cagA genotype and variants in Chinese Helicobacter pylori strains and relationship to gastroduodenal diseases

doi:10.1099/jmm.0.05366-0

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cagA genotype and variants in Chinese Helicobacter pylori strains and relationship to gastroduodenal diseases

Jianchang Zhou^1,2,, Jianzhong Zhang¹, Caipu Xu² and Lihua He¹

¹National Institute for Communicable Disease Control and Prevention, Chinese Center for Disease Control and Prevention, 102206 Beijing, P.R. China ²Department of Gastroenterology, Southwest Hospital, Third Military Medical University, 400038 Chongqing, P.R. China

Correspondence Jianzhong Zhang helico{at}public.bta.net.cn

Received June 27, 2003
Accepted November 28, 2003

Previous studies have implicated CagA [encoded by cytotoxin-associatedgene A (cagA)] in Helicobacter pylori-associated gastroduodenalpathology and distinct subgenotypes of cagA may circulate indifferent pathological manifestations of cagA-positive H. pyloriinfection. To investigate cagA genotype and variants in ChineseH. pylori strains and explore their relationship with gastroduodenaldiseases, the cagA status of 82 Chinese H. pylori strains wasexamined and variation in size of the 3' region of cagA in 71of these strains was analysed by PCR. cagA was detected in 28(100 %) of 28 strains from peptic ulcer patients, two (100 %)of two strains from gastric cancer patients, 32 (94.1 %) of34 strains from chronic gastritis patients and 17 (94.4 %) of18 strains from healthy volunteers. PCR products of the cagA3' variable region were obtained from 71 (92.2 %) of 77 ChineseH. pylori strains and could be classified into subgenotypesI, II and III, which gave PCR products of around 825, 900 and950 bp, respectively. Subgenotype I cagA predominated in ChineseH. pylori strains (67/71), whereas subgenotype II cagA presentedin two isolates from patients with chronic gastritis and subgenotypeIII presented in two isolates from healthy volunteers. Therefore,neither cagA nor its 3' region variants can be used as a solemarker for the presence of particular H. pylori-related gastroduodenaldiseases in the Chinese population.

${dagger}$ Present address: Biochemistry Department, Third Military MedicalUniversity, 400038 Chongqing, P.R. China.

Abbreviation: cagA, cytotoxin-associated gene A.

INTRODUCTION

TOP
INTRODUCTION
METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

It is generally accepted that Helicobacter pylori strains thatproduce CagA, an antigenic outer-membrane protein of variablemolecular mass from 128 to 140 kDa, are highly virulent. Severalstudies have implicated CagA in the development of duodenalulcer and gastric adenocarcinoma in most western populations(Covacci et al., 1993; Blaser et al., 1995; Torres et al., 1998;Bach et al., 1999; Miehlke et al., 2000; Abasiyanik et al., 2002;Nomura et al., 2002a, b; Oliveira et al., 2003; Wu et al., 2003),whereas the majority of reports from east Asiancountries (Miehlke et al., 1996; Pan et al., 1997; Shimoyama et al., 1997;Maeda et al., 1998; Zheng et al., 2000; Groves et al., 2002;Lai et al., 2002), as well as those from Estonia(Andreson et al., 2002) and Argentina (Catalano et al., 2001),showed a very high prevalence of cagA-positive H. pylori, irrespectiveof clinical manifestation. Furthermore, it was reported thata PCR primer set that amplified cagA from H. pylori isolatedin one country failed to detect cagA in isolates from anothercountry (Miehlke et al., 1996; Pan et al., 1997). These discrepancieshave led to the hypotheses that there may be several distinctforms of CagA with an uneven geographical distribution, thatdifferences in cagA subgenotypes may provide a marker for differencesin virulence among cagA-positive H. pylori strains and thatonly some forms of CagA are associated with severe gastroduodenaldiseases.

cagA is noted for its sequence diversity, both within and outsidethe variable 3' region of the molecule. Repeat sequences inthe variable region are the major factor that contributes tothe size variation and antigenic heterogeneity of CagA (Covacci et al., 1993;Yamaoka et al., 1998, 1999). It was also reportedthat strains carrying cagA with a short variable 3' region weredistributed predominantly in Japanese, German and South Africanpatients with duodenal ulcers, and that those with the longestcagA variable 3' region were found more frequently in patientswith gastric cancer (Rudi et al., 1998; Yamaoka et al., 1998,1999; Kidd et al., 1999; Azuma et al., 2002). However, studiesconducted in Brazil (Rota et al., 2001) revealed that variable3' region subgenotypes did not relate to clinical outcome, eventhough the presence of multiple subgenotypes of cagA was associatedwith gastric ulcer incidence.

To determine whether cagA genotype and subgenotype are correlatedwith H. pylori-associated gastroduodenal diseases in China,cagA status was investigated in 82 Chinese H. pylori isolatesand cagA fragments (including the variable 3' region) of 77different Chinese H. pylori isolates were amplified and ampliconsize was compared.

