ERK2 stimulates MYC transcription by anchoring CDK9 to the MYC promoter in a kinase activity–independent manner

细胞周期蛋白依赖激酶9 转录因子 生物 锚固 抄写(语言学) 激酶 蛋白激酶A 癌症研究 化学 细胞周期蛋白依赖激酶2 细胞生物学 基因 心理学 遗传学 哲学 语言学 社会心理学
作者
Lorena Agudo‐Ibáñez,Marta Morante,Lucía García-Gutiérrez,Andrea Quintanilla,Javier Rodríguez,Alberto Múñoz,Javier León,Piero Crespo
出处
期刊:Science Signaling [American Association for the Advancement of Science]
卷期号:16 (794) 被引量:13
标识
DOI:10.1126/scisignal.adg4193
摘要

The transcription factor MYC regulates cell proliferation, transformation, and survival in response to growth factor signaling that is mediated in part by the kinase activity of ERK2. Because ERK2 can also bind to DNA to modify gene expression, we investigated whether it more directly regulates MYC transcription. We identified ERK2 binding sites in the MYC promoter and detected ERK2 at the promoter in various serum-stimulated cell types. Expression of nuclear-localized ERK2 constructs in serum-starved cells revealed that ERK2 in the nucleus—regardless of its kinase activity—increased MYC mRNA expression and MYC protein abundance. ERK2 bound to the promoter through its amino-terminal insert domain and to the cyclin-dependent kinase CDK9 (which activates RNA polymerase II) through its carboxyl-terminal conserved docking domain. Both interactions were essential for ERK2-induced MYC expression, and depleting ERK impaired CDK9 occupancy and RNA polymerase II progression at the MYC promoter. Artificially tethering CDK9 to the MYC promoter by fusing it to the ERK2 insert domain was sufficient to stimulate MYC expression in serum-starved cells. Our findings demonstrate a role for ERK2 at the MYC promoter acting as a kinase-independent anchor for the recruitment of CDK9 to promote MYC expression.
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