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一种杂合突变体EcoRI核酸内切酶增强DNA结合的结构和热力学基础。

Structural and thermodynamic basis for enhanced DNA binding by a promiscuous mutant EcoRI endonuclease.

作者信息

Sapienza Paul J, Rosenberg John M, Jen-Jacobson Linda

机构信息

Department of Biological Sciences, University of Pittsburgh, Pittsburgh, PA 15260, USA.

出版信息

Structure. 2007 Nov;15(11):1368-82. doi: 10.1016/j.str.2007.09.014.

Abstract

Promiscuous mutant EcoRI endonucleases bind to the canonical site GAATTC more tightly than does the wild-type endonuclease, yet cleave variant (EcoRI()) sites more rapidly than does wild-type. The crystal structure of the A138T promiscuous mutant homodimer in complex with a GAATTC site is nearly identical to that of the wild-type complex, except that the Thr138 side chains make packing interactions with bases in the 5'-flanking regions outside the recognition hexanucleotide while excluding two bound water molecules seen in the wild-type complex. Molecular dynamics simulations confirm exclusion of these waters. The structure and simulations suggest possible reasons why binding of the A138T protein to the GAATTC site has DeltaS degrees more favorable and DeltaH degrees less favorable than for wild-type endonuclease binding. The interactions of Thr138 with flanking bases may permit A138T, unlike wild-type enzyme, to form complexes with EcoRI() sites that structurally resemble the specific wild-type complex with GAATTC.

摘要

杂乱突变的EcoRI核酸内切酶与典型位点GAATTC的结合比野生型核酸内切酶更紧密,但切割变体(EcoRI())位点的速度比野生型更快。A138T杂乱突变体同二聚体与GAATTC位点形成复合物的晶体结构与野生型复合物几乎相同,只是Thr138侧链与识别六核苷酸外侧5'侧翼区域的碱基形成堆积相互作用,同时排除了野生型复合物中可见的两个结合水分子。分子动力学模拟证实了这些水分子的排除。该结构和模拟结果表明了A138T蛋白与GAATTC位点结合时的ΔS°比野生型核酸内切酶结合更有利且ΔH°更不利的可能原因。与野生型酶不同,Thr138与侧翼碱基的相互作用可能使A138T能够与EcoRI()位点形成结构上类似于与GAATTC形成的特异性野生型复合物的复合物。

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