METHODS

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INTRODUCTION
METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

H. pylori clinical strains.

Experiments were performed with 82 well-characterized clinicalH. pylori strains that were isolated from Chinese patients undergoingupper endoscopy, as well as the cagA-positive H. pylori referencestrain Sydney Strain 1 (SS1). These strains were obtained fromthe culture collection of the Institute for Infections DiseaseControl and Prevention, Chinese Center for Disease Control andPrevention.

H. pylori cultivation and DNA isolation.

H. pylori was cultured routinely on Columbia agar base (Oxoid)with 10 % sheep blood and Oxoid antibiotic supplement for 3days at 37 °C in a microaerophilic atmosphere (5 % O₂, 10% CO₂ and 85 % N₂). Bacteria were harvested and suspended in0.1 M NaCl, 10 mM Tris/HCl and 1 mM EDTA (pH 8.0), SDS (1 %,w/v) was added and the mixture was heated at 68 °C and thenextracted by the phenol/chloroform/isoamyl alcohol method.

PCR for determining cagA status and size variation of the cagA 3' variable region.

Primers cagAF (5'-GATAGGGATAACAGGCAAGC-3') and cagAR (5'-GGGGGTTGTATGATATTTTC-3'),which were designed to amplify a rather conservative 297 bpregion (nt 151–446 of cagA of strain NCTC 11638) thatwas revealed by aligning 54 cagA gene fragments deposited inGenBank, were used to investigate the cagA status of H. pyloristrains. Primers cagAVF (5'-CAAAAGATAACGG ATAAAGT-3') and cagAVR(5'-CTGTTAGTAGCGTAATTGTC-3'), which corresponded to nt 2335–2354and 3142–3161 of GenBank sequence AF202972, respectively,were used to amplify a fragment that included the cagA variable3' region. According to cagA sequences deposited in GenBank,the expected molecular size of the PCR product of this primerset is 818–1052 bp, depending on the number of repeatsand deletions present in the sequence of the gene. All PCR mixturesconsisted of 10 mM Tris/HCl (pH 8.3), 50 mM KCl, 1.5 mM MgCl₂,200 µM dNTPs, 25 pmol of each of the forward and reverseprimers, 0.05–0.1 ng H. pylori genomic DNA and 2 U Taqpolymerase (Sangon Biotechnological Co. Ltd, Shanghai, China)in a final volume of 50 µl. PCR was performed with a RoboCyclerGradient 40 PCR system (Stratagene) and comprised a preincubationof 3 min at 94 °C, 35 cycles of 1 min at 94 °C, 1 minat 54 °C and 1 min at 72 °C, and a final extension for5 min at 72 °C. PCR products were electrophoresed in 2.0% agarose gels and visualized by staining with ethidium bromideunder short UV light; molecular size of PCR products was estimatedby comparison with a 100 bp DNA ladder (fragment sizes, 100–1000bp in 100 bp increments), aided by scanning spectrophotometryusing SmartView 2001 software (version 5).

Statistical analysis.

Data were analysed by using a S² test. Probability levels (P)of < 0.05 were considered to be statistically significant.

RESULTS

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INTRODUCTION
METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

Properties of the study subjects

H. pylori strains were isolated from 82 Chinese patients. Pathologicalmanifestations of these patients were classified at the timeof endoscopy as peptic ulcer (n = 28), gastric cancer (n = 2),chronic gastritis (n = 34) and normal (n = 18). For analysisof size variation of the cagA 3' region, four strains isolatedfrom patients with chronic gastritis and one with peptic ulcerdisease were exempted from study, due to loss of these strainsduring subculture.

cagA status of Chinese H. pylori strains as determined by PCR

By using primers cagAF and cagAR to amplify the conservativecagA fragment, the expected PCR product of 297 bp was obtainedfrom 77 (93.9 %) of 82 Chinese clinical isolates, as well asfrom the positive control strain, SS1. Two strains that producedno 297 bp amplicon were verified to be cagA-positive by amplifyingthe variable 3' region of the cagA gene (Table 1). In all, 79(96.3 %) of 82 Chinese H. pylori strains were cagA-positive;prevalence of cagA in patients with severe gastroduodenal diseases(30/30, 100 %; two of two gastric cancer and 28 of 28 pepticulcer patients) was not found to be significantly higher thanin patients with gastritis (32 of 34, 94.1 %; P = 0.177) orhealthy volunteers (17 of 18, 94.4 %; P = 0.192).

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Table 1. cagA status of Chinese H. pylori strains, as determined by a PCR that detected a 297 bp consensus region (CR) and the 3' variable region (VR)

Size variation of the cagA 3' variable region of Chinese H. pylori strains

Amplification products of the fragment that included the variablecagA 3' region were obtained from 71 (92.2 %) of 77 DNA samples.Six samples that yielded no amplification products were excludedfrom further analysis. Molecular size of PCR products variedfrom around 825 bp, in 67 (94.4 %) Chinese H. pylori isolatesand SS1, to around 900 bp in two (2.8 %) isolates from patientswith chronic gastritis and around 950 bp in two (2.8 %) isolatesfrom healthy volunteers, which were classified as subgenotypesI, II and III, respectively (Fig. 1, Table 2). These 3' variableregion subgenotypes did not show a significant association withspecific gastroduodenal disease (P = 0.125).

