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通过人拓扑异构酶I的帽状结构域和催化结构域的结合来恢复酶活性。

Reconstitution of enzymatic activity by the association of the cap and catalytic domains of human topoisomerase I.

作者信息

Yang Zheng, Champoux James J

机构信息

Department of Microbiology, School of Medicine, University of Washington, Seattle, WA 98195-7242, USA.

出版信息

J Biol Chem. 2002 Aug 23;277(34):30815-23. doi: 10.1074/jbc.M205302200. Epub 2002 Jun 19.

Abstract

When human topoisomerase I binds DNA, two opposing lobes in the enzyme, the cap region (amino acid, residues 175-433) and the catalytic domain (Deltacap, residues 433 to the COOH terminus) clamp tightly around the DNA helix to form the precleavage complex. Although Deltacap contains all of the residues known to be important for catalysis and binds DNA with an affinity similar to that of the intact enzyme, this fragment lacks catalytic activity. However, a mixture of Deltacap and topo31 (residues 175-433) reconstitutes enzymatic activity as measured by plasmid DNA relaxation and suicide cleavage assays. Although the formation of an active complex between topo31 and Deltacap is too unstable to be detected by pull-down experiments even in the presence of DNA, the association of topo31 with Deltacap persists and is detectable after the complex catalyzes the covalent attachment of the DNA to Deltacap by suicide cleavage. Removal of topo31 from Deltacap-DNA after suicide cleavage reveals that, unlike the cleavage reaction, religation does not require the cap region of the protein. These results suggest that activation of the catalytic domain of the enzyme for cleavage requires both DNA binding and the presence of the cap region of the protein.

摘要

当人类拓扑异构酶I与DNA结合时,该酶中的两个相对叶,即帽区(氨基酸残基175 - 433)和催化结构域(Deltacap,残基433至COOH末端)紧紧围绕DNA螺旋形成预切割复合物。尽管Deltacap包含所有已知对催化重要的残基,并且以与完整酶相似的亲和力结合DNA,但该片段缺乏催化活性。然而,通过质粒DNA松弛和自杀切割试验测量,Deltacap和topo31(残基175 - 433)的混合物可重构酶活性。尽管即使在存在DNA的情况下,通过下拉实验也无法检测到topo31和Deltacap之间形成的活性复合物足够稳定,但topo31与Deltacap的结合持续存在,并且在复合物通过自杀切割催化DNA与Deltacap的共价连接后可被检测到。自杀切割后从Deltacap - DNA中去除topo31表明,与切割反应不同,重新连接不需要蛋白质的帽区。这些结果表明,酶催化结构域的切割激活需要DNA结合和蛋白质帽区的存在。

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