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The Histone Fold Subunits of Drosophila CHRAC Facilitate Nucleosome Sliding through Dynamic DNA Interactions

机译:果蝇CHRAC的组蛋白折叠亚基通过动态DNA相互作用促进核小体滑动。

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The chromatin accessibility complex (CHRAC) is an abundant, evolutionarily conserved nucleosome remodeling machinery able to catalyze histone octamer sliding on DNA. CHRAC differs from the related ACF complex by the presence of two subunits with molecular masses of 14 and 16 kDa, whose structure and function were not known. We determined the structure of Drosophila melanogaster CHRAC14-CHRAC16 by X-ray crystallography at 2.4-? resolution and found that they dimerize via a variant histone fold in a typical handshake structure. In further analogy to histones, CHRAC14-16 contain unstructured N- and C-terminal tail domains that protrude from the handshake structure. A dimer of CHRAC14-16 can associate with the N terminus of ACF1, thereby completing CHRAC. Low-affinity interactions of CHRAC14-16 with DNA significantly improve the efficiency of nucleosome mobilization by limiting amounts of ACF. Deletion of the negatively charged C terminus of CHRAC16 enhances DNA binding 25-fold but leads to inhibition of nucleosome sliding, in striking analogy to the effect of the DNA chaperone HMGB1 on nucleosome sliding. The presence of a surface compatible with DNA interaction and the geometry of an H2A-H2B heterodimer may provide a transient acceptor site for DNA dislocated from the histone surface and therefore facilitate the nucleosome remodeling process.
机译:染色质可及性复合物(CHRAC)是一种丰富的,进化上保守的核小体重塑机制,能够催化在DNA上滑动的组蛋白八聚体。 CHRAC与相关的ACF复合物的区别在于存在两个分子量分别为14和16 kDa的亚基,其结构和功能未知。通过X-射线晶体学在2.4-℃确定了果蝇CHRAC14-CHRAC16的结构。分辨率,发现它们通过典型的握手结构中的组蛋白折叠变二聚。与组蛋白进一步相似,CHRAC14-16包含从握手结构突出的非结构化N和C末端尾结构域。 CHRAC14-16的二聚体可与ACF1的N末端缔合,从而完成CHRAC。 CHRAC14-16与DNA的低亲和力相互作用通过限制ACF的量显着提高了核小体动员的效率。 CHRAC16带负电荷的C末端的删除增强了25倍的DNA结合,但导致了核小体滑动的抑制,这与DNA伴侣HMGB1对核小体滑动的影响类似。与DNA相互作用和H2A-H2B异二聚体的几何形状相容的表面的存在可以为从组蛋白表面脱位的DNA提供瞬时受体位点,因此促进了核小体的重塑过程。

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