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反义 RNA 聚合酶 II 发散转录本依赖于 P-TEFb,是 RNA 外切酶的底物。

Antisense RNA polymerase II divergent transcripts are P-TEFb dependent and substrates for the RNA exosome.

机构信息

David H. Koch Institute for Integrative Cancer Research, Cambridge, MA 02139, USA.

出版信息

Proc Natl Acad Sci U S A. 2011 Jun 28;108(26):10460-5. doi: 10.1073/pnas.1106630108. Epub 2011 Jun 13.

Abstract

Divergent transcription occurs at the majority of RNA polymerase II (RNAPII) promoters in mouse embryonic stem cells (mESCs), and this activity correlates with CpG islands. Here we report the characterization of upstream antisense transcription in regions encoding transcription start site associated RNAs (TSSa-RNAs) at four divergent CpG island promoters: Isg20l1, Tcea1, Txn1, and Sf3b1. We find that upstream antisense RNAs (uaRNAs) have distinct capped 5' termini and heterogeneous nonpolyadenylated 3' ends. uaRNAs are short-lived with average half-lives of 18 minutes and are present at 1-4 copies per cell, approximately one RNA per DNA template. Exosome depletion stabilizes uaRNAs. These uaRNAs are probably initiation products because their capped termini correlate with peaks of paused RNAPII. The pausing factors NELF and DSIF are associated with these antisense polymerases and their sense partners. Knockdown of either NELF or DSIF results in an increase in the levels of uaRNAs. Consistent with P-TEFb controlling release from pausing, treatment with its inhibitor, flavopiridol, decreases uaRNA and nascent mRNA transcripts with similar kinetics. Finally, Isg20l1 induction reveals equivalent increases in transcriptional activity in sense and antisense directions. Together these data show divergent polymerases are regulated after P-TEFb recruitment with uaRNA levels controlled by the exosome.

摘要

在小鼠胚胎干细胞 (mESC) 中,大多数 RNA 聚合酶 II (RNAPII) 启动子都会发生差异转录,这种活性与 CpG 岛相关。在这里,我们报告了在四个发散的 CpG 岛启动子(Isg20l1、Tcea1、Txn1 和 Sf3b1)编码转录起始相关 RNA(TSSa-RNA)的区域中上游反义转录的特征。我们发现上游反义 RNA(uaRNA)具有独特的加帽 5'末端和异质的非多聚腺苷酸化 3'末端。uaRNA 半衰期短,平均半衰期为 18 分钟,每个细胞存在 1-4 个拷贝,大约每个 DNA 模板一个 RNA。外切体耗竭稳定 uaRNA。这些 uaRNA 可能是起始产物,因为它们的加帽末端与暂停的 RNAPII 峰相关。暂停因子 NELF 和 DSIF 与这些反义聚合酶及其有意义的伙伴相关联。敲低 NELF 或 DSIF 都会导致 uaRNA 水平增加。与 P-TEFb 控制从暂停中释放一致,用其抑制剂 flavopiridol 处理会以相似的动力学降低 uaRNA 和新生 mRNA 转录本。最后,Isg20l1 的诱导显示出在有义和反义方向上转录活性的等效增加。这些数据表明,差异聚合酶在 P-TEFb 募集后受到调控,uaRNA 水平受外切体控制。

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