A real-time RT-PCR method for the universal detection and identification of flaviviruses

被引:158
作者
Moureau, G. [1 ]
Temmam, S. [1 ]
Gonzalez, J. P. [2 ]
Charrel, R. N. [1 ]
Grard, G. [1 ]
De Lamballerie, X. [1 ]
机构
[1] Fac Med, Unite Virus Emergents, F-13005 Marseille, France
[2] Mahidol Univ, Res Ctr Emerging Viral Dis, Ctr Vaccine Dev, Inst Sci,IRD UR0178, Nakhon Pathom 73170, Thailand
关键词
D O I
10.1089/vbz.2007.0206
中图分类号
R1 [预防医学、卫生学];
学科分类号
1004 ; 120402 ;
摘要
Here we describe an optimized molecular protocol for the universal detection and identification of flaviviruses. It combines the convenient real-time polymerase chain reaction (PCR) format with a broad spectrum of flavivirus detection. This assay, based on the amplification of a 269-272 nt (depending on the flavivirus tested) region at the N terminal end of the NS5 gene, enabled the amplification of 51 flavivirus species and 3 tentative species. Sequencing of the amplicons produced by reverse transcriptase (RT)-PCR permitted the reliable taxonomic identification of flavivirus species by comparison with reference sequences available in databases, using either the BLASTN algorithm or a simple phylogenetic reconstruction. The limit of detection of the assay (2-20,500 copies/reaction depending on the virus tested) allowed the detection of different flaviviruses from a series of human sera or veterinary samples. Altogether, the characteristics of this technique make it a good candidate for the identification of previously identified flaviviruses in cell culture and the investigation of field samples, and also a promising tool for the discovery and identification of new species, including viruses distantly related to "classical" arthropod-borne flaviviruses.
引用
收藏
页码:467 / 477
页数:11
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