Sensitive detection of Helicobacter pylori by using polymerase chain reaction.

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J Clin Microbiol. 1992 January; 30(1): 192-200

Sensitive detection of Helicobacter pylori by using polymerase chain reaction.

C L Clayton, H Kleanthous, P J Coates, D D Morgan and S Tabaqchali

Department of Medical Microbiology, St. Bartholomew's Hospital Medical College, London, United Kingdom.

ABSTRACT

A polymerase chain reaction (PCR) for the specific detectionof Helicobacter pylori was developed with a single primer pairderived from the nucleotide sequence of the urease A gene ofH. pylori. We achieved specific amplification of a 411-bp DNAfragment in H. pylori. After 35 cycles of amplification, theproduct could be detected by agarose gel electrophoresis andcontained conserved single HinfI and AluI restriction sites.This fragment was amplified in all 50 strains of H. pylori tested,but it was not detected in other bacterial species, showingthe PCR assay to be 100% specific. PCR DNA amplification wasable to detect as few as 10 H. pylori cells. PCR detected H.pylori in 15 of 23 clinical human gastric biopsy samples, whereasculturing and microscopy detected H. pylori in only 7 of thesamples found to be positive by PCR. Additional primer pairsbased on the urease genes enabled the detection of H. pyloriin paraffin-embedded human gastric biopsy samples. The detectionof H. pylori by PCR will enable both retrospective and prospectiveanalyses of clinical samples, elucidating the role of this organismin gastroduodenal disease.

J Clin Microbiol. 1992 January; 30(1): 192-200

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