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Functional architecture of RNA polymerase I

机译:RNA聚合酶I的功能结构

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Synthesis of ribosomal RNA (rRNA) by RNA polymerase (Pol) I is the first step in ribosome biogenesis and a regulatory switch in eukaryotic cell growth. Here we report the 12 angstrom cryoelectron microscopic structure for the complete 14-subunit yeast Pol I, a homology model for the core enzyme, and the crystal structure of the subcomplex A14/43. In the resulting hybrid structure of Pol I, A14/43, the clamp, and the dock domain contribute to a unique surface interacting with promoter-specific initiation factors. The Pol I-specific subunits A49 and A34.5 form a heterodimer near the enzyme funnel that acts as a built-in elongation factor and is related to the Pol II-associated factor TFIIF. In contrast to Pol II, Pol I has a strong intrinsic 3'-RNA cleavage activity, which requires the C-terminal domain of subunit A12.2 and, apparently, enables ribosomal RNA proofreading and 3'-end trimming.
机译:RNA聚合酶(Pol)I合成核糖体RNA(rRNA)是核糖体生物发生的第一步,也是真核细胞生长中的调控开关。在这里,我们报告了完整的14个亚基酵母Pol I的12埃低温电子显微结构,核心酶的同源性模型以及亚复合物A14 / 43的晶体结构。在所得的Pol I杂合结构中,A14 / 43,钳位和对接结构域有助于与启动子特异性起始因子相互作用的独特表面。 Pol I特异的亚基A49和A34.5在酶漏斗附近形成异二聚体,它充当内置的延伸因子,并与Pol II相关因子TFIIF相关。与Pol II相比,Pol I具有很强的内在3'-RNA裂解活性,这需要亚基A12.2的C端结构域,并且显然可以进行核糖体RNA校对和3'-端修剪。

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