The Kinetic Mechanism of 3′-5′ Exonucleolytic Activity of AP Endonuclease Nfo from E. coli

AP站点 基底切除修复术 DNA糖基化酶 核酸外切酶 生物化学 AP核酸内切酶 核苷酸 DNA DNA修复 化学 核酸外切酶 III 排尿 DNA-(无嘌呤或无嘧啶位点)裂解酶 核酸内切酶 DNA损伤 核苷酸切除修复 脱氧核糖 磷酸二酯键 大肠杆菌 DNA聚合酶 核糖核酸 基因
作者
Svetlana I. Senchurova,А. А. Кузнецова,А. А. Ищенко,Murat Saparbaev,Olga S. Fedorova,Nikita А. Kuznetsov
出处
期刊:Cells [MDPI AG]
卷期号:11 (19): 2998-2998 被引量:3
标识
DOI:10.3390/cells11192998
摘要

Escherichia coli apurinic/apyrimidinic (AP) endonuclease Nfo is one of the key participants in DNA repair. The principal biological role of this enzyme is the recognition and hydrolysis of AP sites, which arise in DNA either as a result of the spontaneous hydrolysis of an N-glycosidic bond with intact nitrogenous bases or under the action of DNA glycosylases, which eliminate various damaged bases during base excision repair. Nfo also removes 3'-terminal blocking groups resulting from AP lyase activity of DNA glycosylases. Additionally, Nfo can hydrolyze the phosphodiester linkage on the 5' side of some damaged nucleotides on the nucleotide incision repair pathway. The function of 3'-5'-exonuclease activity of Nfo remains unclear and probably consists of participation (together with the nucleotide incision repair activity) in the repair of cluster lesions. In this work, using polyacrylamide gel electrophoresis and the stopped-flow method, we analyzed the kinetics of the interaction of Nfo with various model DNA substrates containing a 5' single-stranded region. These data helped to describe the mechanism of nucleotide cleavage and to determine the rates of the corresponding stages. It was revealed that the rate-limiting stage of the enzymatic process is a dissociation of the reaction product from the enzyme active site. The stability of the terminal pair of nucleotides in the substrate did not affect the enzymatic-reaction rate. Finally, it was found that 2'-deoxynucleoside monophosphates can effectively inhibit the 3'-5'-exonuclease activity of Nfo.
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