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绘制E2A中的乙酰化位点图谱可确定激活域1中一个保守的赖氨酸残基,该残基可促进CBP/p300的募集和转录激活。

Mapping acetylation sites in E2A identifies a conserved lysine residue in activation domain 1 that promotes CBP/p300 recruitment and transcriptional activation.

作者信息

Hyndman Brandy D, Thompson Patrick, Denis Christopher M, Chitayat Seth, Bayly Richard, Smith Steven P, LeBrun David P

机构信息

Department of Pathology and Molecular Medicine, Queen's University, Kingston, Ontario, Canada.

出版信息

Biochim Biophys Acta. 2012 May;1819(5):375-81. doi: 10.1016/j.bbagrm.2011.11.013. Epub 2011 Dec 20.

DOI:10.1016/j.bbagrm.2011.11.013
PMID:22207202
Abstract

E-proteins are basic helix-loop-helix transcription factors that function in cell type specification. The gene E2A encodes two E-proteins, E12 and E47, which are required in B-lymphopoiesis. E2A proteins can interact directly with the transcriptional co-activators and lysine acetyltranferases (KATs) CBP, p300 and PCAF to induce target gene transcription. Prior investigations have shown that the E2A-encoded isoform E2-5 is acetylated by CBP, p300 or PCAF in vitro or in vivo. However, E2-5 lacks the important N-terminal activation domain AD1. Furthermore, the acetylated residues in E-proteins have not been mapped, and the functional consequences of acetylation are largely unknown. Here, we use mutagenesis to show that a lysine residue at position 34 within AD1 of E12/E47 is acetylated by CBP/p300 and PCAF. Lys34 lies adjacent to a conserved helical LXXLL motif that interacts directly with the KIX domain of CBP/p300. We show that acetylation at Lys34 increases the affinity of AD1 for the KIX domain and enhances AD1-driven transcriptional induction. Our results illustrate for the first time that AD1 can both recruit, and be acetylated by, KATs and that KAT recruitment may promote transcriptional induction in part through acetylation of AD1 itself.

摘要

E蛋白是在细胞类型特异性中发挥作用的碱性螺旋-环-螺旋转录因子。E2A基因编码两种E蛋白,即E12和E47,它们是B淋巴细胞生成所必需的。E2A蛋白可直接与转录共激活因子及赖氨酸乙酰转移酶(KATs)CBP、p300和PCAF相互作用,以诱导靶基因转录。先前的研究表明,E2A编码的异构体E2-5在体外或体内可被CBP、p300或PCAF乙酰化。然而,E2-5缺乏重要的N端激活域AD1。此外,E蛋白中的乙酰化残基尚未定位,乙酰化的功能后果也大多未知。在此,我们通过诱变表明,E12/E47的AD1内第34位的赖氨酸残基可被CBP/p300和PCAF乙酰化。赖氨酸34紧邻一个保守的螺旋LXXLL基序,该基序直接与CBP/p300的KIX结构域相互作用。我们表明,赖氨酸34处的乙酰化增加了AD1对KIX结构域的亲和力,并增强了AD1驱动的转录诱导。我们的结果首次表明,AD1既能招募KATs并被其乙酰化,而且KAT的招募可能部分通过AD1自身的乙酰化促进转录诱导。

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