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通过聚合酶链反应检测西尼罗河病毒并分析核苷酸序列变异。

Detection of West Nile virus by the polymerase chain reaction and analysis of nucleotide sequence variation.

作者信息

Porter K R, Summers P L, Dubois D, Puri B, Nelson W, Henchal E, Oprandy J J, Hayes C G

机构信息

Infectious Diseases Threat Assessment Program, Naval Medical Research Institute, Bethesda, Maryland.

出版信息

Am J Trop Med Hyg. 1993 Mar;48(3):440-6. doi: 10.4269/ajtmh.1993.48.440.

Abstract

A polymerase chain reaction (PCR) assay was developed to rapidly detect and identify West Nile (WN) virus. The RNA from seven isolates of WN virus from six countries and four other flaviviruses (Kunjin, Japanese encephalitis, St. Louis encephalitis, and yellow fever viruses) was reverse-transcribed (RT) and amplified by PCR. The nucleotide sequences of the amplified products were determined by a rapid, automated DNA sequencing method. The WN virus RT/PCR assay detected the target gene segment of sequencing method. The WN virus RT/PCR assay detected the target gene segment of isolates from both the African-Middle Eastern group and the Indian group with a sensitivity of approximately 0.05 pg of viral RNA. Kunjin virus was the only other flavivirus tested that produced a band of the appropriate size. Five of seven WN virus isolates showed 92-98% homology in the nucleotide sequence of their PCR products. The sequence of one isolate was virtually identical to the published sequence of the Nigerian isolate (99.5% homology). No correlation was established between the degree of nucleotide homology, geographic location, time of isolation, or source of the isolates.

摘要

已开发出一种聚合酶链反应(PCR)检测方法,用于快速检测和鉴定西尼罗河(WN)病毒。来自六个国家的七株WN病毒分离株以及其他四种黄病毒(库京病毒、日本脑炎病毒、圣路易斯脑炎病毒和黄热病病毒)的RNA被逆转录(RT),并通过PCR进行扩增。扩增产物的核苷酸序列通过一种快速的自动化DNA测序方法确定。WN病毒RT/PCR检测方法检测到了测序方法的目标基因片段。WN病毒RT/PCR检测方法以约0.05 pg病毒RNA的灵敏度检测到了来自非洲-中东组和印度组分离株的目标基因片段。库京病毒是所检测的唯一产生适当大小条带的其他黄病毒。七株WN病毒分离株中有五株在其PCR产物的核苷酸序列中显示出92%-98%的同源性。一株分离株的序列与已发表的尼日利亚分离株序列几乎相同(99.5%同源性)。在核苷酸同源性程度、地理位置、分离时间或分离株来源之间未建立相关性。

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