首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Nucleotide sequence analysis of enteropathogenic Escherichia coli (EPEC) adherence factor probe and development of PCR for rapid detection of EPEC harboring virulence plasmids.
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Nucleotide sequence analysis of enteropathogenic Escherichia coli (EPEC) adherence factor probe and development of PCR for rapid detection of EPEC harboring virulence plasmids.

机译:肠道致病性大肠埃希菌(EPEC)粘附因子探针的核苷酸序列分析和PCR技术的开发可快速检测出带有毒力的EPEC质粒。

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摘要

The 1-kb BamHI-SalI fragment from plasmid pMAR2 termed the enteropathogenic Escherichia coli (EPEC) adherence factor (EAF) probe was cloned in pUC19 and pK18. The nucleotide sequence of this fragment was determined, and a set of primers was designed to amplify a 397-bp region associated with pMAR2 by PCR. An analysis of the whole EAF sequence with database libraries indicated no significant homology to any known genes. However, between bases 701 and 787 of the fragment, an 82.8% homology between the EAF and the insertion sequence IS630 of Shigella sonnei exists. The results of PCR with primers of the EAF sequence demonstrated that all of the 151 EAF probe-positive EPEC strains with localized adherence to HEp-2 cells yielded positive EAF PCR results. In contrast, none of the 277 EAF probe-negative strains reacted to the EAF PCR. In addition, the PCR assay was successfully used to generate vector-free digoxigenin-labeled EAF fragments that gave valid results in colony blot hybridization assays. The EAF PCR appears to be a specific and efficient method for the detection of EPEC strains carrying the EAF plasmids.
机译:将来自质粒pMAR2的1-kb BamHI-SalI片段克隆到pUC19和pK18中,该片段称为肠致病性大肠杆菌(EPEC)粘附因子(EAF)探针。确定了该片段的核苷酸序列,并设计了一组引物以通过PCR扩增与pMAR2相关的397bp区域。用数据库文库对整个EAF序列进行分析表明与任何已知基因均无显着同源性。然而,在该片段的碱基701和787之间,EAF和索氏志贺氏菌的插入序列IS630之间存在82.8%的同源性。用EAF序列引物进行PCR的结果表明,与HEp-2细胞局部粘附的所有151个EAF探针阳性EPEC菌株均产生阳性EAF PCR结果。相反,277个EAF探针阴性菌株均未对EAF PCR反应。此外,PCR分析已成功用于产生不含载体的洋地黄毒苷标记的EAF片段,该片段在菌落印迹杂交分析中给出了有效的结果。 EAF PCR似乎是检测携带EAF质粒的EPEC菌株的一种特定而有效的方法。

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