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行动受限:活细胞中DNA甲基转移酶活性的直接可视化

Trapped in action: direct visualization of DNA methyltransferase activity in living cells.

作者信息

Schermelleh Lothar, Spada Fabio, Easwaran Hariharan P, Zolghadr Kourosh, Margot Jean B, Cardoso M Cristina, Leonhardt Heinrich

机构信息

Ludwig Maximilians University Munich, Department of Biology II, Planegg-Martinsried, Germany.

出版信息

Nat Methods. 2005 Oct;2(10):751-6. doi: 10.1038/nmeth794.

Abstract

DNA methyltransferases have a central role in the complex regulatory network of epigenetic modifications controlling gene expression in mammalian cells. To study the regulation of DNA methylation in living cells, we developed a trapping assay using transiently expressed fluorescent DNA methyltransferase 1 (Dnmt1) fusions and mechanism-based inhibitors 5-azacytidine (5-aza-C) or 5-aza-2'-deoxycytidine (5-aza-dC). These nucleotide analogs are incorporated into the newly synthesized DNA at nuclear replication sites and cause irreversible immobilization, that is, trapping of Dnmt1 fusions at these sites. We measured trapping by either fluorescence bleaching assays or photoactivation of photoactivatable green fluorescent protein fused to Dnmt1 (paGFP-Dnmt1) in mouse and human cells; mutations affecting the catalytic center of Dnmt1 prevented trapping. This trapping assay monitors kinetic properties and activity-dependent immobilization of DNA methyltransferases in their native environment, and makes it possible to directly compare mutations and inhibitors that affect regulation and catalytic activity of DNA methyltransferases in single living cells.

摘要

DNA甲基转移酶在控制哺乳动物细胞基因表达的表观遗传修饰复杂调控网络中起着核心作用。为了研究活细胞中DNA甲基化的调控,我们开发了一种捕获测定法,使用瞬时表达的荧光DNA甲基转移酶1(Dnmt1)融合蛋白和基于机制的抑制剂5-氮杂胞苷(5-aza-C)或5-氮杂-2'-脱氧胞苷(5-aza-dC)。这些核苷酸类似物在核复制位点掺入新合成的DNA中,并导致不可逆的固定,即Dnmt1融合蛋白在这些位点的捕获。我们通过荧光漂白测定法或在小鼠和人类细胞中对与Dnmt1融合的光激活绿色荧光蛋白(paGFP-Dnmt1)进行光激活来测量捕获;影响Dnmt1催化中心的突变可防止捕获。这种捕获测定法监测DNA甲基转移酶在其天然环境中的动力学特性和活性依赖性固定,并使得能够直接比较影响单个活细胞中DNA甲基转移酶调控和催化活性的突变和抑制剂。

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