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通过靶向分子动力学探究mRNA加帽酶中催化必需的构象动力学。

Catalytically requisite conformational dynamics in the mRNA-capping enzyme probed by targeted molecular dynamics.

作者信息

Swift Robert V, McCammon J Andrew

机构信息

Department of Chemistry and Biochemistry, University of California at San Diego, La Jolla, California, 92039-0365, USA.

出版信息

Biochemistry. 2008 Apr 1;47(13):4102-11. doi: 10.1021/bi8000209. Epub 2008 Mar 11.

DOI:10.1021/bi8000209
PMID:18330997
Abstract

The addition of a N7-methyl guanosine cap to the 5' end of nascent mRNA is carried out by the mRNA-capping enzyme, a two-domain protein that is a member of the nucleotidyltransferase superfamily. The mRNA-capping enzyme is composed of a catalytic nucleotidyltransferase domain and a noncatalytic oligonucleotide/oligosaccharide binding (OB) domain. Large-scale domain motion triggered by substrate binding mediates catalytically requisite conformational rearrangement of the GTP substrate prior to the chemical step. In this study, we employ targeted molecular dynamics (TMD) on the PBCV-1 capping enzyme to probe the global domain dynamics and internal dynamics of conserved residues during the conformational transformation from the open to the closed state. Analysis of the resulting trajectories along with structural and sequence homology to other members of the superfamily allows us to suggest a conserved mechanism of conformational rearrangements spanning all mRNA-capping enzymes and all ATP-dependent DNA ligases. Our results suggest that the OB domain moves quasi-statically toward the nucleotidyltransferase domain, pivoting about a short linker region. The approach of the OB domain brings a conserved RxDK sequence, an element of conserved motif VI, within proximity of the triphosphate of GTP, destabilizing the unreactive conformation and thereby allowing thermal fluctuations to partition the substrate toward the catalytically competent state.

摘要

在新生mRNA的5'端添加N7-甲基鸟苷帽是由mRNA加帽酶完成的,该酶是一种双结构域蛋白,属于核苷酸转移酶超家族。mRNA加帽酶由一个催化性核苷酸转移酶结构域和一个非催化性寡核苷酸/寡糖结合(OB)结构域组成。底物结合引发的大规模结构域运动介导了化学步骤之前GTP底物的催化必需构象重排。在本研究中,我们对PBCV-1加帽酶进行靶向分子动力学(TMD),以探究从开放状态到封闭状态的构象转变过程中保守残基的全局结构域动力学和内部动力学。对所得轨迹的分析以及与超家族其他成员的结构和序列同源性分析,使我们能够提出一种跨越所有mRNA加帽酶和所有ATP依赖性DNA连接酶的保守构象重排机制。我们的结果表明,OB结构域围绕一个短连接区域旋转,准静态地向核苷酸转移酶结构域移动。OB结构域的靠近使保守的RxDK序列(保守基序VI的一个元件)靠近GTP的三磷酸基团,破坏了无反应性的构象,从而使热涨落将底物导向催化活性状态。

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