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用于α疱疹病毒分型的焦磷酸测序检测方法的开发。

Development of a pyrosequencing assay for the typing of alphaherpesviruses.

作者信息

Fusco G, Amoroso M G, Gesualdi Montesano N, Viscardi M

机构信息

Department of Animal Health, Experimental Zooprophylactic Institute of Southern Italy, Via Salute, 2, 80055 Portici (NA), Italy.

Qiagen Srl, Via Grosio 10/8, 20151 Milano, Italy.

出版信息

MethodsX. 2015 Jan 12;2:47-52. doi: 10.1016/j.mex.2015.01.001. eCollection 2015.

Abstract

Identification of herpesvirus in biological material is usually carried out by real-time PCR. With the aim to classify the strain of virus identified, real-time PCR must be often supported by time-consuming capillary electrophoresis sequencing analysis. Here we provide a protocol for the rapid and reliable identification of 5 closely related herpesviruses by PyroMark Q24 sequencing system. PyroMark performs DNA sequencing analysis using pyrosequencing, a technology based on the detection of released pyrophosphate during DNA elongation [1]. PyroMark is designed to detect changes in specified variable positions of the DNA. It can efficiently detect single nucleotide differences in sequences [2]. In the present paper we describe a protocol to pyrosequence a small polymorphic segment of the US8 gene. On the basis of the differences identified in the nucleotide sequence we could readily classify the herpesvirus as Bovine herpesvirus 1.1, Bovine herpesvirus 1.2, Bovine herpesvirus 5, Bubaline herpesvirus 1 or Caprine herpesvirus. The protocol set up offers several advantages with respect to the techniques commonly used: •it requires less than one working day to be carried;•it gives the possibility to analyze, at reasonable costs, up to 24 samples at a time; and•it allows to detect with great reliability and specificity strongly genetically correlated organisms like the herpesviruses named above. The procedure can be easily applied to other families of viruses, with opportune modifications.

摘要

生物材料中疱疹病毒的鉴定通常通过实时聚合酶链反应(PCR)进行。为了对鉴定出的病毒株进行分类,实时PCR通常需要耗时的毛细管电泳测序分析的支持。在此,我们提供一种通过焦磷酸测序Q24系统快速可靠地鉴定5种密切相关疱疹病毒的方法。焦磷酸测序仪利用焦磷酸测序技术进行DNA测序分析,该技术基于检测DNA延伸过程中释放的焦磷酸[1]。焦磷酸测序仪旨在检测DNA特定可变位置的变化。它能够高效地检测序列中的单核苷酸差异[2]。在本文中,我们描述了一种对US8基因的一个小的多态性片段进行焦磷酸测序的方法。基于核苷酸序列中鉴定出的差异,我们能够轻松地将疱疹病毒分类为牛疱疹病毒1.1、牛疱疹病毒1.2、牛疱疹病毒5、水牛疱疹病毒1或山羊疱疹病毒。所建立的方法相对于常用技术具有几个优点:•该方法执行所需时间不到一个工作日;•它能够以合理的成本一次分析多达24个样本;•它能够高度可靠且特异地区分遗传关系密切的生物体,如上述疱疹病毒。经过适当修改后,该程序可轻松应用于其他病毒家族。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8d4a/4487326/00cf3a0281ae/gr1.jpg

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本文引用的文献

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