Colmenares Serafin U, Swenson Joel M, Langley Sasha A, Kennedy Cameron, Costes Sylvain V, Karpen Gary H
Biological Systems and Engineering, Lawrence Berkeley National Laboratory, Berkeley, CA 94720, USA.
Biological Systems and Engineering, Lawrence Berkeley National Laboratory, Berkeley, CA 94720, USA; Department of Molecular and Cellular Biology, University of California, Berkeley, CA 94720, USA.
Dev Cell. 2017 Jul 24;42(2):156-169.e5. doi: 10.1016/j.devcel.2017.06.014.
Eukaryotic genomes are broadly divided between gene-rich euchromatin and the highly repetitive heterochromatin domain, which is enriched for proteins critical for genome stability and transcriptional silencing. This study shows that Drosophila KDM4A (dKDM4A), previously characterized as a euchromatic histone H3 K36 demethylase and transcriptional regulator, predominantly localizes to heterochromatin and regulates heterochromatin position-effect variegation (PEV), organization of repetitive DNAs, and DNA repair. We demonstrate that dKDM4A demethylase activity is dispensable for PEV. In contrast, dKDM4A enzymatic activity is required to relocate heterochromatic double-strand breaks outside the domain, as well as for organismal survival when DNA repair is compromised. Finally, DNA damage triggers dKDM4A-dependent changes in the levels of H3K56me3, suggesting that dKDM4A demethylates this heterochromatic mark to facilitate repair. We conclude that dKDM4A, in addition to its previously characterized role in euchromatin, utilizes both enzymatic and structural mechanisms to regulate heterochromatin organization and functions.
真核生物基因组大致分为富含基因的常染色质和高度重复的异染色质结构域,异染色质结构域富含对基因组稳定性和转录沉默至关重要的蛋白质。这项研究表明,果蝇KDM4A(dKDM4A),先前被表征为常染色质组蛋白H3 K36去甲基化酶和转录调节因子,主要定位于异染色质并调节异染色质位置效应斑驳(PEV)、重复DNA的组织和DNA修复。我们证明dKDM4A去甲基化酶活性对于PEV是可有可无的。相反,dKDM4A酶活性是将异染色质双链断裂重新定位到该结构域之外所必需的,并且在DNA修复受损时对于生物体存活也是必需的。最后,DNA损伤触发H3K56me3水平的dKDM4A依赖性变化,表明dKDM4A使这种异染色质标记去甲基化以促进修复。我们得出结论,dKDM4A除了其先前在常染色质中表征的作用外,还利用酶促和结构机制来调节异染色质组织和功能。