Intragenomic recombination between babA and babB mediates antigenic variations and may help H. pylori colonization. This study determined whether variable genotypes of babA and babB correlate to different clinical disease outcomes, and can distribute over the different gastric niches.
This study enrolled 92 clinical strains (45 from peptic ulcer, 27 from gastritis, and 20 from gastric cancer) to detect whether the babA and babB are at locus A or B by PCR reactions using the primers designed from the upstream and variable region of the babA and babB genes. Four genotypes of babA and babB (A B, AB B, A AB, AB AB) were found. The distribution of the 4 genotypes in 92 clinical strains was significantly different among patients with different gastric diseases (p < 0.05). The isolates from gastric cancer patients had a higher rate of AB AB genotype than those from non-cancer patients (40.0% vs. 9.7%, p < 0.05). The AB AB genotype was associated with a higher intensity of intestinal metaplasia (p < 0.05), but did not correlate with a higher inflammation and colonization density in gastric histology (p > 0.05). Besides, the study enrolled 19 patients to verify whether variable genotypes of babAB existed in the different gastric niches. Among the patients infected with more than one babAB genotypes over antrum and corpus, there were higher rate of genotypes as A B or AB AB in isolates from antrum than in those from corpus (75.0 % vs. 16.7%, p < 0.05).
The H. pylori isolate with the AB AB genotype correlates with an increased gastric cancer risk, and colonize in an antrum predominant manner.
Helicobacter pylori infection increases the risk of peptic ulcers and gastric adenocarcinoma of the human stomach [1-3]. H. pylori adherence to the gastric epithelium and deliver effectors to induce inflammation [4,5]. One of the best-studied adhesins is the blood group antigen binding adhesin (BabA), which binds Lewis b (Leb) and related ABO antigens [6,7]. Putative adhesin, BabB, is encoded by babB, which shares nearly identical N- and C-terminal sequences with babA[7,8]. The reversed chromosomal locations of babA and babB between strain J99 and 26695 prove the recombination events between these two genes [9,10]. The two genes also show both geographic and allelic variation . Moreover, the duplication of babA or babB gene is mediated by gene conversion between the different chromosomal loci [12-14]. Bäckström et al.  demonstrated that the silent babA gene of a Leb-nonbinding strain can be activated by recombination into the babB gene. The rhesus monkey model showed that most recovered isolates have replaced babA with a second copy of babB after several weeks of infection .
In western countries, patients infected with babA-positive H. pylori isolates are associated with an increased risk of peptic ulcer diseases [15,16]. However, this association is not confirmed in patients from the Eastern Asia, or some other western countries [17-19]. Colbeck et al.  used PCR to detect whether the downstream of hpyD (locus A) and s18 (locus B) are babA or babB and found single-colony isolate with mixed babA and babB genotype at the same locus, indicating subpopulations within the bacterial population derived from a single colony. It is worthy to answer whether the genetic profiles of babA and babB could be related to the different clinical disease outcomes or the specific H. pylori-related histological features.
There are different predominant cell types in the antrum and corpus. The parietal cells producing HCl locate in the corpus and make a different pH gradient to the antrum. Our previous study showed patients with chronic H. pylori infection expressed a higher intensity of Lewis b in the gastric epithelium of corpus than in the antrum . Recombination between babA and babB might help H. pylori to change its adhesion ability to adapt different niches within the stomach . Accordingly, it is worthy to determine the genotype distribution of babA and babB in the H. pylori infection over the different topographic locations as either antrum or corpus in human stomach. In this study, we analyzed the clinical significance of babA and babB genotypes and the presence of babA and babB at locus A and B of multiple colonies from different gastric niches to understand the babAB genetic profile of H. pylori isolates across gastric regions within the same host.
