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多重 PCR 快速检测霍乱弧菌 7 次大流行变异株中的基因组岛、噬菌体和整合性接合元件。

Rapid detection by multiplex PCR of Genomic Islands, prophages and Integrative Conjugative Elements in V. cholerae 7th pandemic variants.

机构信息

Dipartimento di Biologia e Biotecnologie Charles Darwin, Sapienza Università di Roma, Via dei Sardi 70, 00185, Rome, Italy.

出版信息

J Microbiol Methods. 2012 Jan;88(1):98-102. doi: 10.1016/j.mimet.2011.10.017. Epub 2011 Oct 28.

Abstract

Vibrio cholerae poses a threat to human health, and new epidemic variants have been reported so far. Seventh pandemic V. cholerae strains are characterized by highly related genomic sequences but can be discriminated by a large set of Genomic Islands, phages and Integrative Conjugative Elements. Classical serotyping and biotyping methods do not easily discriminate among new variants arising worldwide, therefore the establishment of new methods for their identification is required. We developed a multiplex PCR assay for the rapid detection of the major 7th pandemic variants of V. cholerae O1 and O139. Three specific genomic islands (GI-12, GI-14 and GI-15), two phages (Kappa and TLC), Vibrio Seventh Pandemic Island 2 (VSP-II), and the ICEs of the SXT/R391 family were selected as targets of our multiplex PCR based on a comparative genomic approach. The optimization and specificity of the multiplex PCR was assessed on 5 V. cholerae 7th pandemic reference strains, and other 34 V. cholerae strains from various epidemic events were analyzed to validate the reliability of our method. This assay had sufficient specificity to identify twelve different V. cholerae genetic profiles, and therefore has the potential to be used as a rapid screening method.

摘要

霍乱弧菌对人类健康构成威胁,到目前为止已经报告了新的流行变异株。第七次大流行的霍乱弧菌菌株具有高度相关的基因组序列,但可以通过大量基因组岛、噬菌体和整合性 conjugative 元件来区分。经典的血清分型和生物分型方法不容易区分全球出现的新变体,因此需要建立新的方法来识别它们。我们开发了一种多重 PCR 检测方法,用于快速检测主要的第七次大流行霍乱弧菌 O1 和 O139 变体。根据比较基因组学方法,选择了三个特定的基因组岛(GI-12、GI-14 和 GI-15)、两个噬菌体(Kappa 和 TLC)、霍乱弧菌第七次大流行岛 2(VSP-II)和 SXT/R391 家族的 ICEs 作为我们多重 PCR 的靶标。对 5 株第七次大流行的霍乱弧菌参考菌株进行了多重 PCR 的优化和特异性评估,并对其他 34 株来自不同流行事件的霍乱弧菌菌株进行了分析,以验证我们方法的可靠性。该检测方法具有足够的特异性来识别 12 种不同的霍乱弧菌遗传特征,因此具有作为快速筛选方法的潜力。

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