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噬菌体T4 RNA连接酶2的RNA底物特异性及结构导向的突变分析

RNA substrate specificity and structure-guided mutational analysis of bacteriophage T4 RNA ligase 2.

作者信息

Nandakumar Jayakrishnan, Ho C Kiong, Lima Christopher D, Shuman Stewart

机构信息

Molecular Biology and Structural Biology Programs, Sloan-Kettering Institute, New York, New York 10021, USA.

出版信息

J Biol Chem. 2004 Jul 23;279(30):31337-47. doi: 10.1074/jbc.M402394200. Epub 2004 Apr 13.

Abstract

Here we report that bacteriophage T4 RNA ligase 2 (Rnl2) is an efficient catalyst of RNA ligation at a 3'-OH/5'-PO(4) nick in a double-stranded RNA or an RNA.DNA hybrid. The critical role of the template strand in approximating the reactive 3'-OH and 5'-PO(4) termini is underscored by the drastic reductions in the RNA-sealing activity of Rnl2 when the duplex substrates contain gaps or flaps instead of nicks. RNA nick joining requires ATP and a divalent cation cofactor (either Mg or Mn). Neither dATP, GTP, CTP, nor UTP can substitute for ATP. We identify by alanine scanning seven functionally important amino acids (Tyr-5, Arg-33, Lys-54, Gln-106, Asp-135, Arg-155, and Ser-170) within the N-terminal nucleotidyl-transferase domain of Rnl2 and impute specific roles for these residues based on the crystal structure of the AMP-bound enzyme. Mutational analysis of 14 conserved residues in the C-terminal domain of Rnl2 identifies 3 amino acids (Arg-266, Asp-292, and Glu-296) as essential for ligase activity. Our findings consolidate the evolutionary connections between bacteriophage Rnl2 and the RNA-editing ligases of kinetoplastid protozoa.

摘要

在此我们报告,噬菌体T4 RNA连接酶2(Rnl2)是双链RNA或RNA·DNA杂交体中3'-OH/5'-PO(4)切口处RNA连接的高效催化剂。当双链底物含有缺口或侧翼而非切口时,Rnl2的RNA封闭活性急剧降低,这突出了模板链在使反应性3'-OH和5'-PO(4)末端靠近方面的关键作用。RNA切口连接需要ATP和二价阳离子辅因子(Mg或Mn)。dATP、GTP、CTP和UTP均不能替代ATP。我们通过丙氨酸扫描确定了Rnl2 N端核苷酸转移酶结构域内七个功能上重要的氨基酸(Tyr-5、Arg-33、Lys-54、Gln-106、Asp-135、Arg-155和Ser-170),并根据与AMP结合的酶的晶体结构推测了这些残基的特定作用。对Rnl2 C端结构域中14个保守残基的突变分析确定了3个氨基酸(Arg-266、Asp-292和Glu-296)是连接酶活性所必需的。我们的发现巩固了噬菌体Rnl2与动质体原生动物的RNA编辑连接酶之间的进化联系。

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