Distributions of babA and babB genotypes in patients with different clinical diseases
Detection of babAB genotypes was based on the primer design shown in Figure 1. Among 92 strains, the distribution of the four genotypes (A B, AB B, A AB and AB AB) was 46 (50%), 21 (22.8%), 10 (10.9%), and 15 (16.3%), respectively. There was no difference in the gender distribution among the different genotypes (Chi-square test, p > 0.05). The mean age of patients infected with genotype as AB AB was marginally older than those infected with other genotypes (57.6 vs. 50.3 years, Independent-sample t test, p = 0.09). The distributions of the four genotypes were significantly different in the patients with different clinical diseases (Table 1, Chi-square test, p = 0.04). The mean age of GC patients was higher than the other non-cancer patients (58.6 vs. 49.5 years, Independent-sample t test, p = 0.01). The rate of the AB AB genotype in the patients with GC was higher than that in the three groups of non-cancer patients (40.0% [8/20] vs. 9.7% [7/72], Fisher exact test, p < 0.05, odds ratio: 6.2; 95%CI: 1.9-20.3).
Table 1. ThebabAandbabBgenotypes ofH. pylorifrom different clinical patient groups
As the AB AB genotype was higher in the patients with gastric cancer, we further tested whether such a genotype may lead to a higher rate of precancerous changes or more severe histological inflammation. In the patients with GC, the AB AB genotype was associated with a higher intensity of intestinal metaplasia (IM) in the antrum compared to non-AB AB genotype (2.0 vs. 0.27, p = 0.02). However, in the non-cancer patients, the AB AB genotype wasn’t associated with higher acute inflammation scores (sum of antrum, corpus and cardia: 3.43 vs. 2.94, p > 0.05), chronic inflammation scores (sum of antrum, corpus and cardia: 7.29 vs. 7.22, p > 0.05), H. pylori density (sum of antrum, corpus and cardia: 8.14 vs. 8.84, p > 0.05), or the intensity of IM (0.43 vs. 0.51, p > 0.05) compared to non-AB AB genotype.
Difference in the babA and babB genotype between isolates from antrum and corpus
For the 19 patients who provided isolates from different gastric niches over the antrum and corpus, the genotype composition of babA and babB at locus A and B of their antrum and corpus isolates is shown in Table 2. Four patients (no. 7, 12, 29, 30) were infected with an A B genotype strain across the antrum and corpus, and 15 patients were found to have a mixed genotype strains (AB B, A AB or AB AB) in only the corpus, or both gastric niches. In those 15 patients, 3 patients (no. 28, 2, 4) had the same mixed genotypes across the antrum and corpus. Eight of remaining 12 patients had one major genotype across both gastric niches. Combining with the 7 patients (no. 7, 12, 29, 30, 28, 2, 4) with only one genotype, 78.9% (15/19) of our patients had one major genotype distributed across two niches.
Table 2. The genotype compositions of antrum and corpusH. pyloriisolates from 19 patients
Among those 12 patients infected with more than one genotype (Table 2), the frequency of the major dominant genotype, A B combined with AB AB, in the antrum was higher compared with that in the corpus (75% [9/12] vs. 16.2% [2/12], p = 0.012, odds ratio: 15). However, 6 of 12 patients lacked a dominant genotype in their corpus isolates.
Sequence analysis and comparison
At locus A, each patient’s antrum and corpus isolates had specific substitutions of amino acids in the region of BabA (Figure 2 and Table 3). However, there was no obvious difference between the antrum and corpus isolates in the sequencing region, except from patient no. 27 (amino acid 134 and 198). We also found 5 different nonsynonymous substitutions at amino acid 161 in 6 patients’ isolates, as compared with strain J99. The same scenario (sequence specificity in individual patients’ strains but not between the antrum and corpus isolates) was in the babB sequences.
