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转录终止的检测与特征分析

Detection and characterization of transcription termination.

作者信息

Ghazal Ghada, Gagnon Jules, Elela Sherif Abou

机构信息

RNA Group/Groupe ARN, Département de Microbiologie & Infectiologie, Faculté de médecine et des sciences de la santé, Université de Sherbrooke, Sherbrooke, QC, Canada.

出版信息

Methods Mol Biol. 2012;809:593-607. doi: 10.1007/978-1-61779-376-9_38.

Abstract

In most eukaryotes, the generation of the 3' end and transcription termination are initiated by cleavage of the pre-mRNA upstream of the polyadenylation site. This cleavage initiates 5'-3' degradation of the 3' end cleavage product by the exoribonuclease Rat1p leading to the dissociation of the RNA polymerase II (RNAPII) complex. The Rat1p-dependent transcription termination was also shown to be initiated by a polyadenylation-independent cleavage performed by the double-stranded RNA-specific ribonuclease (RNase) III (Rnt1p) suggesting that the majority of transcription termination events are RNase dependent. Therefore, it became essential for future studies on transcription termination to carefully consider both the nature of the RNase-dependent RNA transcripts and the association pattern of the RNAPII with the transcriptional unit. Here, we present methods allowing the evaluation of the impact of yeast RNases on the 3' end formation and their contribution to transcription termination. Northern blot analysis of transcripts generated downstream of known genes in the absence of RNases identifies potential transcription termination sites while chromatin immunoprecipitation of RNAPII differentiates between termination- and transcription-independent processing events.

摘要

在大多数真核生物中,3' 端的生成和转录终止是由聚腺苷酸化位点上游的前体 mRNA 切割引发的。这种切割通过外切核糖核酸酶 Rat1p 启动 3' 端切割产物的 5'-3' 降解,导致 RNA 聚合酶 II(RNAPII)复合物解离。还发现依赖 Rat1p 的转录终止是由双链 RNA 特异性核糖核酸酶(RNase)III(Rnt1p)进行的不依赖聚腺苷酸化的切割引发的,这表明大多数转录终止事件是依赖 RNase 的。因此,对于未来关于转录终止的研究而言,仔细考虑依赖 RNase 的 RNA 转录本的性质以及 RNAPII 与转录单元的结合模式变得至关重要。在此,我们介绍了一些方法,可用于评估酵母 RNase 对 3' 端形成的影响及其对转录终止的贡献。在不存在 RNase 的情况下,对已知基因下游产生的转录本进行 Northern 印迹分析可确定潜在的转录终止位点,而 RNAPII 的染色质免疫沉淀可区分终止依赖性和转录非依赖性加工事件。

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