AIM:To evaluate the utility of the string test to detect genotypic clarithromycin-resistant Helicobacter pylori (H.pylori)by polymerase chain reaction(PCR)-restriction fragment length polymorphism.METHODS:Patients und...AIM:To evaluate the utility of the string test to detect genotypic clarithromycin-resistant Helicobacter pylori (H.pylori)by polymerase chain reaction(PCR)-restriction fragment length polymorphism.METHODS:Patients undergoing endoscopic examinations were enrolled in the present study.String tests were done on the next day of endoscopy.Segments of 23S rRNA were amplified from DNA obtained from string tests.PCR-restriction fragment length polymorphism was accomplished by restriction enzymes BbsI and BsaI recognizing the mutation site A to G at 2143or at 2142 of 23S rRNA domain V,respectively.RESULTS:One hundred and thirty-four patients with H.pylori infection underwent string tests.To compare phenotypic resistance,43 isolates were successfully cultured in 79 patients in whom 23S rRNA was successfully amplified.Of five patients with clarithromycinresistant H.pylori,23S rRNA of H.pylori isolates from four patients could be digested by BsaI.In 38 susceptible isolates,23S rRNA of H.pylori isolates from 36 patients could not be digested by either BsaI or BbsI.The sensitivity and specificity of the string test to detect genotypic clarithromycin resistance were 66.7%and97.3%,respectively.Positive and negative predictive values were 80%and 94.7%,respectively.CONCLUSION:String test with molecular analysis is a less invasive method to detect genotypic resistance before treatment.Further large-scale investigations are necessary to confirm our results.展开更多
基金Supported by Grants from National Science Council of Republic of China,No.NSC96-3111-P-042A-004-Y and No.NSC972314-B-037-047-MY3from Kaohsiung Medical University Hospital,No.KMUH97-7R32 and No.KMUH97-7G49
文摘AIM:To evaluate the utility of the string test to detect genotypic clarithromycin-resistant Helicobacter pylori (H.pylori)by polymerase chain reaction(PCR)-restriction fragment length polymorphism.METHODS:Patients undergoing endoscopic examinations were enrolled in the present study.String tests were done on the next day of endoscopy.Segments of 23S rRNA were amplified from DNA obtained from string tests.PCR-restriction fragment length polymorphism was accomplished by restriction enzymes BbsI and BsaI recognizing the mutation site A to G at 2143or at 2142 of 23S rRNA domain V,respectively.RESULTS:One hundred and thirty-four patients with H.pylori infection underwent string tests.To compare phenotypic resistance,43 isolates were successfully cultured in 79 patients in whom 23S rRNA was successfully amplified.Of five patients with clarithromycinresistant H.pylori,23S rRNA of H.pylori isolates from four patients could be digested by BsaI.In 38 susceptible isolates,23S rRNA of H.pylori isolates from 36 patients could not be digested by either BsaI or BbsI.The sensitivity and specificity of the string test to detect genotypic clarithromycin resistance were 66.7%and97.3%,respectively.Positive and negative predictive values were 80%and 94.7%,respectively.CONCLUSION:String test with molecular analysis is a less invasive method to detect genotypic resistance before treatment.Further large-scale investigations are necessary to confirm our results.