Figure 1. PCR banding patterns of babAB genotypes. (A) Primer pairs used for gene detection at locus A and B. The forward primers, HypDF1 and S18F1, located in the upstream region of babA or babB, are paired with BabAR1 or BabBR1 primers to determine whether the gene at locus A and B is babA or babB. (B) PCR banding patterns of genotype A B, AB B, A AB and AB AB. The AB B genotype showed two bacterial populations in the single-colony isolate, the dominant as babA and the minor as babB, at locus A. The strain with A AB genotype represented a dominant population of babB and a minor population of babA at locus B. The combination of AB B and A AB was defined as an AB AB genotype. Lane M1, a 100 bp molecular marker; lane M2, l HindIII marker. The size of PCR products at locus A and B was 2.1-2.6 kb and 1.0-1.5 kb, respectively.
Table 3. The amino acid substitutions in BabA encoded bybabAat locus A
CT repeats of babA and babB at locus B
Genes at locus B are regulated by CT repeats in the 5’ coding region, and the number of CT repeats (5, 8 and 11) make in-frame protein expression possible [12,20]. The CT repeats of the babB gene at locus B are shown in Table 4. The corpus isolates in 7 of 12 patients had a change of CT repeats of the babB gene at locus B, and antrum isolates of those patients always have the same CT repeats, except patient 17 (Table 4).
Table 4. The number of CT repeats in the 5’ coding region ofbabBat locus B
Genotype and BabA expression
To determine the effect of babA at locus A and B on BabA expression (Figure 3A), we found that the babA at locus B didn’t obviously affect the level of BabA expression, when compared to the isolates 19C3 (A AB) and 19C1 (A B). All the isolates (26A1, A4, C2 and C3) had the A AB genotype, but the CT repeats of the babA at locus B of C2 was out of frame. The expression of BabA was not affected by whether babA at locus B was in or out of frame. We further determined whether a mixed genotype at locus A would affect BabA expression, and found 14C2 and 14C3 with the AB B genotype (BabA/Hsp60 ratio: 0.76 and 0.70) had slightly lower expression than 14A2 and 14A4 with the A B genotype (BabA/Hsp60 ratio: 0.90 and 0.87, Figure 3B). AB AB genotype also had the lower BabA expression than A B (BabA/Hsp60 ratio: 1.09 and 0.89, Figure 3C).
Figure 2. The babA sequences at locus A of the antrum and corpus isolates. Cardinal numbers indicate different patients’ isolates. A1-4 and C1-4 were single-colony isolate isolated from the antrum and the corpus, respectively. White highlighting indicates amino acids different from consensus.
The occurrence of intragenomic recombination between babA and babB has been demonstrated in in vitro and in vivo experiments, implicating this mechanism may possibly assist H. pylori to adapt in the human stomach [12,14]. In addition, mixed genotypes of babA and babB at locus A or B have been demonstrated . The clinical association of the babA and babB genotype of H. pylori strains and genetic profile with infections of the antrum and corpus of a single host are still unclear. In this study, we demonstrated that the AB AB genotype, one dominant genotype in the antrum, was associated with the precancerous lesion as IM, and correlated with gastric cancer. However, H. pylori infection by such AB AB genotype has not lead into a more dense colonization or inflammation severity in gastric histology. Our data indicate H. pylori babA and babB genotypes as AB AB should at least exert with better adaptation to gastric environment during carcinogenesis.
Colbeck et al.  found 9 genotypes (A B, AB B, A AB, A A, B B, B A, B C, C B and B AB) in their study. Nevertheless, our study only found four genotypes (A B, A AB, AB B and AB AB) in the 168 isolates from 19 patients’ antrum and corpus (Table 2). It indicates the genotype diversity of babAB in Taiwanese isolates could be obviously less complicate. Moreover, at least one babA gene at locus A existed in each of the isolates. This finding is compatible with our previous report to reveal the Taiwanese H. pylori isolates are nearly 100% babA-positive , and support the higher prevalence of babA in H. pylori strains from East Asian countries than those from western worlds . Moreover, Matteo et al.  demonstrated that 9 of 34 patients (26.5%) had bab gene variation across the antrum and corpus of a single host at a specific time point. We found that 12 of 19 patients (63.2%) infected by more than one genotype in either one or both gastric niches. The prevalence discrepancy between two studies could be due to the analysis of bab genotype from the bacterial pool or single-colony isolate.
