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RNA聚合酶II和3'端形成因子CstF亚基在秀丽隐杆线虫基因和操纵子上的定位。

Localization of RNAPII and 3' end formation factor CstF subunits on C. elegans genes and operons.

作者信息

Garrido-Lecca Alfonso, Saldi Tassa, Blumenthal Thomas

机构信息

a Department of Molecular, Cellular, and Developmental Biology , University of Colorado , Boulder , CO , USA.

出版信息

Transcription. 2016 May 26;7(3):96-110. doi: 10.1080/21541264.2016.1168509. Epub 2016 Apr 28.

DOI:10.1080/21541264.2016.1168509
PMID:27124504
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4984680/
Abstract

Transcription termination is mechanistically coupled to pre-mRNA 3' end formation to prevent transcription much beyond the gene 3' end. C. elegans, however, engages in polycistronic transcription of operons in which 3' end formation between genes is not accompanied by termination. We have performed RNA polymerase II (RNAPII) and CstF ChIP-seq experiments to investigate at a genome-wide level how RNAPII can transcribe through multiple poly-A signals without causing termination. Our data shows that transcription proceeds in some ways as if operons were composed of multiple adjacent single genes. Total RNAPII shows a small peak at the promoter of the gene cluster and a much larger peak at 3' ends. These 3' peaks coincide with maximal phosphorylation of Ser2 within the C-terminal domain (CTD) of RNAPII and maximal localization of the 3' end formation factor CstF. This pattern occurs at all 3' ends including those at internal sites in operons where termination does not occur. Thus the normal mechanism of 3' end formation does not always result in transcription termination. Furthermore, reduction of CstF50 by RNAi did not substantially alter the pattern of CstF64, total RNAPII, or Ser2 phosphorylation at either internal or terminal 3' ends. However, CstF50 RNAi did result in a subtle reduction of CstF64 binding upstream of the site of 3' cleavage, suggesting that the CstF50/CTD interaction may facilitate bringing the 3' end machinery to the transcription complex.

摘要

转录终止在机制上与前体mRNA的3'末端形成相偶联,以防止转录越过基因3'末端过多。然而,秀丽隐杆线虫进行操纵子的多顺反子转录,其中基因间的3'末端形成并不伴随终止。我们进行了RNA聚合酶II(RNAPII)和CstF染色质免疫沉淀测序实验,以在全基因组水平上研究RNAPII如何能够转录通过多个聚腺苷酸信号而不导致终止。我们的数据表明,转录在某些方面的进行方式就好像操纵子是由多个相邻的单基因组成。总的RNAPII在基因簇的启动子处显示一个小峰,在3'末端显示一个大得多的峰。这些3'峰与RNAPII C末端结构域(CTD)内Ser2的最大磷酸化以及3'末端形成因子CstF的最大定位相一致。这种模式出现在所有3'末端,包括操纵子内部位点处那些不发生终止的3'末端。因此,3'末端形成的正常机制并不总是导致转录终止。此外,通过RNA干扰降低CstF50并没有实质性改变内部或末端3'末端处CstF64、总的RNAPII或Ser2磷酸化的模式。然而,但CstF50 RNA干扰确实导致3'切割位点上游CstF64结合的轻微减少,这表明CstF50/CTD相互作用可能有助于将3'末端机制带到转录复合物中。

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本文引用的文献

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