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Fig. 1. cagA subgenotypes, as revealed by 2.0 % agarose gel electrophoresis, of PCR products of the fragment that included the variable 3' region. PCR products from a representative group of strains are shown. Lane 1, 100 bp DNA ladder (100–1000 bp in 100 bp increments); lanes 2–5, subgenotype I cagA with a PCR product of around 825 bp; lanes 6–7, subgenotype II cagA with a PCR product of around 900 bp; lane 8, subgenotype III cagA with a PCR product of around 950 bp.

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Table 2. Relationship between cagA 3' variable region subgenotypes and H. pylori-related diseases

DISCUSSION

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INTRODUCTION
METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

The first question posed in this study was whether cagA correlatedwith development of severe gastroduodenal diseases in China.Most of the Chinese H. pylori strains were cagA-positive (79/82,96.3 %), irrespective of gastroduodenal pathology; this providesfurther confirmation that cagA is not reliable for discriminatingspecific gastroduodenal disease-associated H. pylori strainsin China (Pan et al., 1997; Groves et al., 2002; Lai et al., 2002).The fact that two of five strains that were not detectableby cagAF and cagAR were verified to be cagA-positive by amplifyingfragments that included the cagA 3' variable region showed thatthe sensitivity of PCR methods for detecting cagA may be crucialfor determining cagA status and its variants, especially whenH. pylori strains are isolated from different populations ordifferent geographical regions. This is in agreement with theresults reported by Miehlke et al. (1996) and Pan et al. (1997).

When determining the size variation of fragments that includedthe cagA 3' variable region, primer cagAVF located 168, 165nt upstream from the forward primers and cagAVR located 11,95 nt downstream from the reverse primers, which were reportedby Yamaoka et al. (1998) and Rudi et al. (1998), respectively,were used to amplify this fragment, as computer-assisted alignmentof cagA sequences deposited in GenBank revealed a 39 nt deletionupstream of the former forward primers and several nucleotidesubstitutions in the former reverse primers in several AsiancagA sequences; therefore, the PCR products obtained with ourprimers may be 179 or 218 bp longer than those amplified withthe primer set of Yamaoka et al. (1998) and 260 or 299 bp longerthan those amplified with the set of Rudi et al. (1998), dependingon the 39 nt deletion. cagA subgenotypes I (around 825 bp) andIII (around 950 bp) in the present study correspond to typesA (642–651 bp) and B/D (756 bp) in Japanese H. pyloristrains (Yamaoka et al., 1998) and to those with a PCR productof 552–558 or 654–660 bp in German H. pylori strains(Rudi et al., 1998), respectively. No subgenotype correspondingto subgenotype II was found in previous reports and no subgenotypecorresponding to that with a PCR product of 450 bp in Germany(Rudi et al., 1998) was found in our strains or Japanese strainsfrom a previous study (Yamaoka et al., 1998), so there may beat least six variants of the cagA 3' region circulating in theworld.

As shown by our results, cagA of subgenotype I (67/71, 94.3%) predominated in Chinese H. pylori strains, which is consistentwith the distributions in Korea (124/128, 96.9 %) and Japan(145/155, 93.5 %) (Yamaoka et al., 1998, 1999), implying thatsimilar cagA subgenotypes may circulate in adjacent geographicalareas. It is interesting that the correlation of cagA subgenotypeC Japanese H. pylori strains with gastric cancer has not beenfound in our isolates or in Korean strains (Yamaoka et al., 1999);as only two strains isolated from gastric cancer werestudied and not all gastric cancer-associated H. pylori strainscarry subgenotype C cagA, this subgenotype may have been excludedfrom our study, although it may be the case that there was nosubgenotype C cagA in our, or Korean, H. pylori strains. Thus,our data did not show that the fragment length of the cagA 3'region correlates with disease in our population. We did notobserve multiple cagA subgenotypes to be present in ChineseH. pylori strains; this finding is in agreement with that inKorean strains (Yamaoka et al., 1999), whereas it is in contrastto the previous finding that multiple cagA subgenotypes weresignificantly more frequent in gastric cancer cases in the USA(Yamaoka et al., 1999) and peptic ulcer cases in Brazil (Rota et al., 2001).One possible reason may be that we have underestimatedthe occurrence of multiple cagA subgenotypes, as only a singlebiopsy was used in our study and a specific cagA subgenotypemay become predominant during H. pylori subculture, or templatecompetition may have occurred during the PCR amplification process.Therefore, to completely elucidate whether specific cagA subgenotypescorrelate to H. pylori-associated diseases, it will be necessaryto further test the cagA subgenotypes of H. pylori strains,especially those isolated from patients with gastric canceror peptic ulcer disease in different geographical regions, aswell as different isolates from one patient.

ACKNOWLEDGEMENTS

TOP
INTRODUCTION
METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

This work was supported by the Chinese National Natural ScienceFoundation, grant no. 39870032.

REFERENCES

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INTRODUCTION
METHODS
RESULTS
DISCUSSION
ACKNOWLEDGEMENTS
REFERENCES

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