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限制性内切酶在特定位点DNA切割中进行间接识别的结构和能量起源

Structural and energetic origins of indirect readout in site-specific DNA cleavage by a restriction endonuclease.

作者信息

Martin A M, Sam M D, Reich N O, Perona J J

机构信息

Department of Chemistry, University of California at Santa Barbara, 93106-9510, USA.

出版信息

Nat Struct Biol. 1999 Mar;6(3):269-77. doi: 10.1038/6707.

Abstract

Specific recognition by EcoRV endonuclease of its cognate, sharply bent GATATC site at the center TA step occurs solely via hydrophobic interaction with thymine methyl groups. Mechanistic kinetic analyses of base analog-substituted DNAs at this position reveal that direct readout provides 5 kcal mol(-1) toward specificity, with an additional 6-10 kcal mol(-1) arising from indirect readout. Crystal structures of several base analog complexes show that the major-groove hydrophobic contacts are crucial to forming required divalent metal-binding sites, and that indirect readout operates in part through the sequence-dependent free-energy cost of unstacking the center base-pair step of the DNA.

摘要

EcoRV 核酸内切酶对其同源的、在中心 TA 步处急剧弯曲的 GATATC 位点的特异性识别仅通过与胸腺嘧啶甲基基团的疏水相互作用发生。对该位置碱基类似物取代的 DNA 进行的机制动力学分析表明,直接读出为特异性提供了 5 千卡/摩尔(-1)的能量,另外 6 - 10 千卡/摩尔(-1)来自间接读出。几种碱基类似物复合物的晶体结构表明,大沟疏水接触对于形成所需的二价金属结合位点至关重要,并且间接读出部分通过 DNA 中心碱基对步的解堆叠的序列依赖性自由能成本起作用。

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