immunity.
We have developed a novel assay for detection of antibodies to H. pylori. This assay uses Western blotting and Enhanced Chemiluminescence (ECL). Using this assay we have demonstrated that approximately 75% of individuals who are negative for H. pylori by routine testing such as the rapid unease test have in fact got detectable antibodies to H. pylori (Fig. 1).
Furthermore, these antibodies are not absorbed by C. jejuni or by E. coli suggesting that this is a specific antibody response (Fig. 2). Of particular note we have performed characterisation of the antigens recognised by these antibodies by molecualr weight, using ECL Western blotting. Sera from un-infected individuals recognize a range of antigens on H. pylori. The most common antigen recognised is a 24 to 25 kDa protein which is recognised in over 70% of individuals who are negative for the organism on Rapid urease testing. Hence this suggests that the 24 to 25 kDa protein may be an immunodominant antigen which evokes a powerful -10immune response in individuals who are negative for the organism. A second protein was identified at 18 to 19 kDa which elicited significant antibody responses in H. pylon-negative children. These proteins have been further characterised by N-terminal and internal sequencing as outlined in the Appendix.
Finally a cytokine produced by macrophages called interleukin 12 may significantly enhance x-interferon production in response to antigen. As stated previously, antigen-specific interferon production is reduced with H. pylori positive individuals. The addition of IL-12 to immunisation schedules with a 25 kDa protein would be expected to boost host immunity to H. pylori by augmenting the tf -interferon response.
Materials. All antibodies were obtained from Dako Ltd., High Wycombe, Bucks., United Kingdom. All other chemicals and solvents were obtained from either the Sigma Chemical Company Ltd., Poole, Dorset, United Kingdom or BDH Chemicals Ltd., Poole, Dorset, United Kingdom.
SDS-PAGE. Discontinuous SDS-PAGE was performed essentially as described by Laemmli (1970)19. A total of 5 mg of acetone-precipitated H. pylori protein were located into each well. Gels were either stained with Coomassie Blue R-250 or processed for immunoblotting. Broad range molecular weight markers were purchased from Bio-Rad Laboratories, 3300 Regatta Blvd., Richmond, CA 94804. The molecular masses are expressed as kDa.
Western Blotting. Proteins from SDS-PAGE gels (30% T/2.67% C) were electroblotted (0.8 mA/cm2 for 1 h) to PVDF membrane using a semi-dry blotting apparatus (LKB/Pharmacia), essentially as described by Towbin et al, (1979). Primary antiboides (human serum; 1/50 —1/100 dilution) were detected using a 1/5,000 dilution of anti-human IgG (horseradish peroxidase—conjugated) in combination with enhanced chemiluminescence. Blots were washed in PBS containing fat-free dried skimmed milk (5%, w/v) and Tween-20 (0.05%, v/v). -11Blots were exposed to Kodak X-OMAT S film for 1-10 s. Exposed films were developed in Kodak LX-24 developer and fixed in Kodak dental X-ray fixer.
Sera. Serum samples were obtained from the Research Centre, Our Ladies Hospital for Sick Children, Crumlin, Dublin, All subjects were attended for medical conditions other than gastroenterological disorders. In addition, blood sample were obtained from a randomly selected cohort of children (Harcourt Street Childrens Hospital, Dublin) or from adults attending die gastenterology unit of St. James’s Hospital, Dublin. All patients had a rapid urease (CLOtest) performed. Patients were defined as H. pylori positive or negative on the basis of positive or negative responses on rapid urease test.
Anti- H. ovlori antiserum. Anti- H. pylori antiserum was a kind of gift from Prof.
B. Drumm and Dr. M. Clyne. The antiserum was raised in New Zealand white rabbits against whole H. pylori using conventional immunizing and boosting procedures.
Protein Measurements. Protein was measured by the method of Markwell et al. (1978)20 with bovine serum albumin as the protein standard.
Absorption of Sera. Antisera were absorbed with either E. coli or C. jejuni by incubating a suspension of die bacteria with patient sera for 2 h at room temperature with gentle mixing. The bacteria were removed from suspension by centrifugation (12,000 x g, 3 min).
Bacterial strains and growth conditions. The clinical isolates H. pylori used in this study were isolated from antral biopsies obtained from patients attending the gastronenterology clinic at St. James’s Hospital, Dublin. H. pylori was grown under microaerophilic conditions for 4 days on 7% lysed horse blood agar at 37°C. Cells were harvested into ice-cold phosphate buffered saline (pH 7.5) containing PMSF (ImM), EDTA (1 mM), and leupeptin (50 pg/ml). The cells were washed -12twice by centrifugation (10,000 x g, 5 min, 4°C) in this buffer before use. C. jejuni was a clinical isolate from stool in a patient with C. jejuni enteritis and was grown for two days exactly as described above with the exception that the incubation temperature was 42°C. The strain of E. coli used in this study is commercially available (Gibco) NTCC 11637 and was kindly provided by Dr. Ciaran Cronin, Dpt. Pharmacology, University College Dublin.
