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一种非放射性同位素定量竞争聚合酶链反应方法:在人疱疹病毒7载量检测中的应用。

A non-radioisotopic quantitative competitive polymerase chain reaction method: application in measurement of human herpesvirus 7 load.

作者信息

Kidd I M, Clark D A, Emery V C

机构信息

Department of Virology, Royal Free and University College Medical School, London, UK.

出版信息

J Virol Methods. 2000 Jun;87(1-2):177-81. doi: 10.1016/s0166-0934(00)00164-6.

Abstract

Quantitative-competitive polymerase chain reaction (QCPCR) is a well-optimised and objective methodology for the determination of viral load in clinical specimens. A major advantage of QCPCR is the ability to control for the differential modulation of the PCR process in the presence of potentially inhibitory material. QCPCR protocols were developed previously for CMV, HHV-6, HHV-7 and HHV-8 and relied upon radioactively labelled primers, followed by autoradiography of the separated and digested PCR products to quantify viral load. Whilst this approach offers high accuracy and dynamic range, non-radioactive approaches would be attractive. Here, an alternative detection system is reported, based on simple ethidium bromide staining and computer analysis of the separated reaction products, which enables its adoption in the analysis of a large number of samples. In calibration experiments using cloned HHV-7 DNA, the ethidium bromide detection method showed an improved correlation with known copy number over that obtained with the isotopic method. In addition, 67 HHV-7 PCR positive blood samples, derived from immunocompromised patients, were quantified using both detection techniques. The results showed a highly significant correlation with no significant difference between the two methods. The applicability of the computerised densitometry method in the routine laboratory is discussed.

摘要

定量竞争聚合酶链反应(QCPCR)是一种用于测定临床标本中病毒载量的优化良好且客观的方法。QCPCR的一个主要优点是能够在存在潜在抑制性物质的情况下控制PCR过程的差异调节。先前已开发出针对巨细胞病毒(CMV)、人疱疹病毒6型(HHV - 6)、人疱疹病毒7型(HHV - 7)和人疱疹病毒8型(HHV - 8)的QCPCR方案,这些方案依赖放射性标记引物,随后对分离和消化后的PCR产物进行放射自显影以定量病毒载量。虽然这种方法具有高精度和宽动态范围,但非放射性方法会更具吸引力。在此,报道了一种基于简单溴化乙锭染色和对分离的反应产物进行计算机分析的替代检测系统,这使得它能够应用于大量样本的分析。在使用克隆的HHV - 7 DNA进行的校准实验中,溴化乙锭检测方法与已知拷贝数的相关性比同位素方法得到的更好。此外,使用这两种检测技术对来自免疫功能低下患者的67份HHV - 7 PCR阳性血液样本进行了定量。结果显示两者具有高度显著的相关性,两种方法之间无显著差异。讨论了计算机密度测定法在常规实验室中的适用性。

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