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DNA 甲基转移酶:从动力学分析中得出的机制模型。

DNA methyltransferases: mechanistic models derived from kinetic analysis.

机构信息

Institute of Molecular Biology, State Research Center of Virology and Biotechnology Vector, Novosibirsk, Russia.

出版信息

Crit Rev Biochem Mol Biol. 2012 Mar-Apr;47(2):97-193. doi: 10.3109/10409238.2011.620942. Epub 2012 Jan 20.

DOI:10.3109/10409238.2011.620942
PMID:22260147
Abstract

The sequence-specific transfer of methyl groups from donor S-adenosyl-L-methionine (AdoMet) to certain positions of DNA-adenine or -cytosine residues by DNA methyltransferases (MTases) is a major form of epigenetic modification. It is virtually ubiquitous, except for some notable exceptions. Site-specific methylation can be regarded as a means to increase DNA information capacity and is involved in a large spectrum of biological processes. The importance of these functions necessitates a deeper understanding of the enzymatic mechanism(s) of DNA methylation. DNA MTases fall into one of two general classes; viz. amino-MTases and [C5-cytosine]-MTases. Amino-MTases, common in prokaryotes and lower eukaryotes, catalyze methylation of the exocyclic amino group of adenine ([N6-adenine]-MTase) or cytosine ([N4-cytosine]-MTase). In contrast, [C5-cytosine]-MTases methylate the cyclic carbon-5 atom of cytosine. Characteristics of DNA MTases are highly variable, differing in their affinity to their substrates or reaction products, their kinetic parameters, or other characteristics (order of substrate binding, rate limiting step in the overall reaction). It is not possible to present a unifying account of the published kinetic analyses of DNA methylation because different authors have used different substrate DNAs and/or reaction conditions. Nevertheless, it would be useful to describe those kinetic data and the mechanistic models that have been derived from them. Thus, this review considers in turn studies carried out with the most consistently and extensively investigated [N6-adenine]-, [N4-cytosine]- and [C5-cytosine]-DNA MTases.

摘要

DNA 甲基转移酶(MTases)将供体 S-腺苷-L-甲硫氨酸(AdoMet)中的甲基基团特异性转移到 DNA-腺嘌呤或-胞嘧啶残基的某些位置是表观遗传修饰的主要形式。这种修饰几乎无处不在,除了一些显著的例外。特异性甲基化可以被视为增加 DNA 信息容量的一种手段,并且涉及到广泛的生物学过程。这些功能的重要性需要我们更深入地了解 DNA 甲基化的酶促机制。DNA MTases分为两类:氨基-MTases 和 [C5-胞嘧啶]-MTases。氨基-MTases 在原核生物和低等真核生物中很常见,催化腺嘌呤([N6-腺嘌呤]-MTase)或胞嘧啶([N4-胞嘧啶]-MTase)的外环氨基甲基化。相比之下,[C5-胞嘧啶]-MTases 甲基化胞嘧啶的环碳-5 原子。DNA MTases 的特征高度可变,其对底物或反应产物的亲和力、动力学参数或其他特性(底物结合顺序、总反应的限速步骤)不同。由于不同的作者使用了不同的底物 DNA 和/或反应条件,因此不可能对 DNA 甲基化的已发表动力学分析提供统一的解释。然而,描述这些动力学数据及其衍生的机制模型将是有用的。因此,本综述依次考虑了用最一致和广泛研究的 [N6-腺嘌呤]-、[N4-胞嘧啶]-和 [C5-胞嘧啶]-DNA MTases 进行的研究。

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