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用于区分临床和环境样本中脊髓灰质炎病毒和肠道病毒的逆转录多重聚合酶链反应

Reverse transcription multiplex PCR for differentiation between polio- and enteroviruses from clinical and environmental samples.

作者信息

Egger D, Pasamontes L, Ostermayer M, Bienz K

机构信息

Institute for Medical Microbiology, University of Basel, Switzerland.

出版信息

J Clin Microbiol. 1995 Jun;33(6):1442-7. doi: 10.1128/jcm.33.6.1442-1447.1995.

Abstract

For the rapid detection of polioviruses and their differentiation from nonpoliovirus enteroviruses, we developed a protocol in which clinical or environmental specimens are first inoculated onto cell cultures in tubes. After overnight incubation, the cultures are subjected to reverse transcription multiplex PCR with a primer pair which detects all enteroviruses (T. Hyypiä, P. Auvinen, and M. Maaronen, J. Gen. Virol. 70:3261-3268 1989) and two newly designed primer pairs specific for all 36 poliovirus strains tested. The PCR products can unequivocally be identified by their lengths in agarose gels, whereas the genetic heterogeneity of the poliovirus strains precludes identification by back-hybridization with internal probes. The proposed protocol is highly insensitive to the inhibitory effects of substances in the sample (stool, sewage). It allows for the detection of polioviruses and for polioviruses to be distinguished from nonpoliovirus enteroviruses within 24 h, and it allows for the concomitant isolation of a viable strain suitable for further typing.

摘要

为了快速检测脊髓灰质炎病毒并将其与非脊髓灰质炎肠道病毒区分开来,我们开发了一种方法,即首先将临床或环境标本接种到试管中的细胞培养物上。过夜培养后,使用一对能检测所有肠道病毒的引物(T. Hyypiä、P. Auvinen和M. Maaronen,《普通病毒学杂志》70:3261 - 3268,1989年)以及另外两对新设计的、针对所有36种测试脊髓灰质炎病毒株的引物对培养物进行逆转录多重PCR。PCR产物可通过其在琼脂糖凝胶中的长度明确鉴定,而脊髓灰质炎病毒株的基因异质性使得无法通过与内部探针的反向杂交进行鉴定。所提出的方法对样品(粪便、污水)中物质的抑制作用高度不敏感。它能够在24小时内检测出脊髓灰质炎病毒,并将脊髓灰质炎病毒与非脊髓灰质炎肠道病毒区分开来,还能同时分离出适合进一步分型的活毒株。

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