Methods used in the identification and partial purification of two novel antigens from Hdicobactcr&vjozi Methods Western Blotting. Proteins from SDS-PAGE gds (30% T/2.6% C) were electroblotted (0.8 mA/cm2 for 1 h) to PVDF membrane using a semi-dry blotting apparatus (LKB/Pharmacia). Primary antibodies (human serum; 1/50 - 1/100 dilution) were detected using a 1/5,000 dilution of anti-human IgG (horseradish peroxidase-conjugated) in combination with enhanced chemiluminescence (see below). Blots were washed in phosphate buffered saline (pH 7.5) containing fatfree dried skimmed milk (5%, w/v) and Tween-20 (0.05%, v/v). Blots were exposed to Kodak X-OMAT S film for 1-10 s. Exposed films were developed in Kodak LX-24 developer and fixed in Kodak dental X-ray fixer.
Enhanced Chemiluminescence (ECU The use of chemiluminescence to detect antibodies in Western blotting in preference to the conventional procedures of employing chromogenic substrates as detection reagents was adopted primarily because of the reporting gain in the sensitivity of detection (approximately 10-fold) over that found when chromogens are used. Oxidized luminol emits visible light and the intensity of this light emission is increased 100-fold in the presence of chemical enhancers (e.g. iodophenol). The method is described below: -13Substrate Concentration/ Amount Luminol 4-Iodophenol Hydrogen Peroxide 1.2 mM (in 0.1 Μ-Tris (50ml), pH 8.8) 0.4 mM (dissolved in DMSO before use) 17 μΐ of a 30% (v/v) solution Blots were incubated in the above mixture for one minute and then exposed to Xray film as described above.
Partial Purification of 18 and 25 kDa Proteins.
Both proteins were partially purified from whole Helicobacter pylori on the basis of molecular weight (Fig. 2) using preparative continuous-elution sodium dodecyl sulphate polyacrylamide gel electrophoresis (SDS-PAGE) on a Model 491 PrepCell (Bio-Rad). This method enables us to quantitatively purify preparative amounts of proteins in a soluble form.
Purification Method mg H. pylori were precipitated with ice-cold acetone, washed once in acetone and the precipitate then solubilised in 3.8 ml SDS-PAGE sample buffer (62 mM Tris, pH 6.8; glycerol (10%, v/v); SDS (2%, v/v); 2-mercaptoethanol (5%, v/v); bromophenol blue (0.002%, v/v)). Published electrophoretic procedures, with very minor modifications, were followed throughout sample preparation.
Loading: The protein mixture, in sample buffer, was loaded onto a 12.5% polyacrylamide tube gel (30% T/2.67% C). The dimensions of foe tube gel were: 28 mm internal diameter; upper surface 3.6 cm2; stacking gel 2 cm; resolving gel 10 cm. -14Running Conditions: Electrophoresis was performed at 40 mA (constant current) overnight at room temperature. Fractions (1 ml) were collected at 0.1 ml/min. Samples of each fraction (5 μΐ) were subjected to analytical SDS-PAGE to assess the purity and antigenicity of each protein. Every fraction within the molecular mass region of interest was screened by both SDS-PAGE (to assess purity) and Western blotting (to assess antigenicity) in an attempt to isolate and characterise the individual immunogenic proteins. The resolution of this technique is such that pure preparations of single proteins may be achieved once optimal electrophoretic conditions have been established. Preliminary optimization protocols entailed electrophoresing mixtures of H. pylori proteins under conditions designed to favour high resolution of low molecular weight proteins. The final electrophoretic conditions used to achieve partial purification of the selected proteins are detailed in the methods section. Using these exact conditions the 18 kDa proteins eluted between 11-14 ml and the 25 kDa protein eluted with 16-20 ml. The molecular weights of the proteins were determined by analytical SDS-PAGE using a range of low molecular weight marker proteins (range: 14.5 kDa - 66 kDa; code: Sigma SDS-7) and Western blotting confirmed that these proteins were the immunogens of interest.
Figure 1 shows Western blot analysis of antibody responses to H. pylori in individulls negative for H. pylori on Rapid urease testing. Western blotting was performed as previously described using an enhanced chemiluminescence detection system. Antibodies to a large range of H. pylori proteins were seen in individuals who are H. pylori negative on Rapid urease testing. The most common antigen to which an antibody was detected was the 25 kDa protein. Figure 3 shows a preparative SDS gel elution profile of the 25 kDa and 18 kDa proteins. These proteins have been further characterised by N-terminal and internal sequencing as outlined in the Appendix. -15CLO negative adults Similarly, a cohort of 19 adult sera was screened for anti- H pylori IgG antibodies. Each of these subjects was CLO negative, yet 83% had detectable antibodies (IgG) to H. pylori (Fig. 1). Taken together, these data suggest extensive prior contact with H. pylori. The most common antigen to which an antibody was detected was a 25 kDa species.
