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. 2011 Apr;105(3):251-9.
doi: 10.1179/136485911X12899838683485.

Characterisation of the genes encoding resistance to metronidazole (rdxA and frxA) and clarithromycin (the 23S-rRNA genes) in South African isolates of Helicobacter pylori

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Characterisation of the genes encoding resistance to metronidazole (rdxA and frxA) and clarithromycin (the 23S-rRNA genes) in South African isolates of Helicobacter pylori

N F Tanih et al. Ann Trop Med Parasitol. 2011 Apr.

Abstract

Helicobacter pylori has been incriminated in human diseases, such as peptic ulcer, gastritis and gastric malignancy. Although modern triple-drug regimens are usually highly effective in the treatment of H. pylori infection, the emergence of resistance to two of the most used antibiotics, metronidazole (Mtz) and clarithromycin (Cla), is a serious and increasing problem. Truncations in the rdxA and frxA genes of H. pylori are thought to be associated with Mtz resistance whereas mutations in the pathogen's 23S-ribosomal-RNA (23S-rRNA) genes are associated with Cla resistance. In a recent study, PCR and sequence analysis of the rdxA, frxA and 23S-rRNA genes were used to explore the genetic basis of resistance to Mtz and Cla in H. pylori. When 200 isolates of H. pylori from the Eastern Cape province of South Africa were tested for antibiotic susceptibility, almost all (95·5%) were found resistant to Mtz and 20·0% were found resistant to Cla. Only the Mtz-resistant isolates showed rdxA and frxA truncation. Two point mutations were detected in the 23S-rRNA genes of the Cla-resistant isolates. Many significant changes (resulting in 13 amino-acid substitutions in nine loci and truncated proteins in 14 loci) were observed in the rdxA genes of the Mtz-resistant isolates, and it appears that, compared with the rarer changes detected in frxA, such mutations may contribute more significantly to the high prevalence of Mtz resistance. To guide empiric treatment, the genotypes and antibiotic susceptibility of H. pylori in the Eastern Cape province of South Africa need to be monitored regularly.

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Figures

Figure 1
Figure 1
The results of the electrophoresis of the amplicons produced in PCR targeting the rdxA gene of Helicobacter pylori. The lanes contained a molecular-weight ‘ladder’ (L), the products from a negative-control reaction (lane 1) and samples produced from test isolates of H. pylori (lanes 2–10).
Figure 2
Figure 2
The results of the electrophoresis of the amplicons produced in PCR targeting the frxA gene of Helicobacter pylori. The lanes contained a molecular-weight ‘ladder’ (L), the products from a negative-control reaction (lane 1) and samples produced from test isolates of H. pylori (lanes 2–10).

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