Detection and quantitation of subgroup C adenovirus DNA in human tissue samples by real-time PCR.

C T Garnett, Ching-I Pao, Linda R Gooding
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引用次数: 19

Abstract

Advances in amplification techniques have revolutionized the ability to detect viruses both quantitatively and qualitatively and to study viral load. Real-time polymerase chain reaction (PCR) amplification depends on the ability to detect and quantify a fluorescent reporter molecule whose signal increases in proportion to the amount of amplification product generated. Recent advances have been made by using probes, such as TaqMan probes, to detect amplified products. Use of these probes offers confirmation of specificity of the PCR product. Here we describe a sensitive real-time PCR assay to quantify subgroup C adenoviral DNA in human lymphocytes derived from mucosal tissues removed in routine tonsillectomy or adenoidectomy. This chapter will describe in detail the methods used for these analyses.

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实时荧光定量PCR检测人体组织标本中C亚群腺病毒DNA。
扩增技术的进步彻底改变了定量和定性检测病毒以及研究病毒载量的能力。实时聚合酶链反应(PCR)扩增依赖于检测和定量荧光报告分子的能力,其信号与扩增产物的数量成比例增加。最近的进展是使用探针,如TaqMan探针,来检测扩增产物。使用这些探针可以确认PCR产物的特异性。在这里,我们描述了一种灵敏的实时PCR方法,用于定量常规扁桃体切除术或腺样体切除术后粘膜组织中提取的人淋巴细胞中的C亚群腺病毒DNA。本章将详细描述用于这些分析的方法。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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