CLO negative children The systemic humoral immune response (IgG) to H. pylori was studied in two groups of children also. None of these subjects had received any form of anti-//. pylori therapy. However, in almost all cases the children had a specific antibody response to H. pylori. The first cohort studies consisted of twenty children (age range: 4 - 15 years), negative for H. pylori on CLO test. Of these, 75% had detectable IgG antibodies to H pylori (Fig. 4).
The second cohort of children (n = 20) were asymptomatic and presented in hospital with conditions other than gastrointestinal disorders. Yet 13/18 (72%) had detectable IgG antibodies to several H. pylori specific antigens. However, from die intensity of the response the data suggest that the antibody response is most likely due to prior contact with the bacterium, when compared to the considerably stronger response observed with H. pylori positive individuals.
Cross reactivity with other Bacteria As many bacteria share common antigenic determinants, we examined the extent of cross-reactivity between H pylori and the closely related C. jejuni, in addition to E. coli, using two complimentary approaches. Firstly, the ability of the anti- H. -16pylori polyclonal antiserum to recognise antigens on both C. jejuni and E. coli was examined by Western blotting (Fig. 2).
Anti- H. pylori antiserum recognised a number of antigenic determinants on both E. coli and C. jejuni. Specifically, the antiserum recognises proteins of molecular mass 72, 50, 40, 36 and 25 kDa on C. jejuni and proteins of molecular mass 200, 116,45 and 38 kDa on E. coli (Fig. 5). Of these, only 3 proteins (70, 25 kDa from C. jejuni and 200 kDa from E. coli) show pronounced cross-reactivity with anti- H. pylori antiserum. Therefore, the observed cross reactivity is clearly not extensive. Secondly, absorption experiments demonstrated that this cross reactive antigen recognition was of minor significance. Serum samples absorbed with clinical isolates of H. pylori and C. jejuni in addition to a commercially available strain of E. coli demonstrated that seroreactivity could be eliminated by absorbing with H. pylori but not with C. jejuni οι E. coli (Fig. 2). Figure 2 is a representative experiment Absorption studies were performed on approximately half of the serum samples screened in this study with similar results to those shown. The 18 and 25 kDa proteins were also detected in H. pylori Reference Strains NTCC 11637 and 11638 in addition to all clinical strains tested.
Having partially purified the 24 - 26 kDa protein by preparative continuouselution electrophoresis as shown in Fig. 3, we confirmed the antigenicity of die 24-26 kDa protein by probing a Western blot of purified 24-26 kDa protein with serum from an uninfected individual (Fig. 6). The example shown in Fig. 6 is a representative experiment where the blot was incubated with the serum from an H. pylori un-infected individual. Clearly, this serum sample contains antibodies that specifically recognise the 24-26 kDa protein and furthermore, the results of this experiment demonstrate that the antigen preparation is highly enriched for this protein and that no other immunogenic proteins are present in this preparation. We have obtained similar results with the 18-20 kDa protein. -17Biotinylation of whole intact Helicobacter pylori Agar-grown H. pylori Vicco harvested in phosphate buffered saline (pH 7.3) and washed twice in this buffer prior to biotinylation of surface exposed proteins. Bacteria (~2 mg ml*1) were resuspended in PBS (1 ml) and prewarmed to 37°C.
Thereafter, biotin-X-NHS (Sulfosuccinimidyl-6-(biotinamido)-hexanoate; Calbiochem) was added to a final concentration of ImM and was prepared immediately before use. After mixing for 10 minutes at 37°C, the labelling reaction was terminated by die addition of 1.5 M Tris-Cl (pH 8) to a final concentration of lOmM. The suspension was washed three times by centrifugation (10,000 g, 1 min) in ice-cold PBS. Examination of the bacteria by light microscopy after the labelling and washing procedures demonstrated that the cells were still intact and motile.
Analysis of biotinylated proteins Biotinylated H. pylori was subjected to both analytical and preparative SDS15 PAGE, followed by Western blotting, to identify die biotinylated proteins. The Western blots were developed with Extravidin-peroxidase (Sigma). Extensive incorporation of the biotin ester into H. pylori proteins was observed (Fig. 7). Furthermore, it is dear from this figure that proteins in the 18-24 kDa region are biotinylated as are a number of other proteins (Table 1), indicating that these proteins are present on the surface of die bacterium. -18Table 1 Biotinylated Protein Apparent molecular weight 1 13,800 2 15,600 3 16,600 4* 17,700 5 20,500 6* 23,500 7 26,400 Method description T-cell immune response to Helicobacter pylori We examined the T-lymphocyte proliferative responses to H pylori using a thymidine incorporation assay. Briefly, lymphocytes were isolated by density gradient centrifugation on a Ficoll-Hypaque gradient. Lymphocytes were seeded into 96-well microtitre plates at a density of 10s cells/well in RPMI 1640 medium containing 10% foetal calf serum. A sonicated irradiated preparation of H. pylori was added at a concentration of 3 pg/ml. Medium alone was added to control wells. In addition interleukin 12 (R & D suppliers) was added at a concentration of500 pg/ml. Cells were then cultured in a 5% CO2 incubator for 4 days at 37°C.
