Development of a dual target-PCR for detection and characterization of measles virus in clinical specimens

被引:56
作者
Jin, L
Richards, A
Brown, DWG
机构
[1] Enteric and Resp. Virus Laboratory, Central Public Health Laboratory, London NW9 5HT
关键词
measles virus; dual target-PCR; genetic characterization of MV strains;
D O I
10.1006/mcpr.1996.0027
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
A polymerase chain reaction (PCR) method was developed for detecting measles virus (MV) RNA in a variety of clinical samples using primer pairs in the nucleocapsid (N) and matrix (M) genes in one reaction (dual target-PCR). The dual target-PCR detected MV RNA in tissue culture fluid containing 1 TCID50 of the MV Loss strain, and was as sensitive as a single target-PCR. Specificity was confirmed by the failure of the dual target-PCR to amplify products from the infected tissue culture containing related paramyxoviruses. Thirty-two of 35 (91.4%) samples collected from 23 patients with confirmed measles infection by the detection of measles specific IgM were found to be positive for MV RNA by PCR. Direct sequencing of the PCR amplicons revealed three different genotypes among the MV strains that were detected in 12 patients. The dual target-PCR method is suitable for the diagnosis of measles infection and, based on the sequencing of the PCR product DNA, for investigating the molecular epidemiology of MV strains. (C) 1996 Academic Press Limited
引用
收藏
页码:191 / 200
页数:10
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