Next generation sequencing of viral RNA genomes

被引:101
作者
Marston, Denise A. [1 ,5 ]
McElhinney, Lorraine M. [1 ,3 ]
Ellis, Richard J. [2 ]
Horton, Daniel L. [1 ]
Wise, Emma L. [1 ]
Leech, Stacey L. [1 ]
David, Dan [4 ]
de Lamballerie, Xavier [5 ]
Fooks, Anthony R. [1 ,3 ]
机构
[1] AHVLA, Wildlife Zoonoses & Vector Borne Dis Res Grp, Addlestone KT15 3NB, Surrey, England
[2] AHVLA, Cent Sequencing Unit, Addlestone KT15 3NB, Surrey, England
[3] Natl Consortium Zoonosis Res, Wirral, Merseyside, England
[4] Kimron Vet Inst, Rabies Lab, IL-50250 Bet Dagan, Israel
[5] Aix Marseille Univ, IRD French Inst Res Dev, EHESP French Sch Publ Hlth, UMR Emergence Pathol Virales D 190, F-13005 Marseille, France
关键词
Next generation sequencing; Pyrosequencing; Lyssavirus; Genome; RNA; Virus; BAT; LYSSAVIRUS; VIRUSES; TECHNOLOGIES;
D O I
10.1186/1471-2164-14-444
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Background: With the advent of Next Generation Sequencing (NGS) technologies, the ability to generate large amounts of sequence data has revolutionized the genomics field. Most RNA viruses have relatively small genomes in comparison to other organisms and as such, would appear to be an obvious success story for the use of NGS technologies. However, due to the relatively low abundance of viral RNA in relation to host RNA, RNA viruses have proved relatively difficult to sequence using NGS technologies. Here we detail a simple, robust methodology, without the use of ultra-centrifugation, filtration or viral enrichment protocols, to prepare RNA from diagnostic clinical tissue samples, cell monolayers and tissue culture supernatant, for subsequent sequencing on the Roche 454 platform. Results: As representative RNA viruses, full genome sequence was successfully obtained from known lyssaviruses belonging to recognized species and a novel lyssavirus species using these protocols and assembling the reads using de novo algorithms. Furthermore, genome sequences were generated from considerably less than 200 ng RNA, indicating that manufacturers' minimum template guidance is conservative. In addition to obtaining genome consensus sequence, a high proportion of SNPs (Single Nucleotide Polymorphisms) were identified in the majority of samples analyzed. Conclusions: The approaches reported clearly facilitate successful full genome lyssavirus sequencing and can be universally applied to discovering and obtaining consensus genome sequences of RNA viruses from a variety of sources.
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页数:12
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