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2型腺相关病毒(AAV)转录组的全面RNA测序分析揭示了新型AAV转录本、剪接变体和衍生蛋白。

A Comprehensive RNA Sequencing Analysis of the Adeno-Associated Virus (AAV) Type 2 Transcriptome Reveals Novel AAV Transcripts, Splice Variants, and Derived Proteins.

作者信息

Stutika Catrin, Gogol-Döring Andreas, Botschen Laura, Mietzsch Mario, Weger Stefan, Feldkamp Mirjam, Chen Wei, Heilbronn Regine

机构信息

Institute of Virology, Campus Benjamin Franklin, Charité Medical School, Berlin, Germany.

German Centre for Integrative Biodiversity Research, Halle-Jena-Leipzig, Germany.

出版信息

J Virol. 2015 Nov 11;90(3):1278-89. doi: 10.1128/JVI.02750-15. Print 2016 Feb 1.

Abstract

UNLABELLED

Adeno-associated virus (AAV) is recognized for its bipartite life cycle with productive replication dependent on coinfection with adenovirus (Ad) and AAV latency being established in the absence of a helper virus. The shift from latent to Ad-dependent AAV replication is mostly regulated at the transcriptional level. The current AAV transcription map displays highly expressed transcripts as found upon coinfection with Ad. So far, AAV transcripts have only been characterized on the plus strand of the AAV single-stranded DNA genome. The AAV minus strand is assumed not to be transcribed. Here, we apply Illumina-based RNA sequencing (RNA-Seq) to characterize the entire AAV2 transcriptome in the absence or presence of Ad. We find known and identify novel AAV transcripts, including additional splice variants, the most abundant of which leads to expression of a novel 18-kDa Rep/VP fusion protein. Furthermore, we identify for the first time transcription on the AAV minus strand with clustered reads upstream of the p5 promoter, confirmed by 5' rapid amplification of cDNA ends and RNase protection assays. The p5 promoter displays considerable activity in both directions, a finding indicative of divergent transcription. Upon infection with AAV alone, low-level transcription of both AAV strands is detectable and is strongly stimulated upon coinfection with Ad.

IMPORTANCE

Next-generation sequencing (NGS) allows unbiased genome-wide analyses of transcription profiles, used here for an in depth analysis of the AAV2 transcriptome during latency and productive infection. RNA-Seq analysis led to the discovery of novel AAV transcripts and splice variants, including a derived, novel 18-kDa Rep/VP fusion protein. Unexpectedly, transcription from the AAV minus strand was discovered, indicative of divergent transcription from the p5 promoter. This finding opens the door for novel concepts of the switch between AAV latency and productive replication. In the absence of a suitable animal model to study AAV in vivo, combined in cellulae and in silico studies will help to forward the understanding of the unique, bipartite AAV life cycle.

摘要

未标记

腺相关病毒(AAV)因其二分生命周期而被人们所认识,其有效复制依赖于与腺病毒(Ad)的共感染,且在没有辅助病毒的情况下建立AAV潜伏期。从潜伏状态到依赖Ad的AAV复制的转变主要在转录水平上受到调控。当前的AAV转录图谱显示了与Ad共感染时高度表达的转录本。到目前为止,AAV转录本仅在AAV单链DNA基因组的正链上得到了表征。人们认为AAV负链不被转录。在此,我们应用基于Illumina的RNA测序(RNA-Seq)来表征在有无Ad的情况下整个AAV2转录组。我们发现了已知的并鉴定出了新的AAV转录本,包括额外的剪接变体,其中最丰富的变体导致一种新的18 kDa Rep/VP融合蛋白的表达。此外,我们首次在p5启动子上游发现了成簇的reads,从而鉴定出AAV负链上的转录,这通过5' cDNA末端快速扩增和核糖核酸酶保护试验得到了证实。p5启动子在两个方向上都表现出相当的活性,这一发现表明存在双向转录。单独感染AAV时,可检测到AAV两条链的低水平转录,与Ad共感染时则会受到强烈刺激。

重要性

下一代测序(NGS)允许对转录谱进行无偏倚的全基因组分析,在此用于深入分析潜伏期和生产性感染期间的AAV2转录组。RNA-Seq分析导致发现了新的AAV转录本和剪接变体,包括一种衍生的新的18 kDa Rep/VP融合蛋白。出乎意料的是,发现了来自AAV负链的转录,这表明从p5启动子存在双向转录。这一发现为AAV潜伏期和生产性复制之间转换的新概念打开了大门。在缺乏合适的体内研究AAV的动物模型的情况下,细胞内和计算机模拟相结合的研究将有助于推进对独特的二分AAV生命周期的理解。

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