代谢衍生的赖氨酸酰化及其邻近修饰调节BET溴结构域与组蛋白H4的结合。
Metabolically Derived Lysine Acylations and Neighboring Modifications Tune the Binding of the BET Bromodomains to Histone H4.
作者信息
Olp Michael D, Zhu Nan, Smith Brian C
机构信息
Department of Biochemistry, Medical College of Wisconsin , Milwaukee, Wisconsin 53226, United States.
Stem Cell Biology and Hematopoiesis Program, Blood Research Institute, Blood Center of Wisconsin , Milwaukee, Wisconsin 53226, United States.
出版信息
Biochemistry. 2017 Oct 17;56(41):5485-5495. doi: 10.1021/acs.biochem.7b00595. Epub 2017 Oct 5.
Recent proteomic studies discovered histone lysines are modified by acylations beyond acetylation. These acylations derive from acyl-CoA metabolites, potentially linking metabolism to transcription. Bromodomains bind lysine acylation on histones and other nuclear proteins to influence transcription. However, the extent bromodomains bind non-acetyl acylations is largely unknown. Also unclear are the effects of neighboring post-translational modifications, especially within heavily modified histone tails. Using peptide arrays, binding assays, sucrose gradients, and computational methods, we quantified 10 distinct acylations for binding to the bromodomain and extraterminal domain (BET) family. Four of these acylations (hydroxyisobutyrylation, malonylation, glutarylation, and homocitrullination) had never been tested for bromodomain binding. We found N-terminal BET bromodomains bound acetylated and propionylated peptides, consistent with previous studies. Interestingly, all other acylations inhibited binding of the BET bromodomains to peptides and nucleosomes. To understand how context tunes bromodomain binding, effects of neighboring methylation, phosphorylation, and acylation within histone H4 tails were determined. Serine 1 phosphorylation inhibited binding of the BRD4 N-terminal bromodomain to polyacetylated H4 tails by >5-fold, whereas methylation had no effect. Furthermore, binding of BRDT and BRD4 N-terminal bromodomains to H4K5acetyl was enhanced 1.4-9.5-fold by any neighboring acylation of lysine 8, indicating a secondary H4K8acyl binding site that is more permissive of non-acetyl acylations than previously appreciated. In contrast, C-terminal BET bromodomains exhibited 9.9-13.5-fold weaker binding for polyacylated than for monoacylated H4 tails, indicating the C-terminal bromodomains do not cooperatively bind multiple acylations. These results suggest acyl-CoA levels tune or block recruitment of the BET bromodomains to histones, linking metabolism to bromodomain-mediated transcription.
近期的蛋白质组学研究发现,组蛋白赖氨酸的修饰除了乙酰化外,还有其他酰化修饰。这些酰化修饰来源于酰基辅酶A代谢产物,可能将代谢与转录联系起来。溴结构域可结合组蛋白和其他核蛋白上的赖氨酸酰化修饰,从而影响转录。然而,溴结构域与非乙酰化酰化修饰的结合程度在很大程度上尚不清楚。相邻的翻译后修饰的影响也不明确,尤其是在高度修饰的组蛋白尾部。我们使用肽阵列、结合试验、蔗糖梯度和计算方法,对与溴结构域和额外末端结构域(BET)家族结合的10种不同酰化修饰进行了定量。其中四种酰化修饰(羟基异丁酰化、丙二酰化、戊二酰化和高瓜氨酸化)从未进行过与溴结构域结合的测试。我们发现,BET溴结构域的N端可结合乙酰化和丙酰化肽段,这与之前的研究一致。有趣的是,所有其他酰化修饰均抑制BET溴结构域与肽段和核小体的结合。为了了解环境如何调节溴结构域的结合,我们确定了组蛋白H4尾部相邻的甲基化、磷酸化和酰化修饰的影响。丝氨酸1磷酸化使BRD4 N端溴结构域与多乙酰化H4尾部的结合抑制超过5倍,而甲基化则没有影响。此外,赖氨酸8的任何相邻酰化修饰使BRDT和BRD4 N端溴结构域与H4K5乙酰化的结合增强1.4至9.5倍,表明存在一个二级H4K8酰化结合位点,该位点对非乙酰化酰化修饰的耐受性比之前认为的更高。相比之下,BET溴结构域的C端对多酰化H4尾部的结合比对单酰化H4尾部的结合弱9.9至13.5倍,表明C端溴结构域不会协同结合多个酰化修饰。这些结果表明,酰基辅酶A水平可调节或阻止BET溴结构域募集到组蛋白上,从而将代谢与溴结构域介导的转录联系起来。
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