Abstract
蔡庆,王蔚,陈友纯,林万明.三对引物同时PCR分型检测产毒素大肠杆菌的方法及在分子流行病学研究中的应用[J].Chinese journal of Epidemiology,1997,18(4):211-213
三对引物同时PCR分型检测产毒素大肠杆菌的方法及在分子流行病学研究中的应用
Study on the Molecular Epidemiology of Diarrhea Caused by Enterotoxigenic Escherichia coli, Using Polymerase Chain Reaction with Multiple Primer Pairs
Received:February 25, 1997  Revised:March 11, 1997
DOI:
KeyWord: 产毒素大肠杆菌  腹泻  聚合酶链反应
English Key Word: Enterotoxigenic Escherichia coli(ETEC)  Diarrhea  Polymerase chain reaction
FundProject:
Author NameAffiliation
Cai Qing Research Center of Clinical Molecular Biology, Genetal Hospital Air Force of PLA, Beijing 100036 
Wang Wei Research Center of Clinical Molecular Biology, Genetal Hospital Air Force of PLA, Beijing 100036 
Chen You-chun Research Center of Clinical Molecular Biology, Genetal Hospital Air Force of PLA, Beijing 100036 
林万明 Research Center of Clinical Molecular Biology, Genetal Hospital Air Force of PLA, Beijing 100036 
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Abstract:
      在产毒素大肠杆菌(ETEC)肠毒素基因内设计合成三对引物,建立了三对引物同时PCR检测ETEC的方法,一次PCR即可扩增出627bp (LTh)、240bp (STIa)和169bp (STIb)三种肠毒素基因片段,可同时分型检测出LTh、STIa、STIb、LTh-STIa、LTh-STIb五种基因型的ETEC,与非ETEC对照菌无交叉反应,最小检出量为10cfu,显示了很高的特异性和敏感性。将建立的方法用于山东省六县市623例大肠杆菌致泻标本的检测,阳性率为40.3%,并能鉴别ETEC的基因型,为ETEC腹泻的分子流行病学研究提供了有效的检测手段。
English Abstract:
      A Polymerase Chain Reaction (PCR) method has been developed for detecting Enterotoxigenic Escherichia coli (ETEC). Three different sets of oligonucleotide primer were simultaneously used to amplify the enterotoxin genes of heat-labile (LTh) and heat-stable (STIa and STIb) enterotoxins of ETEC. These primers amplified the 627, 240 or 169 base pair DNA fragments from LTh, STIa and STIb genes of the reference ETEC strains, respectively.Five types of ETEC strains corresponding to the LTh, STIa,STIb,LTh-STIa,or LTh-STIb genotypes were distinguished by a single procedure of PCR, using the mixture of the three sets of primers.There was no cross-reaction with the non-ETEC strains. The lowest detection level was 10 cfu. A total number of 623 stool specimens of diarrheal patients from Shangdong Province induced by E.coli were examined by PCR and the positive rate of ETEC was 40.3%. The results indicated that PCR is a rapid,sensitive and specific method for detecting ETEC.
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