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哺乳动物胞嘧啶DNA甲基转移酶Dnmt1:酶促机制、新型基于机制的抑制剂以及RNA指导的DNA甲基化

Mammalian cytosine DNA methyltransferase Dnmt1: enzymatic mechanism, novel mechanism-based inhibitors, and RNA-directed DNA methylation.

作者信息

Svedruzić Zeljko M

机构信息

Department of Biophysics and Biochemistry, Washington State University, Pullman, WA 99164, USA.

出版信息

Curr Med Chem. 2008;15(1):92-106. doi: 10.2174/092986708783330700.

DOI:10.2174/092986708783330700
PMID:18220765
Abstract

This is a review of the enzymatic mechanism of DNA methyltransferase Dnmt1 and analysis of its implications on regulation of DNA methylation in mammalian cells and design of novel mechanism-based inhibitors. The methylation reaction by Dnmt1 has different phases that depend on DNA substrate and allosteric regulation. Consequently, depending on the phase, the differences in catalytic rates between unmethylated and pre-methylated DNA can vary between 30-40 fold, 3-6 fold or only 1 fold. The allosteric site and the active site can bind different molecules. Allosteric activity depends on DNA sequence, methylation pattern and DNA structure (single stranded vs. double stranded). Dnmt1 binds poly(ADP-ribose) and some RNA molecules. The results on kinetic preferences, allosteric activity and binding preference of Dnmt1 are combined together in one comprehensive model mechanism that can address regulation of DNA methylation in cells; namely, inhibition of DNA methylation by poly(ADP-ribose), RNA-directed DNA methylation by methylated and unmethylated non-coding RNA molecules, and transient interactions between Dnmt1 and genomic DNA. Analysis of reaction intermediates showed that equilibrium between base-flipping and base-restacking events can be the key mechanism in control of enzymatic activity. The two events have equal but opposite effect on accumulation of early reaction intermediates and methylation rates. The accumulation of early reaction intermediates can be exploited to improve the current inhibitors of Dnmt1 and achieve inhibition without toxic modifications in genomic DNA. [1,2-dihydropyrimidin-2-one]-5-methylene-(methylsulfonium)-adenosyl is described as the lead compound.

摘要

本文综述了DNA甲基转移酶Dnmt1的酶促机制,分析了其对哺乳动物细胞DNA甲基化调控的影响,并设计了基于新机制的抑制剂。Dnmt1催化的甲基化反应有不同阶段,这取决于DNA底物和变构调节。因此,根据阶段不同,未甲基化和预甲基化DNA之间的催化速率差异可能在30至40倍、3至6倍或仅1倍之间变化。变构位点和活性位点可结合不同分子。变构活性取决于DNA序列、甲基化模式和DNA结构(单链与双链)。Dnmt1可结合聚(ADP - 核糖)和一些RNA分子。将Dnmt1的动力学偏好、变构活性和结合偏好的研究结果整合到一个综合模型机制中,该机制可解释细胞中DNA甲基化的调控;即聚(ADP - 核糖)对DNA甲基化的抑制作用、甲基化和未甲基化非编码RNA分子介导的RNA指导的DNA甲基化,以及Dnmt1与基因组DNA之间的瞬时相互作用。对反应中间体的分析表明,碱基翻转和碱基重新堆积事件之间的平衡可能是控制酶活性的关键机制。这两个事件对早期反应中间体的积累和甲基化速率具有相等但相反的影响。早期反应中间体的积累可用于改进目前的Dnmt1抑制剂,并在不产生基因组DNA毒性修饰的情况下实现抑制作用。[1,2 - 二氢嘧啶 - 2 - 酮]-5 - 亚甲基 -(甲基硫鎓)-腺苷被描述为先导化合物。

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