At 4 days tritiated thymidine 1 pCi/ml was added and cultures continued for a further 24 hours before harvesting using a multiple automated sample harvester. In additional experiments, cells were stimulated using OKT3 antibody to the CD3 -19T-cell receptor associated complex in die presence and absence of the H pylori preparation as above. In these studies, interleukin 12 was similarly added. Antibody to interleukin 10 was added in some experiments.
T-cell response to H. pylori is significantly augmented by interleukin 12 In a cohort of patients in whom lymphocyte proliferative responses to H. pylori were examined as described in the methodology, interleukin 12 significantly increased the proliferation of the peripheral blood mononuclear cell population to H. pylori (n=12, p<.05) (Fig. 8). These data demonstrate clearly that interleukin 12 has adjuvant properties in respect of H. pylori immunogenicity.
Interleukin 12 overcomes the suppression of T-cell responses induced by H. pylori The H. pylori antigen preparation significantly inhibited the proliferation induced by the T-cell mitogen OKT3. This inhibition could be abolished using antibody to interleukin 10, a cytokine produced by T-helper 2 cells known te suppress the Thelper 1 cell pathways involved in cell proliferation. These data therefore suggest that the suppression of T-cell responses induced by H. pylori and significantly increased proliferation responses over the baseline OKT3-induced responses sugggesting that this cytokine is capable of overcoming the effects of the H. pylori T-helper 2 pathway.
Fig. 8 illustrates thymidine incorporation of lymphocytes in response te H. pylori in the presence and absence of interleukin 12. Interleukin 12 significantly augmented proliferation of peripheral blood mononuclear cells in response to H. pylori.
Fig. 9 illustrates thymidine incorporation of peripheral blood mononuclear cells in the presence or absence of H. pylori with or without anti-interleukin 10 or -20recombinant interleukin 12. Both interleukin 12 and anti-interleukin 10 significantly abolished//, /ry/ori-induced inhibition of lymphocyte proliferation.
It will be appreciated that interleukin 12 may also be used as an adjuvant with any //. pylori protein or derivative or fragment thereof. Its application is not limited to the specific 25 kDa or 18 kDa proteins referred to above. The interleukin 12 may be conjugated with the //. pylori unit in such a way as to allow the interleukin to be released in vivo, for example by peptic acid and gastric enzymes/or urease.
It will be appreciated by those skilled in the art that while we have referred to a molecular mass of 24 to 25 kDa and 18 to 19 kDa the molecular mass my lie in the 24-26 kDa and 17-19 kDa range. Other related organisms such as //. felts or //. mustelis may produce gastric diseases in animal models.
Cross reactivity between proteins from Helicobacter species may mean that antigens from an individual bacterial species could provide protection in an animal which is not its normal host.
The dominant antigens to which antibody is detected in Helicobacter pylori-Tte&live individuals are the 18-19 and 24-25 kDa antigens. Hence, use of an antigenic preparation containing all antigens less than 30 kDa, preferably less than 29, ideally less than 28 and preferably less than 27 kDa and would be enriched in the immunodominant antigens to be used in putative vaccine.
It will be apparent that cytokine interleukin 12 acts as an adjuvant to potentiate the immunogenicity of //. pylori. In particular, it potentiates the immunogenicity of protein fractions of less than 30 kDa, especially the 18 kDa and 25 kDa protein fractions of //. pylori.
It will he appreciated that interleukin 12 may also be used as an adjuvant with any H. pylori protein or derivative or fragment thereof. Its application is not limited to -21 the specific 25 kDa or 18 kDa proteins referred to above. The interleukin 12 may be conjugated with the H pylori unit in such a way as to allow the interleukin to be realised in vivo, for example by peptic acid and gastric enzymes/or urease.
It will be appreciated by those skilled in the art that while we have referred to a molecular mass of24 - 25 kDa and 18 - 19 kDa the molecular mass may lie in the 24 - 26 kDa and 17-19 kDa range. Other related organisms such as H felis or H. mustelis may produce gastric diseases in animal models.
Cross reactivity between proteins from Helicobacter species may mean that antigens from an individual bacterial species could provide protection in an animal which is not its normal host.
The dominant antigens to which antibody is detected in Helicobacter pylori-negative individuals are the 18-19 and 24-25 kDa antigens. Hence, use of an antigenic preparation containing all antigens less than 30 kDa, preferably less than 29, ideally less than 28 and preferably less than 27 kDa and would be enriched in the immunodominant antigens to be used in putative vaccine.
