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Compaction Kinetics on Single DNAs: Purified Nucleosome Reconstitution Systems versus Crude Extract

机译:单一DNA的压缩动力学:纯化的核小体重建系统与粗提取物的比较

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摘要

Kinetics of compaction on single DNA molecules are studied by fluorescence videomicroscopy in the presence of 1), Xenopus egg extracts and 2), purified nucleosome reconstitution systems using a combination of histones with either the histone chaperone Nucleosome Assembly Protein (NAP-1) or negatively charged macromolecules such as polyglutamic acid and RNA. The comparison shows that the compaction rates can differ by a factor of up to 1000 for the same amount of histones, depending on the system used and on the presence of histone tails, which can be subjected to post-translational modifications. Reactions with purified reconstitution systems follow a slow and sequential mechanism, compatible with the deposition of one (H3-H4)2 tetramer followed by two (H2A-H2B) dimers. Addition of the histone chaperone NAP-1 increases both the rate of the reaction and the packing ratio of the final product. These stimulatory effects cannot be obtained with polyglutamic acid or RNA, suggesting that yNAP-1 impact on the reaction cannot simply be explained in terms of charge screening. Faster compaction kinetics and higher packing ratios are reproducibly reached with extracts, indicating a role of additional components present in this system. Data are discussed and models proposed to account for the kinetics obtained in our single-molecule assay.
机译:在1),爪蟾卵提取物和2),结合组蛋白与组蛋白伴侣蛋白核小体组装蛋白(NAP-1)或阴性组合使用的纯化核小体重建系统的存在下,通过荧光显微镜研究了单个DNA分子的紧缩动力学。带电的大分子,例如聚谷氨酸和RNA。比较表明,对于相同量的组蛋白,压实率的差异可能高达1000倍,这取决于所使用的系统和组蛋白尾部的存在,可以对它们进行翻译后修饰。与纯化的重建系统进行的反应遵循缓慢且顺序的机制,与一个(H3-H4)2四聚体随后是两个(H2A-H2B)二聚体的沉积相容。组蛋白伴侣NAP-1的加入增加了反应速率和最终产物的堆积率。用聚谷氨酸或RNA不能获得这些刺激作用,这表明不能简单地用电荷筛选来解释yNAP-1对反应的影响。提取物可重现更快的压实动力学和更高的填充率,表明该系统中存在其他组分的作用。讨论了数据并提出了模型,以解释我们单分子分析中获得的动力学。

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