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改进的重复元件PCR指纹图谱法用于解析大肠杆菌中的致病和非致病系统发育群体。

Improved repetitive-element PCR fingerprinting for resolving pathogenic and nonpathogenic phylogenetic groups within Escherichia coli.

作者信息

Johnson J R, O'Bryan T T

机构信息

VA Medical Center and Department of Medicine, University of Minnesota, Minneapolis, Minnesota, USA.

出版信息

Clin Diagn Lab Immunol. 2000 Mar;7(2):265-73. doi: 10.1128/CDLI.7.2.265-273.2000.

Abstract

Repetitive-element PCR (rep-PCR) fingerprinting is a promising molecular typing tool for Escherichia coli, including for discriminating between pathogenic and nonpathogenic clones, but is plagued by irreproducibility. Using the ERIC2 and BOXA1R primers and 15 E. coli strains from the ECOR reference collection (three from each phylogenetic group, as defined by multilocus enzyme electrophoresis [MLEE], including virulence-associated group B2), we rigorously assessed the effect of extremely elevated annealing temperatures on rep-PCR's reproducibility, discriminating power, and ability to reveal MLEE-defined phylogenetic relationships. Modified cycling conditions significantly improved assay reproducibility and discriminating power, allowing fingerprints from different cyclers to be analyzed together with minimal loss of resolution. The correspondence of rep-PCR with MLEE with respect to tree structure and regression analysis of distances was substantially better with modified than with standard cycling conditions. Nonetheless, rep-PCR was only a fair surrogate for MLEE, and when fingerprints from different days were compared, it failed to distinguish between different clones within all-important phylogenetic group B2. These findings indicate that although the performance and phylogenetic fidelity of rep-PCR fingerprinting can be improved substantially with modified assay conditions, even when so improved rep-PCR cannot fully substitute for MLEE as a phylogenetic typing method for pathogenic E. coli.

摘要

重复元件PCR(rep-PCR)指纹图谱是一种很有前景的用于大肠杆菌的分子分型工具,包括用于区分致病性和非致病性克隆,但存在重复性差的问题。使用ERIC2和BOXA1R引物以及来自ECOR参考菌株库的15株大肠杆菌(根据多位点酶电泳[MLEE]定义的每个系统发育组各3株,包括与毒力相关的B2组),我们严格评估了极高退火温度对rep-PCR的重复性、鉴别力以及揭示MLEE定义的系统发育关系能力的影响。改良的循环条件显著提高了检测的重复性和鉴别力,使得来自不同循环仪的指纹图谱能够一起分析,分辨率损失最小。与标准循环条件相比,改良条件下rep-PCR与MLEE在树形结构和距离回归分析方面的对应性要好得多。尽管如此,rep-PCR只是MLEE的一个相当的替代方法,当比较不同日期的指纹图谱时,它无法区分所有重要的系统发育组B2内的不同克隆。这些发现表明,尽管通过改良检测条件可以大幅提高rep-PCR指纹图谱的性能和系统发育保真度,但即使如此改进,rep-PCR仍不能完全替代MLEE作为致病性大肠杆菌的系统发育分型方法。

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