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人烷基化修复蛋白同源物1(ALKBH1)的AP裂解酶和mA去甲基酶活性的生化特性

Biochemical Characterization of AP Lyase and mA Demethylase Activities of Human AlkB Homologue 1 (ALKBH1).

作者信息

Müller Tina A, Tobar Michael A, Perian Madison N, Hausinger Robert P

机构信息

Department of Microbiology and Molecular Genetics, Michigan State University , East Lansing, Michigan 48824, United States.

Biology Department, Kalamazoo College , Kalamazoo, Michigan 49006, United States.

出版信息

Biochemistry. 2017 Apr 4;56(13):1899-1910. doi: 10.1021/acs.biochem.7b00060. Epub 2017 Mar 21.

DOI:10.1021/acs.biochem.7b00060
PMID:28290676
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5444387/
Abstract

Alkbh1 is one of nine mammalian homologues of Escherichia coli AlkB, a 2-oxoglutarate-dependent dioxygenase that catalyzes direct DNA repair by removing alkyl lesions from DNA. Six distinct enzymatic activities have been reported for Alkbh1, including hydroxylation of variously methylated DNA, mRNA, tRNA, or histone substrates along with the cleavage of DNA at apurinic/apyrimidinic (AP) sites followed by covalent attachment to the 5'-product. The studies described here extend the biochemical characterization of two of these enzymatic activities using human ALKBH1: the AP lyase and 6-methyl adenine DNA demethylase activities. The steady-state and single-turnover kinetic parameters for ALKBH1 cleavage of AP sites in DNA were determined and shown to be comparable to those of other AP lyases. The α,β-unsaturated aldehyde of the 5'-product arising from DNA cleavage reacts predominantly with C129 of ALKBH1, but secondary sites also generate covalent adducts. The 6-methyl adenine demethylase activity was examined with a newly developed assay using a methylation-sensitive restriction endonuclease, and the enzymatic rate was found to be very low. Indeed, the demethylase activity was less than half that of the AP lyase activity when ALKBH1 samples were assayed using identical buffer conditions. The two enzymatic activities were examined using a series of site-directed variant proteins, revealing the presence of distinct but partially overlapping active sites for the two reactions. We postulate that the very low 6-methyl adenine oxygenase activity associated with ALKBH1 is unlikely to represent the major function of the enzyme in the cell, while the cellular role of the lyase activity (including its subsequent covalent attachment to DNA) remains uncertain.

摘要

Alkbh1是大肠杆菌AlkB的九个哺乳动物同源物之一,AlkB是一种依赖于2-氧代戊二酸的双加氧酶,通过从DNA中去除烷基损伤来催化直接DNA修复。已报道Alkbh1具有六种不同的酶活性,包括对各种甲基化的DNA、mRNA、tRNA或组蛋白底物进行羟基化,以及在无嘌呤/无嘧啶(AP)位点切割DNA,随后与5'-产物共价连接。本文所述的研究扩展了对人ALKBH1的其中两种酶活性的生化特性研究:AP裂解酶活性和6-甲基腺嘌呤DNA去甲基酶活性。测定了ALKBH1切割DNA中AP位点的稳态和单周转动力学参数,结果表明这些参数与其他AP裂解酶的参数相当。DNA切割产生的5'-产物的α,β-不饱和醛主要与ALKBH1的C129反应,但次要位点也会生成共价加合物。使用一种新开发的基于甲基化敏感限制性内切酶的测定方法检测了6-甲基腺嘌呤去甲基酶活性,发现酶促反应速率非常低。实际上,当在相同缓冲条件下测定ALKBH1样品时,去甲基酶活性不到AP裂解酶活性的一半。使用一系列定点变体蛋白检测了这两种酶活性,结果表明这两个反应存在不同但部分重叠的活性位点。我们推测,与ALKBH1相关的极低的6-甲基腺嘌呤加氧酶活性不太可能代表该酶在细胞中的主要功能,而裂解酶活性(包括其随后与DNA的共价连接)在细胞中的作用仍不确定。

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