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Centromeres are maintained by fastening CENP-A to DNA and directing an arginine anchor-dependent nucleosome transition

机译:通过将CENP-A固定在DNA上并指导精氨酸锚依赖性核小体的转化来维持着丝粒

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摘要

Maintaining centromere identity relies upon the persistence of the epigenetic mark provided by the histone H3 variant, centromere protein A (CENP-A), but the molecular mechanisms that underlie its remarkable stability remain unclear. Here, we define the contributions of each of the three candidate CENP-A nucleosome-binding domains (two on CENP-C and one on CENP-N) to CENP-A stability using gene replacement and rapid protein degradation. Surprisingly, the most conserved domain, the CENP-C motif, is dispensable. Instead, the stability is conferred by the unfolded central domain of CENP-C and the folded N-terminal domain of CENP-N that becomes rigidified 1,000-fold upon crossbridging CENP-A and its adjacent nucleosomal DNA. Disrupting the ‘arginine anchor' on CENP-C for the nucleosomal acidic patch disrupts the CENP-A nucleosome structural transition and removes CENP-A nucleosomes from centromeres. CENP-A nucleosome retention at centromeres requires a core centromeric nucleosome complex where CENP-C clamps down a stable nucleosome conformation and CENP-N fastens CENP-A to the DNA.
机译:维持着丝粒身份取决于赖于组蛋白H3变体着丝粒蛋白A(CENP-A)提供的表观遗传标记的持久性,但其显着稳定性的分子机制仍不清楚。在这里,我们定义了三个候选CENP-A核小体结合结构域(两个位于CENP-C上,一个位于CENP-N上)对CENP-A稳定性的贡献,使用基因置换和快速蛋白质降解。令人惊讶的是,最保守的结构域CENP-C基序是可有可无的。相反,稳定性由CENP-C的未折叠中央结构域和CENP-N的折叠N末端结构域赋予,该结构在将CENP-A及其相邻的核小体DNA交叉杂交时变得坚固了1000倍。破坏CENP-C上核糖体酸性补丁的“精氨酸锚”会破坏C​​ENP-A核小体的结构转变,并从着丝粒中去除CENP-A核小体。 CENP-A核小体保留在着丝粒上需要核心着丝粒核小体复合体,其中CENP-C钳制稳定的核小体构象,CENP-N将CENP-A固定在DNA上。

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