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用于探针合成及在牛冠状病毒检测中直接扩增的聚合酶链反应。

Polymerase chain reaction for probe synthesis and for direct amplification in detection of bovine coronavirus.

作者信息

Verbeek A, Tijssen P

机构信息

Centre de recherche en médicine comparée, Institut Armand-Frappier, Université du Québec, Laval-des-Rapides, Canada.

出版信息

J Virol Methods. 1990 Sep;29(3):243-55. doi: 10.1016/0166-0934(90)90052-h.

Abstract

The polymerase chain reaction (PCR) was used to synthesize ds and ss probes for the detection of bovine coronavirus (BCV) using recombinant plasmids as template molecules. The ds probes detected a minimum of about 2 X 10(5) viral genomes after exposure for 1 h, a detection limit similar to nick-translated probes after exposure of the films for 60 h. More than 8 h exposure to blots probed with these ds probes resulted in complete darkening of the film. The ss probes, synthesized by asymmetric PCR on linearized plasmids, permitted the detection of 5 X 10(4) genomes, which equalled the capacity of random-primed probes. Prolonged exposure did not increase the background as in case of ds PCR-probed blots. Probes, synthesized by asymmetric PCR and random-priming were labeled to similar specific activities and were better in terms of sensitivity and detectability as opposed to nick-translated probes. However, the specificity of detection with ss probes as to random primed probes was increased further. About 10 viral genomes, after fragment-specific amplification by PCR, were detected by agarose-gel analysis. PCR-probe synthesis was simple, highly reproducible, and allowed the synthesis of probes for specific fragments.

摘要

采用聚合酶链反应(PCR),以重组质粒为模板分子合成双链和单链探针,用于检测牛冠状病毒(BCV)。双链探针在曝光1小时后可检测到至少约2×10⁵个病毒基因组,这一检测限与缺口平移探针曝光60小时后的检测限相似。用这些双链探针探测印迹超过8小时会导致胶片完全变黑。通过在线性化质粒上进行不对称PCR合成的单链探针可检测到5×10⁴个基因组,这与随机引物探针的检测能力相当。与双链PCR探测的印迹不同,长时间曝光不会增加背景。通过不对称PCR和随机引物合成的探针标记到相似的比活性,并且在灵敏度和可检测性方面比缺口平移探针更好。然而,单链探针相对于随机引物探针的检测特异性进一步提高。通过PCR进行片段特异性扩增后,约10个病毒基因组可通过琼脂糖凝胶分析检测到。PCR探针合成简单、高度可重复,并允许合成特定片段的探针。

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