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Architecture of the Yeast RNA Polymerase II Open Complex and Regulation of Activity by TFIIF

机译:酵母RNA聚合酶II开放复合体的体系结构和TFIIF对活性的调节

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摘要

To investigate the function and architecture of the open complex state of RNA polymerase II (Pol II), Saccharomyces cerevisiae minimal open complexes were assembled by using a series of heteroduplex HIS4 promoters, TATA binding protein (TBP), TFIIB, and Pol II. The yeast system demonstrates great flexibility in the position of active open complexes, spanning 30 to 80 bp downstream from TATA, consistent with the transcription start site scanning behavior of yeast Pol II. TFIIF unexpectedly modulates the activity of the open complexes, either repressing or stimulating initiation. The response to TFIIF was dependent on the sequence of the template strand within the single-stranded bubble. Mutations in the TFIIB reader and linker region, which were inactive on duplex DNA, were suppressed by the heteroduplex templates, showing that a major function of the TFIIB reader and linker is in the initiation or stabilization of single-stranded DNA. Probing of the architecture of the minimal open complexes with TFIIB-FeBABE [TFIIB–p-bromoacetamidobenzyl–EDTA-iron(III)] derivatives showed that the TFIIB core domain is surprisingly positioned away from Pol II, and the addition of TFIIF repositions the TFIIB core domain to the Pol II wall domain. Together, our results show an unexpected architecture of minimal open complexes and the regulation of activity by TFIIF and the TFIIB core domain.
机译:为了研究RNA聚合酶II(Pol II)开放复合体状态的功能和结构,通过使用一系列异源双链体HIS4启动子,TATA结合蛋白(TBP),TFIIB和Pol II,将酿酒酵母的最小开放复合体组装在一起。酵母系统显示出活性开放复合物的位置具有很大的灵活性,与TATA下游的转录起始位点扫描行为一致,该活性开放复合物位于TATA下游30到80 bp之间。 TFIIF意外地调节了开放复合物的活性,从而抑制或刺激了起始。对TFIIF的反应取决于单链气泡中模板链的序列。异源双链体模板抑制了在双链DNA上无活性的TFIIB阅读器和接头区域中的突变,表明TFIIB阅读器和接头的主要功能在于单链DNA的起始或稳定。用TFIIB-FeBABE [TFIIB–p-溴乙酰氨基苄基–EDTA-铁(III)]衍生物对最小开放络合物的体系结构进行的研究表明,TFIIB核心域的位置出乎意料地远离Pol II,并且添加TFIIF可以重新定位TFIIB核心域到Pol II墙域。在一起,我们的结果显示了最小开放复合体的意外架构以及TFIIF和TFIIB核心域对活性的调节。

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