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. 1998 Apr;36(4):944-8.
doi: 10.1128/JCM.36.4.944-948.1998.

Diversity of Helicobacter pylori vacA and cagA genes and relationship to VacA and CagA protein expression, cytotoxin production, and associated diseases

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Diversity of Helicobacter pylori vacA and cagA genes and relationship to VacA and CagA protein expression, cytotoxin production, and associated diseases

J Rudi et al. J Clin Microbiol. 1998 Apr.

Abstract

The vacuolating cytotoxin and the cytotoxin-associated protein, encoded by vacA and cagA, respectively, are important virulence determinants of Helicobacter pylori. Sixty-five H. pylori strains were isolated from dyspeptic patients (19 with peptic ulcer disease, 43 with chronic gastritis, and 3 with gastric cancer) and studied for differences in the vacA and cagA genes and their relationship to VacA and CagA expression, cytotoxin activity, and the clinical outcome of infection. By PCR, fifty-four (83.1%) of 65 strains had the vacA signal sequence genotype s1 and only 10 (15.4%) had the type s2. After primer modification, the vacA middle-region types m1 and m2 were detected in 24 (36.9%) and 41 (63.1%) strains, respectively. The combinations s1-m2 (31 [47.7%]) and s1-m1 (23 [35.4%]) occurred more frequently than s2-m2 (10 [15.4%]) (P = 0.01). No strain with the combination s2-m1 was found. All 19 patients with peptic ulcers harbored type s1 strains, in contrast to 32 (74.4%) of 43 patients with gastritis (P = 0.02). The vacA genotype s1 was associated with the presence of cagA (P < 0.0001), VacA expression (P < 0.0001), and cytotoxin activity (P = 0.003). The cagA gene was detectable in 48 (73.8%) of 65 isolates and present in 16 (84.2%) of 19 ulcer patients and 29 (67.4%) of 43 patients with gastritis (P = 0.17). The vacA genotypes of German H. pylori isolates are identical to those previously reported. H. pylori strains of vacA type s1 are associated with the occurrence of peptic ulceration and the presence of cagA, cytotoxin activity, and VacA expression.

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Figures

FIG. 1
FIG. 1
PAGE after PCR amplification of H. pylori DNA using primers vac1F-vac1R and NlaIII digestion. Only DNA amplicons obtained with vacA genotype s1 are cut by NlaIII into fragments of 107 and 94 bp. Lanes: M, 100-bp DNA marker; 1, strain H. pylori 60190 (vacA genotype s1); 2, Tx30a (vacA genotype s2); 3 to 8, type s1 isolates; 9 to 11, type s2 isolates. (The photographs in this and subsequent figures were scanned with a Hewlett-Packard Scan Jet 4c using the PaperPort Software Version 3.0.1 for Windows [Visioneer Communications, Inc.])
FIG. 2
FIG. 2
PAGE after PCR amplification of H. pylori DNA using primers vac3F-vac3R (a) and vac4F-vac4R (b). Lanes: M, 100-bp DNA marker; 1 to 11, H. pylori strains as described in the legend to Fig. 1.
FIG. 3
FIG. 3
PAGE after PCR amplification of H. pylori DNA using primers cag1-cag3. Lanes: M, 100-bp DNA marker; 1 to 11, H. pylori strains as described in the legend to Fig. 1.
FIG. 4
FIG. 4
PAGE after PCR amplification of H. pylori DNA using primers cag2-cag4. Lanes: M, 100-bp DNA marker; 1 to 11, H. pylori strains as described in the legend to Fig. 1. Note the size variation of DNA amplicons of different H. pylori strains.

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