一种用于转录错误的基因检测揭示了RNA聚合酶II保真度的多层控制。

A genetic assay for transcription errors reveals multilayer control of RNA polymerase II fidelity.

作者信息

Irvin Jordan D, Kireeva Maria L, Gotte Deanna R, Shafer Brenda K, Huang Ingold, Kashlev Mikhail, Strathern Jeffrey N

机构信息

NCI Center for Cancer Research, Frederick, Maryland, United States of America; U.S. Army Medical Research and Materiel Command, Fort Detrick, Maryland, United States of America.

NCI Center for Cancer Research, Frederick, Maryland, United States of America.

出版信息

PLoS Genet. 2014 Sep 18;10(9):e1004532. doi: 10.1371/journal.pgen.1004532. eCollection 2014 Sep.

DOI:10.1371/journal.pgen.1004532

PMID:25232834

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4168980/

Abstract

We developed a highly sensitive assay to detect transcription errors in vivo. The assay is based on suppression of a missense mutation in the active site tyrosine in the Cre recombinase. Because Cre acts as tetramer, background from translation errors are negligible. Functional Cre resulting from rare transcription errors that restore the tyrosine codon can be detected by Cre-dependent rearrangement of reporter genes. Hence, transient transcription errors are captured as stable genetic changes. We used this Cre-based reporter to screen for mutations of Saccharomyces cerevisiae RPB1 (RPO21) that increase the level of misincorporation during transcription. The mutations are in three domains of Rpb1, the trigger loop, the bridge helix, and in sites involved in binding to TFIIS. Biochemical characterization demonstrates that these variants have elevated misincorporation, and/or ability to extend mispaired bases, or defects in TFIIS mediated editing.

摘要

我们开发了一种高灵敏度的检测方法来检测体内转录错误。该检测方法基于对Cre重组酶活性位点酪氨酸处错义突变的抑制。由于Cre以四聚体形式发挥作用，翻译错误产生的背景可以忽略不计。由罕见转录错误恢复酪氨酸密码子而产生的功能性Cre可通过报告基因的Cre依赖性重排来检测。因此，瞬时转录错误被捕获为稳定的基因变化。我们使用这种基于Cre的报告基因来筛选酿酒酵母RPB1（RPO21）的突变，这些突变会增加转录过程中错误掺入的水平。这些突变位于Rpb1的三个结构域中，即触发环、桥螺旋以及与TFIIS结合的位点。生化特性表明，这些变体具有更高的错误掺入率和/或延伸错配碱基的能力，或者在TFIIS介导的编辑中存在缺陷。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a289/4168980/f90f0792fce2/pgen.1004532.g001.jpg

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一种用于转录错误的基因检测揭示了RNA聚合酶II保真度的多层控制。

A genetic assay for transcription errors reveals multilayer control of RNA polymerase II fidelity.

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