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Extended Recognition of the Histone H3 Tail by Histone Demethylase KDM5A

机译:组蛋白去甲基化酶 KDM5A 对组蛋白 H3 尾部的扩展识别

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摘要

Human lysine demethylase KDM5A is a chromatin-modifying enzyme associated with transcriptional regulation, because of its ability to catalyze removal of methyl groups from methylated lysine 4 of histone H3 (H3K4me3). Amplification of KDM5A is observed in many cancers, including breast cancer, prostate cancer, hepatocellular carcinoma, lung cancer, and gastric cancer. In this study, we employed alanine scanning mutagenesis to investigate substrate recognition of KDM5A and identify the H3 tail residues necessary for KDM5A-catalyzed demethylation. Our data show that the H3Q5 residue is critical for substrate recognition by KDM5A. Our data also reveal that the protein-protein interactions between KDM5A and the histone H3 tail extend beyond the amino acids proximal to the substrate mark. Specifically, demethylation activity assays show that deletion or mutation of residues at positions 14-18 on the H3 tail results in an 8-fold increase in the K-M(app), compared to wild-type 18mer peptide, suggesting that this distal epitope is important in histone engagement. Finally, we demonstrate that post-translational modifications on this distal epitope can modulate KDM5A-dependent demethylation. Our findings provide insights into H3K4-specific recognition by KDM5A, as well as how chromatin context can regulate KDM5A activity and H3K4 methylation status.
机译:人赖氨酸去甲基化酶 KDM5A 是一种与转录调控相关的染色质修饰酶,因为它能够催化从组蛋白 H3 (H3K4me3) 的甲基化赖氨酸 4 中去除甲基。在许多癌症中观察到 KDM5A 的扩增,包括乳腺癌、前列腺癌、肝细胞癌、肺癌和胃癌。在这项研究中,我们采用丙氨酸扫描诱变来研究KDM5A的底物识别,并鉴定KDM5A催化的去甲基化所需的H3尾残基。我们的数据表明,H3Q5残基对KDM5A的底物识别至关重要。我们的数据还表明,KDM5A 和组蛋白 H3 尾部之间的蛋白质-蛋白质相互作用超出了底物标记近端的氨基酸。具体而言,去甲基化活性测定表明,与野生型 18mer 肽相比,H3 尾部 14-18 位残基的缺失或突变导致 K-M(app) 增加 8 倍,这表明该远端表位在组蛋白结合中很重要。最后,我们证明该远端表位的翻译后修饰可以调节KDM5A依赖性去甲基化。我们的研究结果为KDM5A对H3K4的特异性识别以及染色质环境如何调节KDM5A活性和H3K4甲基化状态提供了见解。

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