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CREB结合蛋白在功能重要位点使造血转录因子GATA-1发生乙酰化。

CREB-Binding protein acetylates hematopoietic transcription factor GATA-1 at functionally important sites.

作者信息

Hung H L, Lau J, Kim A Y, Weiss M J, Blobel G A

机构信息

Division of Hematology, Children's Hospital of Philadelphia, Philadelphia, Pennsylvania 19104, USA.

出版信息

Mol Cell Biol. 1999 May;19(5):3496-505. doi: 10.1128/MCB.19.5.3496.

Abstract

The transcription factor GATA-1 is a key regulator of erythroid-cell differentiation and survival. We have previously shown that the transcriptional cofactor CREB-binding protein (CBP) binds to the zinc finger domain of GATA-1, markedly stimulates the transcriptional activity of GATA-1, and is required for erythroid differentiation. Here we report that CBP, but not p/CAF, acetylates GATA-1 at two highly conserved lysine-rich motifs present at the C-terminal tails of both zinc fingers. Using [3H]acetate labelling experiments and anti-acetyl lysine immunoprecipitations, we show that GATA-1 is acetylated in vivo at the same sites acetylated by CBP in vitro. In addition, we show that CBP stimulates GATA-1 acetylation in vivo in an E1A-sensitive manner, thus establishing a correlation between acetylation and transcriptional activity of GATA-1. Acetylation in vitro did not alter the ability of GATA-1 to bind DNA, and mutations in either motif did not affect DNA binding of GATA-1 expressed in mammalian cells. Since certain functions of GATA-1 are revealed only in an erythroid environment, GATA-1 constructs were examined for their ability to trigger terminal differentiation when introduced into a GATA-1-deficient erythroid cell line. We found that mutations in either acetylation motif partially impaired the ability of GATA-1 to induce differentiation while mutations in both motifs abrogated it completely. Taken together, these data indicate that CBP is an important cofactor for GATA-1 and suggest a novel mechanism in which acetylation by CBP regulates GATA-1 activity in erythroid cells.

摘要

转录因子GATA-1是红系细胞分化和存活的关键调节因子。我们之前已经表明,转录辅因子CREB结合蛋白(CBP)与GATA-1的锌指结构域结合,显著刺激GATA-1的转录活性,并且是红系分化所必需的。在此我们报告,CBP而非p/CAF可在两个锌指结构域C末端富含赖氨酸的高度保守基序处使GATA-1发生乙酰化。通过[3H]乙酸盐标记实验和抗乙酰赖氨酸免疫沉淀,我们表明GATA-1在体内的乙酰化位点与CBP在体外使其乙酰化的位点相同。此外,我们表明CBP以E1A敏感的方式在体内刺激GATA-1的乙酰化,从而建立了GATA-1乙酰化与转录活性之间的相关性。体外乙酰化并未改变GATA-1结合DNA的能力,并且任一基序中的突变均不影响在哺乳动物细胞中表达的GATA-1与DNA的结合。由于GATA-1的某些功能仅在红系环境中才得以揭示,因此我们检测了GATA-1构建体在导入GATA-1缺陷型红系细胞系时触发终末分化的能力。我们发现,任一乙酰化基序中的突变均部分损害了GATA-1诱导分化的能力,而两个基序中的突变则完全消除了这种能力。综上所述,这些数据表明CBP是GATA-1的重要辅因子,并提示了一种新机制,即CBP介导的乙酰化在红系细胞中调节GATA-1的活性。

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