Partial sequencing of the two antigens from Helicobater pylori N-terminal sequence analysis Purified 18 and 24 kDa proteins were electroblotted to PVDF and ProBlott, respectively, from 12.5% polyacrylamide gels. The proteins were located on the membranes by staining with 0.1% amido black (in 1% acetic acid, 40% methanol) for 15s followed by destaining in several changes of distilled deionized water. The membranes were air-dried thoroughly and submitted for sequence analysis using the Edman degradation procedure as described by Matsudaira (198921). -22The N-terminal amino add sequence of the 25 and 18 kDa protein are given in Sequence Id No’s 1 and 2 respectivdy.
Peptide Mapping The N-chlorosucdnimide peptide mapping method of Lischwe and Ochs (1982)22 was used with minor modifications. Bands of interest were located on SDSPAGE gds (12.5% T) by briefly staining the gd with 0.1% Coomassie Blue R250 (in 50% methanol, 10% acetic add) and then excised with a scalpel blade. The protein present in the gd slices was digested with N-chlorosucdnimide (15 mM) in acetic add/urea/water (1:1:1 v/w/v) for 30 min at 20°C. The treated gel slices were then washed with several changes of water and equilibrated with SDSPAGE sample buffer exactly as described by Lischwe and Ochs. Finally, the gel slices were placed in the sample wells of a 15 % polyacrylamide SDS-PAGE gd and electrophoresed. Following electrophoresis, the separated peptides were transferred to either PVDF or ProBlott by Western blotting. Peptides were visualised by staining the membrane with 0.1% amido blade in acetic add (1%) and methanol (40%). After extensive washing with water, the peptides were submitted for sequencing without any further modifications.
Mercaptoacetic add (2 mM) was induded in the upper electrode buffer during all SDS-PAGE dectrophoretic procedures. This mobile thiol behaves as a free radical scavenger and thus prevents N-blocking.
Amino add sequences for internal peptides from the 18 and 25 kDa protein are given in Sequence Id. No.’s 3 and 4 respectivdy.
Extraction of Helicobacter pylori chromosomal DNA Chromosomal DNA was extracted as described (Silhavy et al., 1984. Experiments with gene fusion. C.S.H. publications). -23Amplifying the sequence of the 18-19 protein kDa gene of using degenerate primers.
Degenerate DNA sequence was deduced from the amino arid sequence listed in Sequence Id. No’s 2 and 3. Four degenerate primers were designed from these sequences, to allow for a two stage, nested, PCR reaction. Eagl restriction enzyme sites were built into each primer, to allow for subsequent cloning of the fragment. Where three or more bases were possible at any site, inosine was incorporated instead of all possible bases, except, where such sites were four bases or less from die primers 3’ (3 prime) terminal, in which case all possible bases were included. Inosine was also avoided at positions immediately adjacent to the Eagl sites.
Degenerate primer for gene pl8: I 1. GAARACGGCC GARATIYTIA ARCAY YTICA RGC 2. TCYTC GGCCG TYTCY TCIGT NGCY 3. RATIY TCGGC CGYYICARGCIGAYG C 4. ATYTC GGCCGTIGCYTTRTG NAC Genomic DNA for the 18 to 19 kDa protein gene pl8 was amplified as follows using die outer set of primers for 3 minutes to denature the DNA, followed by 35 cycles of 94 degrees C for 30 seconds, 56 degrees C for 40 seconds and 72 degrees C for 30 seconds. 100 pmol of each primer was used, in the presence of 2.5 mM MgCl2 and 0.2 mM dNTPs, in a reaction volume of 50 μΐ. 1 μΐ of this reaction was used as die substrate for the ’nested’ reaction. This reaction was the same as outlined for the above reaction, except that the inner primers (primers 3 & 4) were substituted for the external primers, and a concentration of 2.0 mM MgCl2 was used. Electrophoresis of the* products of the reaction resulted in a dearly visible band on a 2% agarose gel, estimated at approximately 120 bp in size (as judged by a molecular size ladder). -24Sequencing the amplified DNA sequence.
The nested PCR fragment corresponding to the 18 - 19 kDa protein gene was cloned by digesting the fragment with Eagl and ligating this into die unique Eagl site in the Bluescript vector (Stratagene). E. coli cells were transformed (according to standard procedures) and plasmid DNA was harvested using the alkaline lysis method (Sambrook et al., 1989. Molecular cloning : A laboratory manual 2nd. Ed., CSH publications) followed by an RNAase digestion step, phenol/chloroform extraction and precipitation using 2.5M ammonium acetate and 2 volumes of ethanol. Two independent isolates of plasmid DNA were sequenced using forward and reverse universal sequencing primers. The inserted DNA derived from the pl8 gene was sequenced in the forward and reverse orientations. Sequencing was performed using an ABI automated sequencer and a Genpak PCR based fluorescent dideoxy chain terminator termini sequencing kit.
The sequence of bases between the terminal of the internal PCR primers is: GATCGTGTTATTTATGAAAGTGCATAACTTCCATTGGAATGTGAAAG GCACCGATTTTTTCAAT This sequence of bases translates into the amino add sequence listed in Sequence Id. No. 5.
