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SIRT1 包含增强去乙酰化酶活性的 N-端和 C-端区域。

SIRT1 contains N- and C-terminal regions that potentiate deacetylase activity.

机构信息

Wistar Institute, University of Pennsylvania, Philadelphia, Pennsylvania 19104, USA.

出版信息

J Biol Chem. 2012 Jan 20;287(4):2468-76. doi: 10.1074/jbc.M111.285031. Epub 2011 Dec 7.

Abstract

SIRT1 is one of seven mammalian sirtuin (silent information regulator 2-related) proteins that harbor NAD(+)-dependent protein deacetylase activity and is implicated in multiple metabolic and age-associated pathways and disorders. The sirtuin proteins contain a central region of high sequence conservation that is required for catalytic activity, but more variable N- and C-terminal regions have been proposed to mediate protein specific activities. Here we show that the conserved catalytic core domain of SIRT1 has very low catalytic activity toward several known protein substrates, but that regions N- and C-terminal to the catalytic core potentiate catalytic efficiency by between 12- and 45-fold, with the N-terminal domain contributing predominantly to catalytic rate, relatively independent of the nature of the acetyl-lysine protein substrate, and the C-terminal domain contributing significantly to the K(m) for NAD(+). We show that the N- and C-terminal regions stimulate SIRT1 deacetylase activity intramolecularly and that the C-terminal region stably associates with the catalytic core domain to form a SIRT1 holoenzyme. We also demonstrate that the C-terminal region of SIRT1 can influence the inhibitory activity of some sirtuin inhibitors that are known to function through the catalytic core domain. Together, these studies highlight the unique properties of the SIRT1 member of the sirtuin proteins and have implications for the development of SIRT1-specific regulatory molecules.

摘要

SIRT1 是七类哺乳动物沉默信息调节因子 2 相关蛋白(sirtuin)之一,具有 NAD(+) 依赖的蛋白去乙酰化酶活性,与多种代谢和与年龄相关的途径和疾病有关。sirtuin 蛋白含有一个中央高度序列保守区域,该区域对于催化活性是必需的,但更可变的 N- 和 C- 末端区域被认为可以介导蛋白的特定活性。在这里,我们显示 SIRT1 的保守催化核心域对几种已知的蛋白底物的催化活性非常低,但催化核心域的 N- 和 C- 末端区域可使催化效率提高 12-45 倍,其中 N- 末端区域主要贡献于催化速率,相对独立于乙酰-赖氨酸蛋白底物的性质,而 C- 末端区域对 NAD(+) 的 K(m) 有显著贡献。我们表明,N- 和 C- 末端区域可在分子内刺激 SIRT1 的去乙酰化酶活性,并且 C- 末端区域可与催化核心域稳定结合形成 SIRT1 全酶。我们还证明 SIRT1 的 C- 末端区域可以影响一些已知通过催化核心域起作用的 sirtuin 抑制剂的抑制活性。总之,这些研究强调了 sirtuin 蛋白中 SIRT1 成员的独特性质,并对 SIRT1 特异性调节分子的开发具有影响。

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