DNMT1型
磷酸化
DNA甲基转移酶
生物
生物化学
分子生物学
HMG盒
蛋白激酶A
酪蛋白激酶2
DNA
化学
甲基转移酶
甲基化
丝裂原活化蛋白激酶激酶
DNA结合蛋白
基因
转录因子
作者
Yasunori Sugiyama,Naoya Hatano,Noriyuki Sueyoshi,Isao Suetake,Shoji Tajima,Eiji Kinoshita,Emiko Kinoshita‐Kikuta,Tohru Koike,Isamu Kameshita
摘要
Dnmt1 (DNA methyltansferase 1) is an enzyme that recognizes and methylates hemimethylated DNA during DNA replication to maintain methylation patterns. The N-terminal region of Dnmt1 is known to form an independent domain structure that interacts with various regulatory proteins and DNA. In the present study, we investigated protein kinases in the mouse brain that could bind and phosphorylate the N-terminal regulatory domain of Dnmt1. A protein fraction containing protein kinase activity for phosphorylation of Dnmt1(1–290) was prepared using Dnmt1(1–290)-affinity, DNA–cellulose and gel-filtration columns. When the proteins in this fraction were analysed by LC-MS/MS (liquid chromatography tandem MS), CK1δ/ε (casein kinase 1δ/ε) was the only protein kinase identified. Recombinant CK1δ/ε was found to bind to the N-terminal domain of Dnmt1 and significantly phosphorylated this domain, especially in the presence of DNA. Phosphorylation analyses using various truncation and point mutants of Dnmt1 revealed that the major priming site phosphorylated by CK1δ/ε was Ser146, and that subsequent phosphorylation at other sites may occur after phosphorylation of the priming site. When the DNA-binding activity of phosphorylated Dnmt1 was compared with that of the non-phosphorylated form, phosphorylation of Dnmt1 was found to decrease the affinity for DNA. These results suggest that CK1δ/ε binds to and phosphorylates the N-terminal domain of Dnmt1 and regulates Dnmt1 function by reducing the DNA-binding activity.
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