This sequence (Sequence Id. No. 5) overlaps with both the 18 kDa protein Nterminal amino add sequence listed in Sequence Id. No. 2 and the 18 kDa protein internal amino add sequence listed in Sequence No. 3, to give the enlarged Nterminal amino add sequence listed in Sequence Id. No. 6.
Many variations on the specific embodiments described will be readily apparent and accordingly the invention is not limited to the embodiments hereinbefore described which may be varied in detail. -25LIST OF REFERENCES 1. Marshall, B. J. and Warren, J. R. (1984). Unidentified curved bacilli in the stomach of patients with gastritis and peptic ulceration. Lancet 1, 13111314. 2. Blaser M. J. (1990). Helicobacter pylori and the pathogenesis of gastrodudodenal inflammation. 7. Infect. Dis. 161,626-633. 3. Rauws, E.A.J. and Tytgat, G. N. J. (1990). Eradication of Helicobacter pylori cures duodenal ulcer: Lancet 1,1233-1235. 4. Lambert, J. R., Borromeo, M., Finkard, K. J., Turner, H., Chapman, C. B., and Smith, M. L. (1987). Colonisation of gnotobiotic pigs with Campylobacter pylori - an animal model ? 7. Infect. Dis. 155,1344.
. Marshall, B. J., Armstrong, J. A., McGechie, D. B., and Glancy, R. J. (1985). Attempt to fulfil Koch’s postulates for pyloric Campylobacter. Med. J. Aust. 142,436439. 6. Morris, A. and Nicholson, G. (1987). Ingestion of Campylobacter pylori causes gastritis and raises fasting gastric pH. Am. J. Gastronenterol. 82, 192—199. 7. Jiang, S. J., Liu, W. Z., Zhang, D. Z., Shi, Y., Xiao, S. D., Zhang, N. Z., and Liu, D. Y., (1987). Campylobacter-like organisms in chronic gastritis, peptic ulcer and gastric carcinoma. Scand. J. Gastronenterol. 22, 553-558. 8. Lambert, J. R., Dunn, K. A., Eaves, E. R., Korman, M. G. and Hansky, J. (1986). Campylobacter pyloridis in diseases of the human upper gastronintestional tract. Gastroenterology^,1509. -269. Crabtree, J. E., Figura, N., Taylor, J. D., Bugnoli, M., Armellini, D., and Tompkins, D. S. (1992). Expression of 120 kDa protein and cytotoxicity in Helicobacterpylori. J. Clin. Pathol. 45, 733-734.
. Crabtree, J. E., Wyatt, J. I., Sobala, G. M., Miller, G., Tompkins, D. S., Primrose, J. N., and Morgan, A. G. (1993). Systemic and mucosal humoral responses to Helicobacterpylori in gastric cancer. 11. Forman, D., Sitas, F., and Newell, D. G. (1990). Geographic association of Helicobacter pylori antibody prevalence and gastric cancer mortality in rural China. Int. J. Cancer 46, 608-611. 12. Forman, D., Newell, D. G., Fullerton, F., Yarnell, J. W. G.,Stacey, A. R., Wald, N., and Sitas, F. (1991). Association between infection with Helicobacter pylori and risk of gastric cancer *. evidence from a prospective investigation. BW302,1302-1305. 13. Nomura, A., Stemmermann, G. N., Chyou, P. H., Kato, I., Perez-Perez, G. I., and Blaser, M. J. (1991). Helicobacter pylori infection and gastric carcinoma amongst Japanese Americans in Hawaii, N. Engl. J. Med. 325, 1132-1136. 14. Paxsonnet, J., Friedman, G. D., Vandersteen, D. P. Chang, Y., Vogelman, J. H., Orentreich, N., and Sibley, R. K. (1991). Helicobacter pylori infection and the risk of gastric carcinoma. N. Engl. J. Med. 325,1127-1131.
. Forman, D. (1993). An international association between Helicobacter pylori infection and gastric cancer. The EUROGAST Study Group. Lancet 341,1359-1362. -2716. Blaser, M. J. (1992). Hypothesis on the pathogenesis and natural history of//i?/zcoZwcf^r/>y/i7ri-mduced inflammation. Gastroenterology 102, 720-727. 17. Taylor, D. N. and Blaser, M. J. (1991). Epidemiology of Helicobacter pylori infection. Epidemiol. Rev. 13,42-59. 18. Fan, X. J., Chua, A., Shahi, C. N., McDevitt, J., Keeling, P. W. N. and Kelleher, D. (1994) Gastric T lymphocyte responses to Helicobacter pylori colonisation. Gut 35,1379-1384. 19. Laemmli, U. K. (1970). Nature 227,680-685.
