Pre-steady-state kinetic analysis of damage recognition by human single-strand selective monofunctional uracil-DNA glycosylase SMUG1†

IF 3.743 Q2 Biochemistry, Genetics and Molecular Biology Molecular BioSystems Pub Date : 2017-10-11 DOI:10.1039/C7MB00457E
Alexandra A. Kuznetsova, Danila A. Iakovlev, Inna V. Misovets, Alexander A. Ishchenko, Murat K. Saparbaev, Nikita A. Kuznetsov and Olga S. Fedorova
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引用次数: 22

Abstract

In all organisms, DNA glycosylases initiate base excision repair pathways resulting in removal of aberrant bases from DNA. Human SMUG1 belongs to the superfamily of uracil-DNA glycosylases catalyzing the hydrolysis of the N-glycosidic bond of uridine and uridine lesions bearing oxidized groups at C5: 5-hydroxymethyluridine (5hmU), 5-formyluridine (5fU), and 5-hydroxyuridine (5hoU). An apurinic/apyrimidinic (AP) site formed as the product of an N-glycosylase reaction is tightly bound to hSMUG1, thus inhibiting the downstream action of AP-endonuclease APE1. The steady-state kinetic parameters (kcat and KM; obtained from the literature) correspond to the enzyme turnover process limited by the release of hSMUG1 from the complex with the AP-site. In the present study, our objective was to carry out a stopped-flow fluorescence analysis of the interaction of hSMUG1 with a DNA substrate containing a dU:dG base pair to follow the pre-steady-state kinetics of conformational changes in both molecules. A comparison of kinetic data obtained by means of Trp and 2-aminopurine fluorescence and F?rster resonance energy transfer (FRET) detection allowed us to elucidate the stages of specific and nonspecific DNA binding, to propose the mechanism of damaged base recognition by hSMUG1, and to determine the true rate of the catalytic step. Our results shed light on the kinetic mechanism underlying the initiation of base excision repair by hSMUG1 using the “wedge” strategy for DNA lesion search.

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人单链选择性单功能尿嘧啶- dna糖基酶SMUG1†损伤识别的预稳态动力学分析
在所有生物体中,DNA糖基酶启动碱基切除修复途径,导致从DNA中去除异常碱基。人类SMUG1属于尿嘧啶- dna糖基酶的超家族,它催化尿嘧啶和尿嘧啶的n -糖苷键的水解,尿嘧啶的C5氧化基团为5-羟甲基尿嘧啶(5hmU)、5-甲酰基尿嘧啶(5fU)和5-羟尿嘧啶(5hoU)。作为n -糖基化酶反应产物形成的apurinic/apyrimidinic (AP)位点与hSMUG1紧密结合,从而抑制AP内切酶APE1的下游作用。稳态动力学参数(kcat和KM;从文献中获得)对应于酶周转过程,该过程受到hSMUG1从ap位点复合物释放的限制。在本研究中,我们的目的是对hSMUG1与含有dU:dG碱基对的DNA底物的相互作用进行停流荧光分析,以跟踪两个分子的预稳态构象变化动力学。色氨酸和2-氨基嘌呤荧光与F?ster共振能量转移(FRET)检测使我们能够阐明特异性和非特异性DNA结合的阶段,提出hSMUG1识别受损碱基的机制,并确定催化步骤的真实速率。我们的研究结果揭示了hSMUG1使用DNA损伤搜索的“楔子”策略启动碱基切除修复的动力学机制。
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来源期刊
Molecular BioSystems
Molecular BioSystems 生物-生化与分子生物学
CiteScore
2.94
自引率
0.00%
发文量
0
审稿时长
2.6 months
期刊介绍: Molecular Omics publishes molecular level experimental and bioinformatics research in the -omics sciences, including genomics, proteomics, transcriptomics and metabolomics. We will also welcome multidisciplinary papers presenting studies combining different types of omics, or the interface of omics and other fields such as systems biology or chemical biology.
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