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Novel gel-based and real-time PCR assays for the improved detection of African horse sickness virus.

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Article
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Rodriguez-Sanchez, B. ; Fernandez-Pinero, J. ; Sailleau, Corinne ; Zientara, Stéphan ; Belak, S. ; Arias, M. ; Sanchez-Vizcaino, J.M.

Journal of virological methods

UMR Virologie 1161 AFSSA INRA ENVA, 23 Avenue General de Gaulle, 94704 Maisons-Alfort Cedex, France

2008

Article

Abstract In order to improve, ensure and accelerate the diagnosis of African horse sickness, a highly devastating, transboundary animal disease listed by the World Animal Health Organisation, (OIE) three novel diagnostic PCR assays were developed and tested in this study. The reverse transcription-PCR (RT-PCR) tests were the following: (a) a conventional, gel-based RT-PCR, (b) a real-time PCR with SYBR-Green-named rRT-PCR SYBR-Green-, and (c) a real-time PCR rRT-PCR with TaqMan probe (termed rRT-PCR TaqMan). The same pair of primers-directed against African Horse Sickness Virus (AHSV) segment 5, encoding the non-structural protein NS1, is used in the three tests listed above. The three PCR assays detected similarly the nine AHSV serotypes from cultivated viral suspensions of different origins. The RT-PCR assays provided high sensitivity ranging from 0.1 to 1.2TCID(50)/ml. The specificity was also high, considering that related viruses, such as Bluetongue virus, and other equine viruses, such as West Nile Virus, remained negative for RT-PCR amplification. The detection of AHSV virus can be completed within 2-3h. These results indicate that the novel PCR methods described in this paper provide robust and versatile tools that allow rapid and highly specific, simultaneous detection of all AHSV serotypes.
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