Affiliation:
1. Department of Experimental Medicine and Biochemical Sciences
2. Clinical Microbiology Laboratories, Policlinic of Tor Vergata, 00133 Rome
3. Department of Biology
4. Department of Internal Medicine, “Tor Vergata” University of Rome
5. Clinica San Raffaele, Velletri, Italy
Abstract
ABSTRACT
The recognition of the role of
Helicobacter pylori
in gastric diseases has led to the widespread use of antibiotics in the eradication of this pathogen. The most advocated therapy, triple therapy, often includes clarithromycin. It is well known that clarithromycin resistance is one of the major causes of eradication failure. The development of a rapid noninvasive technique that could easily be performed on fecal samples and that could also provide information about the antibiotic resistance of this microorganism is therefore advisable. Previous findings have demonstrated that clarithromycin resistance is due to a single point mutation in the 23S rRNA. All the mutations described have been associated with specific restriction sites, namely
Bsa
I (A2143G),
Mbo
II (A2142C/G), and
Hha
I (T2717C). On this basis we have developed a new method, a seminested PCR, allowing screening for clarithromycin resistance of
H. pylori
directly on stool samples. This method furnished a 783-bp fragment of the 23S rRNA, which was subsequently digested by
Mbo
II,
Bsa
I, and
Hha
I, in order to identify single point mutations associated with clarithromycin resistance. Of a total of 283 stool samples examined, 125 were
H. pylori
positive and two of them were shown to contain clarithromycin-resistant strains due to the presence of a mutation at position 2717, whereas no PCR products contained mutations at position 2142 or 2143. In order to evaluate the reliability of the new system, we compared the results of restriction analysis of the PCR products with the MICs shown by the
H. pylori
isolates by culturing gastric biopsies from the same patients.
Publisher
American Society for Microbiology
Cited by
36 articles.
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