. MarkweU, M. A. K., Haas, S. M., Bieber, L. L. and Tolbert, N. E. (1978) Analytical Biochemistry, 87,206-210. 21. Matsudaira, P. T. (1989). A practical guide to protein and peptide purification for microsequencing. Academic Press, San Diego. 22. Lischwe, M. A. and Ochs, D. (1982). A new method for partial peptide mapping using N- chlorosuccinimide/urea and peptide silver staining in sodium dodecyl sulfate polyacrylamide gels. Analytical Biochemistry 127, 453-457. -28APPENDIX SEQUENCE LISTING (1) GENERAL INFORMATION (I) Applicant (A) Name: Rican Limited (B) Street: 1 Stokes Place, (C) City: Dublin 2, (D) Country: Ireland (E) Postal Code: (F) Telephone: 353 -1 - 2881230 (G) Telefax: 353 -1 - 2883439 (Π) Title of Invention: Heucobacter Proteins and Vaccines (HI) Number of Sequences: 6 (IV) (V) Current Application Data: Application No.: (2) INFORMATION FOR SEQUENCE ID. NO.: 1 (I) Sequence Characteristics (A) Length: 20 Amino Acids (B) Type: Amino Acid -29(C) Topology: Linear (II) Molecule Type: Protein (IV) Original Source: (A) Organism : Helicobacter pylori (XI) Sequence Description: SEP. ID. NO, 1 Met-Leu-Val-Thr-Lys-Leu-Ala-Pro-Asp-Phe-Lys-Ala-Pro-Ala-Val-Leu-Gly-Asn5 10 15 Asn-Glu (3) INFORMATION FOR SEQUENCE ID. NO. 2 : (I) Sequence Characteristics (A) Length: 20 Amino Acids (B) Type: Amino Acids (C) Topology: Linear (Π) Molecule Type: Protein (TV) Original Source : (A) Organism: Helicobacter pylori (XI) Sequence Description: SEP. ID. NO. 2 Met-Lys-Thr-Phe-Glu-Ile-Leu-Lys-His-Leu-Gln-Ala-Asp-Ala-Ile-Val-Leu-Phe5 10 15 Met-Lys -30(4) INFORMATIONFORSEQUENCEID.NO. :3 (I) Sequence Characteristics (A) Length: 20 Amino Acids (B) Type: Amino Acid (C) Topology: Linear (Π) Molecule Type: Protein (IV) Original Source : (A) Organism: Helicobacter pylori (XI) Sequence Description: SEP. ID. NO. 3 Asn-Val-Lys-Gly-Thr-Asp-Phe-Phe-Asn-Val-His-Lys-Ala-Thr-Glu-Glu-Ile-Tyr5 10 15 Glu-Glu (5) INFORMATION FOR SEQUENCE ID. NO.: 4 (Π) Sequence Characteristics (A) Length: 4 Amino Acids (B) Type: Amino Acid (C) Topology: Linear (Π) Molecule Type: Protein (V) Original Source: -31(A) Organism: Helicobacter pylori (XI) Sequence Description : SEP. ID, NO. 4.
Lys-Asp-Thr-Pro (6) INFORMATION FOR SEQUENCE ID. NO. 5 : (ΙΠ) Sequence Characteristics (A) Length: 21 Amino Acids (B) Type: Amino Acid (C) Topology : Linear (II) Molecule Type : Protein (VI) Original Source : (A) Organism: Helicobacter pylori (XI) Sequence Description: SEP. ID, NO. 5 Ile-Val-Leu-Phe-Met-Lys-Val-His-Asn-Phe-His-Trp-Asn-Val-Lys-Gly-Thr-Asp5 10 15 Phe-Phe-Asn (7) INFORMATION FOR SEQUENCE ID. NO.: 6 (TV) Sequence Characteristics (A) Length: 46 Amino Acids (B) Type: Amino Acid •Λ (Π) (VID -32(C) Topology: Linear Molecule Type: Protein Original Source: (A) Organism: Helicobacter pylori Met-Lys-Thr-Phe-Glu-Ile-Leu-Lys-His-Leu-Gln-Ala-Asp-Ala-Ile-Val-Leu-Phe5 10 15 Met-Lys-V al-His-Asn-Phe-His-Trp-Asn-Val-Lys-Gly-Thr-Asp-Phe-Phe-Asn-Val 20 25 30 35 His-Lys-Ala-Thr-Glu-Glu-Ile-Tyr-Glu-Glu 40 45

Claims (28)

1. A vaccine prepared for the treatment or prophylaxis of Helicobacter pylori infection or Helicobacter pylori associated disease, the vaccine comprising Helicobacter pylori protein or a derivative or fragment or mutant thereof to which immunoreactivity is detected in Helicobacter pylori negative individuals, the protein including one or both of a Helicobacter pylori protein having a molecular weight of 18 to 19 kDa and/or a Helicobacter pylori protein having a molecular weight of 24 to 25 kDa.
2. A vaccine as daimed in daim 1 wherein the immunoreactivity is antibody based.
3. A vaccine as claimed in daim 1 or 2, wherein the vaccine comprises Helicobacter pylori protein having a molecular weight of 18 to 19 kDa, or a derivative or fragment or mutant thereof.
4. A vaccine as claimed in daim 3, wherein the vaccine comprises Helicobacter pylori protein having a molecular weight of 18 to 19 kDa.
