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The highly conserved glutamic acid 791 of Rpb2 is involved in the binding of NTP and Mg(B) in the active center of human RNA polymerase II

机译:Rpb2的高度保守的谷氨酸791在人RNA聚合酶II的活性中心参与NTP和Mg(B)的结合

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摘要

During transcription by RNA polymerase (RNAP) II, the incoming ribonucleoside triphosphate (NTP) enters the catalytic center in association with an Mg2+ ion, termed metal B [Mg(B)]. When bound to RNAP II, Mg(B) is coordinated by the β and γ phosphates of the NTP, Rpb1 residues D481 and D483 and Rpb2 residue D837. Rpb2 residue D837 is highly conserved across species. Notably, its neighboring residue, E836 (E791 in human RNAP II), is also highly conserved. To probe the role of E791 in transcription, we have affinity purified and characterized a human RNAP II mutant in which this residue was substituted for alanine. Our results indicate that the transcription activity of the Rpb2 E791A mutant is impaired at low NTP concentrations both in vitro and in vivo. They also revealed that both its NTP polymerization and transcript cleavage activities are decreased at low Mg concentrations. Because Rpb2 residue E791 appears to be located too far from the NTP–Mg(B) complex to make direct contact at either the entry (E) or addition (A) site, we propose alternative mechanisms by which this highly conserved residue participates in loading NTP–Mg(B) in the active site during transcription.
机译:在通过RNA聚合酶(RNAP)II转录的过程中,传入的核糖核苷三磷酸(NTP)与称为金属B [Mg(B)]的Mg2 +离子一起进入催化中心。当与RNAP II结合时,Mg(B)由NTP,Rpb1残基D481和D483和Rpb2残基D837的β和γ磷酸配位。 Rpb2残基D837在物种间高度保守。值得注意的是,它的相邻残基E836(人RNAP II中的E791)也高度保守。为了探测E791在转录中的作用,我们进行了亲和纯化并鉴定了一个人类RNAP II突变体,其中该残基取代了丙氨酸。我们的结果表明,在体外和体内,在低NTP浓度下,Rpb2 E791A突变体的转录活性都会受到损害。他们还发现,在低镁浓度下,其NTP聚合和转录物裂解活性均降低。由于Rpb2残基E791似乎距离NTP–Mg(B)复合物太远,无法在入口(E)或加成(A)位置直接接触,因此我们提出了这种高度保守的残基参与装载的替代机制转录过程中活动位点中的NTP–Mg(B)。

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