多平台下一代测序鉴定了从培养细胞中分离出的内源性逆转录病毒的新型RNA分子和转录异构体。
Multiplatform next-generation sequencing identifies novel RNA molecules and transcript isoforms of the endogenous retrovirus isolated from cultured cells.
作者信息
Moldován Norbert, Szucs Attila, Tombácz Dóra, Balázs Zsolt, Csabai Zsolt, Snyder Michael, Boldogkoi Zsolt
机构信息
Department of Medical Biology, Faculty of Medicine, University of Szeged, Szeged H-6720, Hungary.
Department of Genetics, School of Medicine, Stanford University, Stanford, CA 94305, USA.
出版信息
FEMS Microbiol Lett. 2018 Mar 1;365(5). doi: 10.1093/femsle/fny013.
Abstract
In this study, we applied short- and long-read RNA sequencing techniques, as well as PCR analysis to investigate the transcriptome of the porcine endogenous retrovirus (PERV) expressed from cultured porcine kidney cell line PK-15. This analysis has revealed six novel transcripts and eight transcript isoforms, including five length and three splice variants. We were able to establish whether a deletion in a transcript is the result of the splicing of mRNAs or of genomic deletion in one of the PERV clones. Additionally, we re-annotated the formerly identified RNA molecules. Our analysis revealed a higher complexity of PERV transcriptome than it was earlier believed.
摘要
在本研究中,我们应用短读长和长读长RNA测序技术以及PCR分析,来研究从培养的猪肾细胞系PK-15中表达的猪内源性逆转录病毒(PERV)的转录组。该分析揭示了6种新转录本和8种转录异构体,包括5种长度变体和3种剪接变体。我们能够确定转录本中的缺失是mRNA剪接的结果还是PERV克隆之一中基因组缺失的结果。此外,我们对先前鉴定的RNA分子进行了重新注释。我们的分析表明,PERV转录组的复杂性比之前认为的更高。
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