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首页> 外文期刊>Nucleic Acids Research >Branch site bulge conformations in domain 6 determine functional sugar puckers in group II intron splicing
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Branch site bulge conformations in domain 6 determine functional sugar puckers in group II intron splicing

机译:结构域6中的分支站点凸起构象确定II组内含子拼接的功能糖褶皱

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Although group II intron ribozymes are intensively studied the question how structural dynamics affects splicing catalysis has remained elusive. We report for the first time that the group II intron domain 6 exists in a secondary structure equilibrium between a single- and a two-nucleotide bulge conformation, which is directly linked to a switch between sugar puckers of the branch site adenosine. Our study determined a functional sugar pucker equilibrium between the transesterification active C2 '-endo conformation of the branch site adenosine in the 1nt bulge and an inactive C3 '-endo state in the 2nt bulge fold, allowing the group II intron to switch its activity from the branching to the exon ligation step. Our detailed NMR spectroscopic investigation identified magnesium (II) ions and the branching reaction as regulators of the equilibrium populations. The tuneable secondary structure/sugar pucker equilibrium supports a conformational selection mechanism to up- and downregulate catalytically active and inactive states of the branch site adenosine to orchestrate the multi-step splicing process. The conformational dynamics of group II intron domain 6 is also proposed to be a key aspect for the directionality selection in reversible splicing.
机译:虽然II族内含子核素核素研究了结构动态如何影响剪接催化仍然难以捉摸。我们首次报告了第II族内部结构域6在单核苷酸和双核苷酸凸起构象之间的二级结构平衡中,其与分支位点腺苷的糖褶皱之间的开关直接连接。我们的研究确定了在2NT凸起中的酯交换活性C2'-Endo构象之间的酯交换活性C2'-Endo构象与2NT凸起折叠中的非活性C3'-Endo状态,允许II族内含子切换其活动分支到外显子结扎步骤。我们详细的NMR光谱研究确定了镁(II)离子和支化反应作为平衡群的调节剂。可调谐的二级结构/糖褶皱平衡支持构象选择机制,以升高和下调分支位点腺苷的催化活性和无活性状态,以协调多步拼接过程。 II族内部区域6的构象动态也被提出为可逆剪接方向性选择的关键方面。

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