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p300组蛋白乙酰转移酶结构域自身乙酰化的动力学和质谱分析

Kinetic and mass spectrometric analysis of p300 histone acetyltransferase domain autoacetylation.

作者信息

Karanam Balasubramanyam, Jiang Lihua, Wang Ling, Kelleher Neil L, Cole Philip A

机构信息

Department of Pharmacology and Molecular Sciences, Johns Hopkins University School of Medicine, Baltimore, MD 21205, USA.

出版信息

J Biol Chem. 2006 Dec 29;281(52):40292-301. doi: 10.1074/jbc.M608813200. Epub 2006 Oct 25.

DOI:10.1074/jbc.M608813200
PMID:17065153
Abstract

Acetylation of proteins by p300 histone acetyltransferase plays a critical role in the regulation of gene expression. The prior discovery of an autoacetylated regulatory loop in the p300 histone acetyltransferase (HAT) domain prompted us to further explore the mechanisms of p300 autoacetylation. Here we have described a kinetic and mass spectrometric analysis of p300 HAT autoacetylation. The rate of p300 HAT autoacetylation was approximately fourth order with respect to p300 HAT domain concentration and thus appeared to be a highly cooperative process. By showing that a catalytically defective p300 HAT domain could be efficiently acetylated by active p300 HAT, we deduced that autoacetylation occurs primarily by an intermolecular mechanism. This was further confirmed using a semisynthetic biotinylated p300 HAT domain that could be physically separated from the catalytically defective p300 HAT by avidin affinity chromatography. Autoacetylation catalyzed by p300 HAT was approximately 1000-fold more efficient than PCAF (p300/CREB-binding protein-associated factor)-mediated acetylation of catalytically defective p300 HAT. Using a novel tandem mass spectrometric approach, it was found to be possible to observe up to 17 autoacetylation events within the intact p300 regulatory loop. Kinetic analysis of the site specificity of p300 autoacetylation reveals a class of rapid events followed by a slower set of modifications. Several of these rapid autoacetylation sites correlate with an acetyltransferase-activating function based on prior mutagenesis analysis.

摘要

p300组蛋白乙酰转移酶对蛋白质的乙酰化作用在基因表达调控中起着关键作用。此前在p300组蛋白乙酰转移酶(HAT)结构域中发现的自乙酰化调节环促使我们进一步探索p300自乙酰化的机制。在此,我们描述了对p300 HAT自乙酰化的动力学和质谱分析。p300 HAT自乙酰化速率相对于p300 HAT结构域浓度约为四级反应,因此似乎是一个高度协同的过程。通过表明催化缺陷的p300 HAT结构域可被活性p300 HAT有效乙酰化,我们推断自乙酰化主要通过分子间机制发生。使用可通过抗生物素蛋白亲和色谱与催化缺陷的p300 HAT物理分离的半合成生物素化p300 HAT结构域进一步证实了这一点。p300 HAT催化的自乙酰化比PCAF(p300/CREB结合蛋白相关因子)介导的催化缺陷p300 HAT的乙酰化效率高约1000倍。使用一种新型串联质谱方法,发现在完整的p300调节环内最多可观察到17个自乙酰化事件。对p300自乙酰化位点特异性的动力学分析揭示了一类快速事件,随后是一组较慢的修饰。基于先前的诱变分析,这些快速自乙酰化位点中的几个与乙酰转移酶激活功能相关。

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