Rapid detection of clarithromycin resistance in Helicobacter pylori using a PCR-based denaturing HPLC assay

doi:10.1093/jac/dki406

JAC Advance Access originally published online on November 11, 2005
Journal of Antimicrobial Chemotherapy 2006 57(1):71-78; doi:10.1093/jac/dki406

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© The Author 2005. Published by Oxford University Press on behalf of the British Society for Antimicrobial Chemotherapy. All rights reserved. For Permissions, please e-mail: journals.permissions@oxfordjournals.org

Rapid detection of clarithromycin resistance in Helicobacter pylori using a PCR-based denaturing HPLC assay

Patrizia Posteraro¹, Giovanna Branca², Maurizio Sanguinetti²^,*, Stefania Ranno², Giovanni Cammarota⁴, Siavash Rahimi³, Mario De Carlo¹, Brunella Posteraro² and Giovanni Fadda²

¹ Laboratory of Clinical Pathology and Microbiology, Ospedale San Carlo-Istituto Dermopatico dell'Immacolata, Rome, Italy; ² Institute of Microbiology, Università Cattolica del Sacro Cuore, Rome, Italy; ³ Service of Histopathology, Ospedale San Carlo-Istituto Dermopatico dell'Immacolata, Rome, Italy; ⁴ Department of Internal Medicine and Gastroenterology, Università Cattolica del Sacro Cuore, Rome, Italy

Received 10 August 2005; returned 9 September 2005; revised 30 September 2005; accepted 10 October 2005

^* Corresponding author. Tel: +39-6-30154964; Fax: +39-6-3051152; E-mail: msanguinetti{at}rm.unicatt.it

Objectives: We evaluated a new approach for the rapid detectionof clarithromycin resistance in Helicobacter pylori, based onPCR and denaturing HPLC (DHPLC).

Methods: A 180 bp fragment of the 23S rRNA gene was amplifiedusing DNA from 81 clinical H. pylori isolates (51 isolates wereshown to be resistant to clarithromycin by Etest), and, directly,from 101 gastric biopsies from patients with digestive diseases,who were infected with H. pylori as assessed by a ¹³C-urea breathtest, histology and/or culture. DHPLC was used to detect mutationsin all the PCR products.

Results: DHPLC profiles for the 30 susceptible isolates allshowed homoduplex peaks; the resistant isolates consistentlygenerated heteroduplex peaks that were easily distinguishablefrom the wild-type H. pylori reference strain. Sequencing revealedpoint mutations in all the resistant isolates. Overall, fivedifferent mutations were detected. Four of these mutations (A2142G,A2142C, A2143G and T2182C) are known to be associated with clarithromycinresistance; the remaining mutation (C2195T) has not been previouslydescribed. This novel single-base substitution was found incombination with the common mutation A2143G. Of the biopsiestested, 25 specimens generated heteroduplexes due to sequencealterations (mutation A2142G, A2142C or A2143G). In one of thesespecimens, A2143G was found together with the novel mutationT2221C; in another, a mixture of wild-type and mutant (A2143G)sequences was detected. For 20 culture-positive out of the 25biopsies DHPLC results confirmed the presence of clarithromycinresistance.

Conclusions: Our results suggest that the PCR–DHPLC assayis a valid tool for rapid assessment of clarithromycin resistancein H. pylori and that in the future it could be used directlyon biopsy specimens, avoiding the need for culture-based methods.

Keywords: 23S rRNA gene , mutations , Etest

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