Author: Huang, Jauâ€Ling; Lin, Huiâ€Tsu; Wang, Yuâ€Ming; Weng, Mingâ€Hui; Ji, Daâ€Der; Kuo, Mingâ€Der; Liu, Huanâ€Wun; Lin, Changâ€Shen
Title: Sensitive and specific detection of strains of Japanese encephalitis virus using a oneâ€step TaqMan RTâ€PCR technique Cord-id: biua91v4 Document date: 2004_10_13
ID: biua91v4
Snippet: A rapid, sensitive, and accurate laboratory diagnostic test is needed for distinguishing Japanese encephalitis virus (JEV) from other diseases featuring similar clinical symptoms and also for preventing potential outbreaks. In this study, a TaqMan reverse transcription (RT)â€polymerase chain reaction (PCR) assay was developed for rapid detection and quantification of the viral RNA of various JEV strains. A consensus JEV NS3 region was chosen to design the primers and the TaqMan probe. The JEV T
Document: A rapid, sensitive, and accurate laboratory diagnostic test is needed for distinguishing Japanese encephalitis virus (JEV) from other diseases featuring similar clinical symptoms and also for preventing potential outbreaks. In this study, a TaqMan reverse transcription (RT)â€polymerase chain reaction (PCR) assay was developed for rapid detection and quantification of the viral RNA of various JEV strains. A consensus JEV NS3 region was chosen to design the primers and the TaqMan probe. The JEV TaqMan assay used the EZâ€rTtH RTâ€PCR system featuring advantages such as a oneâ€step, highâ€temperature RT reaction modality and preventing carryâ€over contamination. The sensitivity of the JEV TaqMan assay for detecting in vitroâ€transcribed JEV NS3 RNA was estimated to be one to five copies of RNA per reaction. For cultured JE virions, less than 40 plaque forming unit (PFU)/ml of virus load (corresponding to 0.07 PFU/test) could be detected. In addition, the JEV TaqMan assay could detect all seven strains of JEV tested, but provided negative results for nine other flaviviruses and encephalitis viruses tested. The JEV TaqMan assay demonstrated greater sensitivity and specificity than traditional RTâ€PCR methods as has been previously reported. The application of the JEV TaqMan assay herein has been shown to the sensitive detection of the JEV from both mosquito pools and also JEVâ€spiking human blood. The assay should be of use in diagnostic laboratory conduct and could be used to replace or complement timeâ€consuming viralâ€culture methods, thus achieving more rapid, sensitive, and highly specific identification of JEV infection. J. Med. Virol. 74:589–596, 2004. © 2004 Wileyâ€Liss, Inc.
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