Dorighi Kristel M, Swigut Tomek, Henriques Telmo, Bhanu Natarajan V, Scruggs Benjamin S, Nady Nataliya, Still Christopher D, Garcia Benjamin A, Adelman Karen, Wysocka Joanna
Department of Chemical and Systems Biology, Stanford University School of Medicine, Stanford, CA 94305, USA.
Epigenetics and Stem Cell Biology Laboratory, National Institute of Environmental Health Sciences, Research Triangle Park, NC 27709, USA.
Mol Cell. 2017 May 18;66(4):568-576.e4. doi: 10.1016/j.molcel.2017.04.018. Epub 2017 May 5.
Monomethylation of histone H3 at lysine 4 (H3K4me1) and acetylation of histone H3 at lysine 27 (H3K27ac) are correlated with transcriptionally engaged enhancer elements, but the functional impact of these modifications on enhancer activity is not well understood. Here we used CRISPR/Cas9 genome editing to separate catalytic activity-dependent and independent functions of Mll3 (Kmt2c) and Mll4 (Kmt2d, Mll2), the major enhancer H3K4 monomethyltransferases. Loss of H3K4me1 from enhancers in Mll3/4 catalytically deficient cells causes partial reduction of H3K27ac, but has surprisingly minor effects on transcription from either enhancers or promoters. In contrast, loss of Mll3/4 proteins leads to strong depletion of enhancer Pol II occupancy and eRNA synthesis, concomitant with downregulation of target genes. Interestingly, downregulated genes exhibit reduced polymerase levels in gene bodies, but not at promoters, suggestive of pause-release defects. Altogether, our results suggest that enhancer H3K4me1 provides only a minor contribution to the long-range coactivator function of Mll3/4.
组蛋白H3赖氨酸4位点的单甲基化(H3K4me1)和组蛋白H3赖氨酸27位点的乙酰化(H3K27ac)与转录活跃的增强子元件相关,但这些修饰对增强子活性的功能影响尚未得到充分理解。在这里,我们使用CRISPR/Cas9基因组编辑来区分主要的增强子H3K4单甲基转移酶Mll3(Kmt2c)和Mll4(Kmt2d,Mll2)的催化活性依赖性和非依赖性功能。在Mll3/4催化缺陷细胞中,增强子上H3K4me1的缺失会导致H3K27ac部分减少,但对增强子或启动子的转录影响出人意料地小。相比之下,Mll3/4蛋白的缺失会导致增强子Pol II占据率和eRNA合成的强烈减少,同时伴随着靶基因的下调。有趣的是,下调的基因在基因体内的聚合酶水平降低,但在启动子处没有,这表明存在暂停释放缺陷。总之,我们的结果表明,增强子H3K4me1对Mll