Analysis of the sequences of babA and babB revealed that nonsynonymous substitutions of amino acids occurred between the individual strains (Figure 2, Table 3 and data not shown), but did not differ between the gastric niches. Pride et al.  also showed high allelic diversity within babA and babB in the strains from different patients. Judging by the 6 different nonsynonymous substitutions of amino acid 161 in the 6 patients’ strains, that codon was a highly variable site. This is worth further investigation, as it may be a special site responsible for adapting to differences in individual stomachs.
CT repeats in the 5’ coding region of babA and babB are more commonly found at locus B than locus A . We found that the corpus isolates had a higher frequency of changes in number of CT repeats of babB at locus B than the antrum isolates (Table 4). Among those 7 patients infected by the corpus isolates with a change of CT repeats, only one (patient no. 27) had the isolate changing CT repeats to in-frame (CT = 8) (Table 4). This data indicates that BabB expression could be tightly controlled by phase variation due to out of frame repeats in the corpus. Among 12 patients infected by isolates with more than one genotype, their isolates from antrum have a higher rate of A B and AB AB as dominant genotypes than corpus (9/12 vs. 2/12, p < 0.05). Moreover, half of those patients lacked a dominant genotype in their corpus isolates. These results suggest the environment in the corpus may favor different adaptation for the isolates with different H. pylori genetic diversities.
The presence of the AB AB genotype was higher in GC patients with older age (Table 1). In addition, the AB AB genotype is not correlated with more severe inflammation or precancerous changes in the non-cancer patients. Based on this cross-sectional clinical histological data, it suggests the AB AB strains may have a better adaptation to the cancerous environment in stomach, instead of leading into more toxicity in gastric carcinogenesis. In Figure 3A, we show that the babA gene at locus A dominantly determines BabA expression, and the mixed genotype as AB at locus A may decrease the BabA expression (Figure 3B and 3C). It is thus possible a mixed genotype as AB at locus A may make H. pylori isolates to contain a subpopulation losing BabA expression. Alternatively, the mixed genotype as AB at locus B may possibly allow H. pylori to change BabB expression and thus deserves further study.
In addition, our previous data have shown that the intensity of Lewis b become decreased in antrum atrophy, but can be preserved in corpus to mediate higher colonization of bug overthere . So, it shall be also implicative to test whether the AB AB genotype dominantly in antrum can have advantage to adapt the gastric epithelium with weak Lewis b expression in future.
The H. pylori isolate with babA and babB genotype as AB AB genotype correlates with an increased gastric cancer risk, and colonize in an antrum predominant manner. Such AB AB genotype shall be associated with a better adaptation to the gastric precancerous or cancer environment, and possibly generate subpopulations losing BabA or BabB.
Patients and bacterial isolates
A total of 92 H. pylori strains were cultured from the biopsy specimens of patients with different clinical diseases as duodenal ulcer (DU, n = 18), gastric ulcer (GU, n = 27), gastritis (n = 27), or gastric cancer (GCA, n = 20), defined by endoscopy with histological confirmation. All patients had given informed consent and underwent panendoscopy in our institute. During panendoscopy for each patient, five bits of gastric biopsy, including 2 from the antrum, 2 from the corpus, and 1 from the cardia were obtained. The bacterial culture and histological examination were applied as the previous article . This study was approved by 'Human Experiment and Ethics Committee of National Cheng Kung University Hospital' (No. HR-98-023).
Single-colony isolates from the antrum and corpus were randomly picked from the primary culture plates. For each site, at least 3-4 single-colony isolates were randomly selected to determine the babAB genotype. Colony culture for DNA extraction was less than 8 passages to decrease the possibility of genetic variation in vitro. Each of the 19 patients infected in the antrum and corpus by isolates with the same RAPD banding pattern was described previously .
