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果蝇的转录衔接子ADA3对于组蛋白修饰、位置效应斑驳及转录是必需的。

Transcriptional adaptor ADA3 of Drosophila melanogaster is required for histone modification, position effect variegation, and transcription.

作者信息

Grau Benjamin, Popescu Cristina, Torroja Laura, Ortuño-Sahagún Daniel, Boros Imre, Ferrús Alberto

机构信息

Department of Cellular, Molecular, and Developmental Neurobiology, Cajal Institute, CSIC, Ave. Dr. Arce 37, 28002 Madrid, Spain.

出版信息

Mol Cell Biol. 2008 Jan;28(1):376-85. doi: 10.1128/MCB.01307-07. Epub 2007 Oct 29.

Abstract

The Drosophila melanogaster gene diskette (also known as dik or dAda3) encodes a protein 29% identical to human ADA3, a subunit of GCN5-containing histone acetyltransferase (HAT) complexes. The fly dADA3 is a major contributor to oogenesis, and it is also required for somatic cell viability. dADA3 localizes to chromosomes, and it is significantly reduced in dGcn5 and dAda2a, but not in dAda2b, mutant backgrounds. In dAda3 mutants, acetylation at histone H3 K9 and K14, but not K18, and at histone H4 K12, but not K5, K8, and K16, is significantly reduced. Also, phosphorylation at H3 S10 is reduced in dAda3 and dGcn5 mutants. Variegation for white (w(m4)) and scute (Hw(v)) genes, caused by rearrangements of X chromosome heterochromatin, is modified in a dAda3(+) gene-dosage-dependent manner. The effect is not observed with rearrangements involving Y heterochromatin (bw(D)), euchromatin (Scutoid), or transvection effects on chromosomal pairing (white and zeste interaction). Activity of scute gene enhancers, targets for Iroquoi transcription factors, is abolished in dAda3 mutants. Also, Iroquoi-associated phenotypes are sensitive to dAda3(+) gene dosage. We conclude that dADA3 plays a role in HAT complexes which acetylate H3 and H4 at specific residues. In turn, this acetylation results in chromatin structure effects of certain rearrangements and transcription of specific genes.

摘要

果蝇基因磁盘(也称为dik或dAda3)编码一种与人类ADA3有29%同源性的蛋白质,人类ADA3是含GCN5的组蛋白乙酰转移酶(HAT)复合物的一个亚基。果蝇dADA3是卵子发生的主要贡献者,也是体细胞存活所必需的。dADA3定位于染色体,在dGcn5和dAda2a突变背景中显著减少,但在dAda2b突变背景中没有减少。在dAda3突变体中,组蛋白H3 K9和K14(而非K18)以及组蛋白H4 K12(而非K5、K8和K16)的乙酰化显著减少。此外,dAda3和dGcn5突变体中H3 S10的磷酸化减少。由X染色体异染色质重排引起的白色(w(m4))和盾片(Hw(v))基因的斑驳现象,以dAda3(+)基因剂量依赖的方式被修饰。涉及Y异染色质(bw(D))、常染色质(Scutoid)或对染色体配对的转位效应(白色和zeste相互作用)的重排未观察到这种效应。dAda3突变体中,Iroquoi转录因子的靶标——盾片基因增强子的活性被消除。此外,与Iroquoi相关的表型对dAda3(+)基因剂量敏感。我们得出结论,dADA3在特定残基处使H3和H4乙酰化的HAT复合物中发挥作用。反过来,这种乙酰化导致某些重排的染色质结构效应和特定基因的转录。

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