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利用全基因组系统发育和比较来开发多重PCR检测方法以鉴定36型副溶血性弧菌

Use of Whole-Genome Phylogeny and Comparisons for Development of a Multiplex PCR Assay To Identify Sequence Type 36 Vibrio parahaemolyticus.

作者信息

Whistler Cheryl A, Hall Jeffrey A, Xu Feng, Ilyas Saba, Siwakoti Puskar, Cooper Vaughn S, Jones Stephen H

机构信息

Department of Molecular, Cellular and Biomedical Sciences, University of New Hampshire, Durham, New Hampshire, USA Northeast Center for Vibrio Disease and Ecology, University of New Hampshire, Durham, New Hampshire, USA

Department of Molecular, Cellular and Biomedical Sciences, University of New Hampshire, Durham, New Hampshire, USA Northeast Center for Vibrio Disease and Ecology, University of New Hampshire, Durham, New Hampshire, USA.

出版信息

J Clin Microbiol. 2015 Jun;53(6):1864-72. doi: 10.1128/JCM.00034-15. Epub 2015 Apr 1.

Abstract

Vibrio parahaemolyticus sequence type 36 (ST36) strains that are native to the Pacific Ocean have recently caused multistate outbreaks of gastroenteritis linked to shellfish harvested from the Atlantic Ocean. Whole-genome comparisons of 295 genomes of V. parahaemolyticus, including several traced to northeastern U.S. sources, were used to identify diagnostic loci, one putatively encoding an endonuclease (prp), and two others potentially conferring O-antigenic properties (cps and flp). The combination of all three loci was present in only one clade of closely related strains of ST36, ST59, and one additional unknown sequence type. However, each locus was also identified outside this clade, with prp and flp occurring in only two nonclade isolates and cps in four. Based on the distribution of these loci in sequenced genomes, prp identified clade strains with >99% accuracy, but the addition of one more locus increased accuracy to 100%. Oligonucleotide primers targeting prp and cps were combined in a multiplex PCR method that defines species using the tlh locus and determines the presence of both the tdh and trh hemolysin-encoding genes, which are also present in ST36. Application of the method in vitro to a collection of 94 clinical isolates collected over a 4-year period in three northeastern U.S. states and 87 environmental isolates revealed that the prp and cps amplicons were detected only in clinical isolates identified as belonging to the ST36 clade and in no environmental isolates from the region. The assay should improve detection and surveillance, thereby reducing infections.

摘要

原产于太平洋的副溶血性弧菌序列类型36(ST36)菌株最近引发了与从大西洋捕捞的贝类相关的多州肠胃炎疫情。对295个副溶血性弧菌基因组进行全基因组比较,其中包括一些追溯到美国东北部来源的基因组,以确定诊断位点,一个推测编码内切核酸酶(prp),另外两个可能赋予O抗原特性(cps和flp)。所有三个位点的组合仅存在于ST36、ST59的一个密切相关菌株分支以及另一个未知序列类型中。然而,每个位点在该分支之外也被发现,prp和flp仅出现在两个非分支分离株中,cps出现在四个非分支分离株中。根据这些位点在测序基因组中的分布,prp识别分支菌株的准确率>99%,但增加一个位点可将准确率提高到100%。靶向prp和cps的寡核苷酸引物被组合成一种多重PCR方法,该方法使用tlh位点定义物种,并确定tdh和trh溶血素编码基因的存在,这两个基因也存在于ST36中。该方法在体外应用于美国东北部三个州4年期间收集的94份临床分离株和87份环境分离株,结果显示,prp和cps扩增子仅在被鉴定为属于ST36分支的临床分离株中检测到,而在该地区的环境分离株中未检测到。该检测方法应能改善检测和监测,从而减少感染。

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