Department of Pathology, Keck School of Medicine of USC, Los Angeles, CA 90033, USA.
Bioinformatics Service, Department of Health Sciences Libraries, Keck School of Medicine of USC, Los Angeles, CA 90033, USA.
Mol Cell. 2019 Jun 20;74(6):1138-1147.e6. doi: 10.1016/j.molcel.2019.03.018. Epub 2019 Apr 11.
Adenine N6 methylation in DNA (6mA) is widespread among bacteria and phage and is detected in mammalian genomes, where its function is largely unexplored. Here we show that 6mA deposition and removal are catalyzed by the Mettl4 methyltransferase and Alkbh4 dioxygenase, respectively, and that 6mA accumulation in genic elements corresponds with transcriptional silencing. Inactivation of murine Mettl4 depletes 6mA and causes sublethality and craniofacial dysmorphism in incross progeny. We identify distinct 6mA sensor domains of prokaryotic origin within the MPND deubiquitinase and ASXL1, a component of the Polycomb repressive deubiquitinase (PR-DUB) complex, both of which act to remove monoubiquitin from histone H2A (H2A-K119Ub), a repressive mark. Deposition of 6mA by Mettl4 triggers the proteolytic destruction of both sensor proteins, preserving genome-wide H2A-K119Ub levels. Expression of the bacterial 6mA methyltransferase Dam, in contrast, fails to destroy either sensor. These findings uncover a native, adversarial 6mA network architecture that preserves Polycomb silencing.
DNA 中的腺嘌呤 N6 甲基化(6mA)在细菌和噬菌体中广泛存在,并在哺乳动物基因组中被检测到,但其功能在很大程度上尚未被探索。在这里,我们表明 6mA 的沉积和去除分别由 Mettl4 甲基转移酶和 Alkbh4 双加氧酶催化,并且基因元件中的 6mA 积累与转录沉默相对应。鼠 Mettl4 的失活会耗尽 6mA,并导致近交后代的亚致死性和颅面畸形。我们在 MPND 去泛素酶和 ASXL1 中鉴定出具有原核起源的不同 6mA 传感器结构域,后者是多梳抑制去泛素酶(PR-DUB)复合物的一个组成部分,两者都可以从组蛋白 H2A(H2A-K119Ub)上去除单泛素,这是一种抑制标记。Mettl4 沉积的 6mA 触发了这两种传感器蛋白的蛋白水解破坏,从而维持全基因组 H2A-K119Ub 水平。相比之下,细菌 6mA 甲基转移酶 Dam 的表达既不能破坏这两种传感器。这些发现揭示了一种天然的、对抗性的 6mA 网络架构,它可以维持多梳抑制沉默。
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