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人肠道病毒的种特异性逆转录聚合酶链反应扩增:一种用于快速鉴定未分类肠道病毒种类的工具。

Species-specific RT-PCR amplification of human enteroviruses: a tool for rapid species identification of uncharacterized enteroviruses.

作者信息

Oberste M Steven, Maher Kaija, Williams Alford J, Dybdahl-Sissoko Naomi, Brown Betty A, Gookin Michelle S, Peñaranda Silvia, Mishrik Nada, Uddin Moyez, Pallansch Mark A

机构信息

Respiratory and Enteric Viruses Branch, Division of Viral and Rickettsial Diseases, National Center for Infectious Diseases, Centers for Disease Control and Prevention, 1600 Clifton Road NE, Mailstop G-17, Atlanta, GA 30333, USA.

Institute of Public Health, Dhaka, Bangladesh.

出版信息

J Gen Virol. 2006 Jan;87(Pt 1):119-128. doi: 10.1099/vir.0.81179-0.

Abstract

The 65 serotypes of human enteroviruses are classified into four species, Human enterovirus (HEV) A to D, based largely on phylogenetic relationships in multiple genome regions. The 3'-non-translated region of enteroviruses is highly conserved within a species but highly divergent between species. From this information, species-specific RT-PCR primers were developed that can be used to rapidly screen collections of enterovirus isolates to identify species of interest. The four primer pairs were 100 % specific when tested against enterovirus prototype strains and panels of isolates of known serotype (a total of 193 isolates). For evaluation in a typical application, the species-specific primers were used to screen 186 previously uncharacterized non-polio enterovirus isolates. The HEV-B primers amplified 68.3 % of isolates, while the HEV-A and HEV-C primers accounted for 9.7 and 11.3 % of isolates, respectively; no isolates were amplified with the HEV-D primers. Twelve isolates (6.5 %) were amplified by more than one primer set and eight isolates (4.3 %) were not amplified by any of the four primer pairs. Serotypes were identified by partial sequencing of the VP1 capsid gene, and in every case sequencing confirmed that the species-specific PCR result was correct; the isolates that were amplified by more than one species-specific primer pair were mixtures of two (11 isolates) or three (one isolate) species of viruses. The eight isolates that were not amplified by the species-specific primers comprised four new serotypes (EV76, EV89, EV90 and EV91) that appear to be unique members of HEV-A based on VP1, 3D and 3'-non-translated region sequences.

摘要

人类肠道病毒的65个血清型主要根据多个基因组区域的系统发育关系分为四个种,即人类肠道病毒A至D。肠道病毒的3'非翻译区在种内高度保守,但在种间差异很大。基于这些信息,开发了种特异性逆转录聚合酶链反应(RT-PCR)引物,可用于快速筛选肠道病毒分离株,以鉴定感兴趣的种。当针对肠道病毒原型株和已知血清型的分离株面板(总共193株分离株)进行测试时,这四对引物具有100%的特异性。为了在典型应用中进行评估,使用种特异性引物筛选了186株先前未鉴定的非脊髓灰质炎肠道病毒分离株。HEV-B引物扩增了68.3%的分离株,而HEV-A和HEV-C引物分别扩增了9.7%和11.3%的分离株;没有分离株被HEV-D引物扩增。12株分离株(6.5%)被不止一组引物扩增,8株分离株(4.3%)未被四对引物中的任何一对扩增。通过对VP1衣壳基因进行部分测序来鉴定血清型,在每种情况下,测序都证实种特异性PCR结果是正确的;被不止一种种特异性引物对扩增的分离株是两种(11株分离株)或三种(1株分离株)病毒的混合物。未被种特异性引物扩增的8株分离株包括四种新血清型(EV76、EV89、EV90和EV91),根据VP1、3D和3'非翻译区序列,它们似乎是HEV-A的独特成员。

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