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DNA修复酶核酸内切酶III晶体结构中的新型DNA结合基序。

Novel DNA binding motifs in the DNA repair enzyme endonuclease III crystal structure.

作者信息

Thayer M M, Ahern H, Xing D, Cunningham R P, Tainer J A

机构信息

Scripps Research Institute, Department of Molecular Biology-MB4, La Jolla, CA 92037, USA.

出版信息

EMBO J. 1995 Aug 15;14(16):4108-20. doi: 10.1002/j.1460-2075.1995.tb00083.x.

Abstract

The 1.85 A crystal structure of endonuclease III, combined with mutational analysis, suggests the structural basis for the DNA binding and catalytic activity of the enzyme. Helix-hairpin-helix (HhH) and [4Fe-4S] cluster loop (FCL) motifs, which we have named for their secondary structure, bracket the cleft separating the two alpha-helical domains of the enzyme. These two novel DNA binding motifs and the solvent-filled pocket in the cleft between them all lie within a positively charged and sequence-conserved surface region. Lys120 and Asp138, both shown by mutagenesis to be catalytically important, lie at the mouth of this pocket, suggesting that this pocket is part of the active site. The positions of the HhH motif and protruding FCL motif, which contains the DNA binding residue Lys191, can accommodate B-form DNA, with a flipped-out base bound within the active site pocket. The identification of HhH and FCL sequence patterns in other DNA binding proteins suggests that these motifs may be a recurrent structural theme for DNA binding proteins.

摘要

核酸内切酶III的1.85埃晶体结构,结合突变分析,揭示了该酶DNA结合和催化活性的结构基础。我们根据其二级结构命名的螺旋-发夹-螺旋(HhH)和[4Fe-4S]簇环(FCL)基序,包围着分隔该酶两个α-螺旋结构域的裂隙。这两个新颖的DNA结合基序以及它们之间裂隙中的溶剂填充口袋,都位于一个带正电荷且序列保守的表面区域内。通过诱变显示对催化作用很重要的赖氨酸120和天冬氨酸138,位于这个口袋的开口处,表明这个口袋是活性位点的一部分。HhH基序和突出的FCL基序(包含DNA结合残基赖氨酸191)的位置,可以容纳B型DNA,其中一个翻转出来的碱基结合在活性位点口袋内。在其他DNA结合蛋白中对HhH和FCL序列模式的鉴定表明,这些基序可能是DNA结合蛋白中反复出现的结构主题。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/161b/394490/a8173d83d4bc/emboj00040-0268-a.jpg

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