Detection of babA and babB genotypes
The detection of babA and babB genotypes was based on the method of Colbeck et al. HypDF1-BabAR1 and HypDF1-BabBR1 primers were used to determine whether the gene at locus A was babA or babB. In the same way, S18F1-BabAR1 and S18F1-BabBR1 primers were applied to determine whether the gene at locus B was babA or babB (Figure 1A). The 40 cycles of amplification reactions were performed with 20 pmoles of primer, 0.15 mM each deoxynucleoside triphosphate, reaction buffer with MgCl2 and 1 U Taq DNA polymerase (New England Biolabs, Beverly, MA, USA) in a final volume of 50 μl. The conditions of thermal cycling were described previously . Each amplified product (20 μl) was analyzed on a 1% agarose gel stained with ethidium bromide.
Figure 3. babAat locus A dominantly determined BabA expression. (A) Effect of babA at locus B on the BabA expression.The isolate (19C3) had babA at locus A and in-frame CT repeats of babA at locus B, which were compared with the isolate only having babA at locus A (19C1). The presence of babA at locus A and B was in the isolates 26A1, A4, C2 and C3, but C2 had an out of frame babA at locus B. (B) Effect of mixed genotype at locus A on the BabA expression. The isolates from one patient (no. 14) had a mixed genotype at locus A (14C2 and C3), which was compared with those with babA only at locus A (14A2 and A4). (C) Comparison of BabA between AB AB and A B genotypes. Hsp60 was as an internal control.
The babA and babB genotype of each single-colony isolate was based on the previous description . A J99-like isolate showed the expected PCR bands of babA at locus A and babB at locus B and was defined as the “A B genotype” (Figure 1B-a). A single-colony isolate containing both babA and babB at the same locus was defined as “mixed genotype” (such as AB B, A AB, and AB AB), indicating that there were subpopulations within the bacterial population derived from a single colony. An isolate with an AB B genotype contained one population with babA and the other population with babB at the same locus A (Figure 1B-b). The A AB genotype represented two bacterial populations, the dominant one with babB and the minor one with babA at locus B, although both derived from a single colony (Figure 1B-c). A mixed genotype detected at both locus A and B was defined as an AB AB (Figure 1B-d). A minor band from babB at locus B could be non-specific binding because its size is larger than the prediction.
The PCR products were sequenced by using either the BabAR1 or BabBR1 primer, depending on the amplification of babA or babB. The sequencing was conducted by the Mission Biotech Company, Taipei, Taiwan.
H. pylori grew for 2 days, was harvested, and suspended in ddH2O. We used the Bio-Rad Protein Assay (Bio-Rad Laboratories, Hercules, CA, USA) to determine and adjust protein concentration of each bacterial suspension. An equal amount (2μg) of bacterial protein was loaded to perform SDS-PAGE and a 1:2000 dilution of anti-BabA polyclonal antibody (Ab, a gift from Prof. Odenbreit) was used in a western blot . The detection of BabA protein was performed with Super Signal® West Pio Chemiluminescent substrate (Thermo Fisher Scientific Inc., Rockford, IL, USA) and exposed in an LAS-3000 imaging system (Fujifilm, Tokyo, Japan).
Statistical analysis was performed by the Chi-square test, Fisher exact test, Mann-Whitney U test and Student’s t test as appropriate. The difference was considered significant with a p value less than 0.05.
Dr. Sheu MS has made contributions to the experimental design, acquisition and analysis of data. Dr. Sheu BS and Dr. Wu JJ coordinated the conduct of the whole study and made interpretation of data. Chiang WC, Kao CY and Wu HM conducted the acquisition of data. Dr. Yang HB reviewed the pathology. All authors read and approved the final manuscript.
We thank Robert M. Jonas for his comments on this article. The study was financially supported in part by grants 98-2628-B-006-013-MY3 from the National Science Council, grant NHRI-EX99-9908BI from the National Health Research Institute, and grant DOH99-TD-C-111-003 from Department of Health, Taiwan.
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Clin Microbiol Infect 2009, 15:253-259. PubMed Abstract