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MAML1 依赖性 Notch 反应基因表现出转录激活对辅助因子的不同需求。

MAML1-Dependent Notch-Responsive Genes Exhibit Differing Cofactor Requirements for Transcriptional Activation.

机构信息

Department of Biological Chemistry and Molecular Pharmacology, Blavatnik Institute, Harvard Medical School, Boston, Massachusetts, USA.

Department of Pathology, Brigham and Women's Hospital, Boston, Massachusetts, USA.

出版信息

Mol Cell Biol. 2020 May 14;40(11). doi: 10.1128/MCB.00014-20.

DOI:10.1128/MCB.00014-20
PMID:32179552
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7225564/
Abstract

Mastermind proteins are required for transcription of Notch target genes, yet the molecular basis for mastermind function remains incompletely understood. Previous work has shown that Notch can induce transcriptional responses by binding to promoters but more often by binding to enhancers, with and as representative mammalian examples of promoter and enhancer responsiveness, respectively. Here, we show that mastermind dependence of the Notch response at these loci is differentially encoded in Jurkat T-cell acute lymphoblastic leukemia (T-ALL) cells. Knockout of Mastermind-like 1 (MAML1) eliminates Notch-responsive activation of both these genes, and reduced target gene expression is accompanied by a decrease in H3K27 acetylation, consistent with the importance of MAML1 for p300 activity. Add-back of MAML1 variants in knockout cells identifies residues 151 to 350 of MAML1 as essential for expression of either Notch-responsive gene. Fusion of the Notch-binding region of MAML1 to the histone acetyltransferase (HAT) domain of p300 rescues expression of but not , suggesting that an additional activity of MAML1 is needed for gene induction at a distance. Together, these studies establish the functional importance of the MAML1 region from residues 151 to 350 for Notch-dependent transcriptional induction and reveal differential requirements for MAML1-dependent recruitment activities at different Notch-responsive loci, highlighting the molecular complexity of Notch-stimulated transcription.

摘要

调控蛋白对于 Notch 靶基因的转录是必需的,但调控蛋白的功能的分子基础仍不完全清楚。以前的工作表明,Notch 可以通过结合启动子诱导转录反应,但更常见的是通过结合增强子诱导转录反应, 和 分别作为启动子和增强子反应性的代表性哺乳动物例子。在这里,我们表明,Notch 在这些基因座的反应中对调控蛋白的依赖性在 Jurkat T 细胞急性淋巴细胞白血病 (T-ALL) 细胞中存在差异编码。敲除调控蛋白样 1 (MAML1) 消除了这两个基因的 Notch 反应性激活,靶基因表达的减少伴随着 H3K27 乙酰化的减少,这与 MAML1 对 p300 活性的重要性一致。在敲除细胞中添加 MAML1 变体,确定 MAML1 的 151 到 350 位残基对于 Notch 反应基因的表达是必需的。MAML1 的 Notch 结合区与 p300 的组蛋白乙酰转移酶 (HAT) 结构域融合挽救了 基因的表达,但不能挽救 基因的表达,这表明在远距离诱导基因表达需要调控蛋白的其他活性。这些研究共同确立了 MAML1 残基从 151 到 350 位对于 Notch 依赖性转录诱导的功能重要性,并揭示了不同的 Notch 反应基因座对 MAML1 依赖性募集活性的不同需求,突出了 Notch 刺激转录的分子复杂性。

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