Strategies for the sequence determination of viral dsRNA genomes

被引:162
作者
Attoui, H
Billoir, F
Cantaloube, JF
Biagini, P
de Micco, P
de Lamballerie, X
机构
[1] Univ Mediterranee, Fac Med Marseille, Lab Virol Mol Trop & Transfus, Unite Virus Emergents, F-13005 Marseille 5, France
[2] EFS Alpes Mediterranee, Mol Virol Lab, Unite Virus Emergents, F-13005 Marseille, France
关键词
dsRNA cloning; dsRNA viruses; non cultivable dsRNA viruses; sequence determination;
D O I
10.1016/S0166-0934(00)00212-3
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
The genetic study of viruses having dsRNA genomes is hampered by the technical difficulty of complete sequence determination of dsRNA. Optimised methods are described here for sequencing dsRNAs, which meet three different situations: (1) genomes that can be obtained in fairly high amounts (> 20 ng per separated segment); (2) genomes with limited amounts of RNA that can be detected by electrophoretic gel separation and staining; (3) genomes that cannot be detected by electrophoretic gel separation and staining. These methods include improved Single Primer Amplification Technique protocols, an adaptation of the SMART(TM) methodology, and a new method permitting the selective enzymatic removal of dsRNA segments. Strategies permitting adaptation of these protocols to the full-length determination of dsRNA viral genomes are described. Each of the protocols is described for sequence determination of a chosen dsRNA virus. (C) 2000 Elsevier Science B.V. All rights reserved.
引用
收藏
页码:147 / 158
页数:12
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