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通过实时聚合酶链式反应检测和监测病毒感染

Detection and monitoring of virus infections by real-time PCR.

作者信息

Watzinger F, Ebner K, Lion T

机构信息

Children's Cancer Research Institute, St. Anna Kinderspital, A-1090 Vienna, Austria.

出版信息

Mol Aspects Med. 2006 Apr-Jun;27(2-3):254-98. doi: 10.1016/j.mam.2005.12.001. Epub 2006 Feb 14.

Abstract

The employment of polymerase chain reaction (PCR) techniques for virus detection and quantification offers the advantages of high sensitivity and reproducibility, combined with an extremely broad dynamic range. A number of qualitative and quantitative PCR virus assays have been described, but commercial PCR kits are available for quantitative analysis of a limited number of clinically important viruses only. In addition to permitting the assessment of viral load at a given time point, quantitative PCR tests offer the possibility of determining the dynamics of virus proliferation, monitoring of the response to treatment and, in viruses displaying persistence in defined cell types, distinction between latent and active infection. Moreover, from a technical point of view, the employment of sequential quantitative PCR assays in virus monitoring helps identifying false positive results caused by inadvertent contamination of samples with traces of viral nucleic acids or PCR products. In this review, we provide a survey of the current state-of-the-art in the application of the real-time PCR technology to virus analysis. Advantages and limitations of the RQ-PCR methodology, and quality control issues related to standardization and validation of diagnostic assays are discussed.

摘要

采用聚合酶链反应(PCR)技术进行病毒检测和定量具有高灵敏度、可重复性强以及动态范围极广等优点。已经描述了多种定性和定量PCR病毒检测方法,但商业PCR试剂盒仅可用于对少数几种临床重要病毒进行定量分析。除了能够在给定时间点评估病毒载量外,定量PCR检测还提供了确定病毒增殖动态、监测治疗反应的可能性,并且对于在特定细胞类型中具有持续性的病毒,能够区分潜伏感染和活跃感染。此外,从技术角度来看,在病毒监测中采用连续定量PCR检测有助于识别因样品被痕量病毒核酸或PCR产物意外污染而导致的假阳性结果。在本综述中,我们对实时PCR技术在病毒分析中的应用现状进行了概述。讨论了相对定量PCR方法的优点和局限性,以及与诊断检测标准化和验证相关的质量控制问题。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6062/7112306/b5fd4843301e/gr1.jpg

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