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一种基于实时定量PCR的猿猴病毒40检测和定量方法。

A real time quantitative PCR-based method for the detection and quantification of simian virus 40.

作者信息

Shi L, Ho J, Norling L A, Roy M, Xu Y

机构信息

Genentech, Inc., 1 DNA Way, South San Francisco, CA 94080, USA.

出版信息

Biologicals. 1999 Sep;27(3):241-52. doi: 10.1006/biol.1999.0212.

Abstract

A real time quantitative PCR-based simian virus 40 (SV40) detection and quantification method has been developed. This method takes advantage of the 5' to 3'-exonuclease activity of Taq DNA polymerase and utilizes the PRISM 7700 sequence detection system of PE Applied Biosystems for direct monitoring of PCR product accumulation through a dual-labelled fluorogenic probe. This method provides accurate, precise and reproducible quantification of SV40 DNA over a linear dynamic range of at least 100,000-fold with a minimum detection level of 6.4 copy equivalents/microL of SV40 viral particle in test samples. The sample preparation procedure employed allows for efficient and consistent recovery of SV40 DNA from test samples. High concentrations of protein and cellular DNA presenting in test samples have been demonstrated to have no impact on SV40 quantification. This method offers significant advantages over other PCR methods and cell-based infectivity assays currently available for SV40 detection and quantification. The availability of this method should greatly facilitate the pathogenic investigation of SV40, as well as viral clearance evaluations required for the development of new biological products.

摘要

一种基于实时定量PCR的猿猴病毒40(SV40)检测和定量方法已经开发出来。该方法利用了Taq DNA聚合酶的5'至3'外切核酸酶活性,并使用PE应用生物系统公司的PRISM 7700序列检测系统,通过双标记荧光探针直接监测PCR产物的积累。该方法在至少100,000倍的线性动态范围内提供准确、精确和可重复的SV40 DNA定量,测试样品中SV40病毒颗粒的最低检测水平为6.4拷贝当量/微升。所采用的样品制备程序能够从测试样品中高效、一致地回收SV40 DNA。已证明测试样品中存在的高浓度蛋白质和细胞DNA对SV40定量没有影响。该方法比目前可用于SV40检测和定量的其他PCR方法和基于细胞的感染性测定具有显著优势。这种方法的可用性应极大地促进SV40的致病性研究以及新生物制品开发所需的病毒清除评估。

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