5. A vaccine as daimed in daim 3 or 4, wherein the 18 te 19 kDa protein has an N-terminal amino add sequence as listed in Sequence Id. No. 2, or a portion thereof.
6. A vaccine as claimed in daim 3, 4 or 5, wherein the 18 to 19 kDa protein has an internal amino add sequence as listed in Sequence Id. No. 3, or a portion thereof.
7. A vaccine as daimed in any of claims 3 to 6, wherein the 18 to 19 kDa protein has a N-terminal amino add sequence as listed in Sequence Id. No. 6, or a portion thereof. -348. A vaccine as claimed in any preceding claim, wherein die vaccine comprises Helicobacter pylori protein having a molecular weight of 24 to 25 kDa, or a derivative or fragment or mutant thereof.
8. 9. A vaccine as claimed in any preceding claim, wherein the vaccine comprises Helicobacter pylori protein having a molecular weight of 24 to 25 kDa.
9. 10. A vaccine as claimed in claim 8 or 9, wherein the 24 to 25 kDa protein has an N-terminal amino arid sequence as listed in Sequence Id. No. 1, or a portion thereof.
10. 11. A vaccine as claimed in claim 8, 9 or 10 wherein the 24 to 25 kDa protein has an internal amino arid sequence as listed in Sequence Id. No. 4, or a portion thereof.
11. 12. A vaccine as claimed in any preceding claim including a pharmaceutically acceptable carrier.
12. 13. A vaccine as claimed in any preceding claim in combination with a pharmacologically suitable adjuvant.
13. 14. A vaccine as claimed in claim 13 wherein the adjuvant is interleukin 12.
14. 15. A vaccine as claimed in claim 13 or 14 wherein the adjuvant is a heat shock protein.
15. 16. A vaccine as claimed in any preceding claim including at least one other pharmaceutical product.
16. 17. A vaccine as claimed in claim 16 wherein the pharmaceutical product is an antibiotic. -3518. A vaccine as claimed in claim 17 wherein the antibiotic is selected from one or more metronidazole, amoxycillin, tetracycline or erythromycin, clarithromycin or tinidazole. 5 19. A vaccine as claimed in any of claims 16 to 18 wherein the pharmaceutical product includes an antibiotic agent such as bismuth salts.
17. 20. A vaccine as claimed in any preceding claim in a form for oral administration.
18. 21. A vaccine as claimed in any of claims 1 to 19 in a form for intranasal administration.
19. 22. A vaccine as claimed in any of claims 1 to 19 in a form for intravenous 15 administration.
20. 23. A vaccine as claimed in any of claims 1 to 19 in a form for intramuscular administration. 20
21. 24. A vaccine as claimed in any of claims 1 to 19 including a peptide delivery system.
22. 25. The use of Helicobacter pylori protein or a derivative or fragment or mutant thereof, to which immunoreactivity is detected in Helicobacter pylori 25 negative individuals, the protein including one or both of a Helicobacter pylori protein having a molecular weight of 18 to 19 kDa and/or a Helicobacter pylori protein having a molecular weight of 24 to 25 kDa, in the preparation of a medicament for use in a method for the treatment or prophylaxis of Helicobacter pylori infection or Helicobacter pylori associated 30 disease in a host.
23. 26. The use as claimed in claim 25 wherein the medicament which is prepared is a vaccine as daimed in any of daims 2 to 24. -3627. A method for preparing a vaccine which treats or prevents Helicobacter pylori infection or Helicobacter pylori associated disease, the method comprising obtaining a Helicobacter pylori protein or a derivative or fragment or mutant thereof to which immunoreactivity is detected in Helicobacter pylori negative individuals, the protein including one or both of a Helicobacterpylori protein having a molecular weight of 18 to 19 kDa and /or a Helicobacter pylori protein having a molecular weight of 24 to 25 kDa; and forming a vaccine preparation comprised of said protein or derivative or fragment or mutant, which is suited for administration to a host and which when administered raises an immune response.
24. 28. A method as claimed in claim 27 wherein the medicament which is prepared is a vaccine as claimed in any of claims 2 to 24.
25. 29. Monoclonal or polyclonal antibodies or fragments thereof, to Helicobacter pylori protein or a derivative or fragment or mutant thereof, to which immunoreactivity is detected in Helicobacter pylori negative individuals, the protein including a Helicobacter pylori protein having a molecular weight of 18 to 19 kDa.
26. 30. Purified antibodies or serum obtained by immunisation of an animal with a vaccine according to any of claims 1 to 24.
27. 31. The use of the antibodies or fragments of claim 29 in die preparation of a medicament for treatment or prophylaxis of Helicobacter pylori infection or Helicobacter pylori associated disease.
28. 32. The use of the antibodies or serum of claim 30 in the preparation of a medicament for treatment or prophylaxis of Helicobacter pylori infection or Helicobacter pylori associated disease. -3733. Use of interleukin 12 as an adjuvant in Helicobacter vaccines.
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