TC Jenkins Department of Biophysics, Johns Hopkins University, Baltimore, MD 21218-2685, USA.
Mol Cell. 2010 Sep 10;39(5):711-23. doi: 10.1016/j.molcel.2010.08.012.
Chromatin remodelers are ATP-driven machines that assemble, slide, and remove nucleosomes from DNA, but how the ATPase motors of remodelers are regulated is poorly understood. Here we show that the double chromodomain unit of the Chd1 remodeler blocks DNA binding and activation of the ATPase motor in the absence of nucleosome substrates. The Chd1 crystal structure reveals that an acidic helix joining the chromodomains can pack against a DNA-binding surface of the ATPase motor. Disruption of the chromodomain-ATPase interface prevents discrimination between nucleosomes and naked DNA and reduces the reliance on the histone H4 tail for nucleosome sliding. We propose that the chromodomains allow Chd1 to distinguish between nucleosomes and naked DNA by physically gating access to the ATPase motor, and we hypothesize that related ATPase motors may employ a similar strategy to discriminate among DNA-containing substrates.
染色质重塑因子是一种 ATP 驱动的机器,能够将核小体从 DNA 上组装、滑动和去除,但对于重塑因子的 ATP 酶马达如何被调控,我们知之甚少。在这里,我们表明 Chd1 重塑因子的双 chromodomain 单元在缺乏核小体底物的情况下会阻断 DNA 结合和 ATP 酶马达的激活。Chd1 晶体结构显示,连接 chromodomains 的酸性螺旋可以与 ATP 酶马达的 DNA 结合表面结合。破坏 chromodomain-ATPase 界面会阻止核小体和裸露 DNA 之间的区分,并减少对组蛋白 H4 尾巴的依赖,以实现核小体滑动。我们提出 chromodomains 通过物理阻断 ATP 酶马达的进入来区分核小体和裸露 DNA,并且我们假设相关的 ATP 酶马达可能采用类似的策略来区分含 DNA 的底物。