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RT-PCR and its detection limit for cell culture grown bluetongue virus 1 using NS1 gene group specific primers.

作者信息

Prasad G, Malik Y, Maan S

机构信息

Department of Veterinary Microbiology, CCS Haryana Agricultural University, Hisar, India.

出版信息

Indian J Exp Biol. 1999 Dec;37(12):1255-8.

PMID:10865895
Abstract

RT-PCR was standardised for the detection of bluetongue viral RNA using highly expressed non structural protein 1 gene as the target gene with specific primers targeted to 274 bp of 5' end of NS1 gene. PCR product was consistently obtained in 30 PCR cycles. Further, detection limit of RT-PCR was estimated using serial 10 fold dilutions of BHK 21 cells grown BTV 1. The study suggested that RT-PCR can be used for detection of BTV in Indian conditions with the sensitivity limit of 10 infectious particles of the virus. The study suggested that this technique may be used as a tool for sensitive detection of BTV in carrier/reservoir animals, insect vectors and certification of animals and their germ- plasm for export and import purposes.

摘要

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引用本文的文献

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Vet Q. 2020 Dec;40(1):258-321. doi: 10.1080/01652176.2020.1831708.
2
Identification and differentiation of the twenty six bluetongue virus serotypes by RT-PCR amplification of the serotype-specific genome segment 2.应用 RT-PCR 扩增血清型特异性基因组片段 2 对 26 种蓝舌病病毒血清型进行鉴定和区分。
PLoS One. 2012;7(2):e32601. doi: 10.1371/journal.pone.0032601. Epub 2012 Feb 28.
3
Oncolytic bluetongue viruses: promise, progress, and perspectives.
溶瘤性蓝舌病毒:前景、进展与展望
Front Microbiol. 2011 Mar 16;2:46. doi: 10.3389/fmicb.2011.00046. eCollection 2011.