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Single-molecule compaction of megabase-long chromatin molecules by multivalent cations

机译:多价阳离子对百万碱基长的染色质分子的单分子压实

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摘要

To gain insight into the conformational properties and compaction of megabase-long chromatin molecules, we reconstituted chromatin from T4 phage DNA (165 kb) and recombinant human histone octamers (HO). The unimolecular compaction, induced by divalent Mg2+ or tetravalent spermine4+ cations, studied by single-molecule fluorescence microscopy (FM) and dynamic light scattering (DLS) techniques, resulted in the formation of 250–400 nm chromatin condensates. The compaction on this scale of DNA size is comparable to that of chromatin topologically associated domains (TAD) in vivo. Variation of HO loading revealed a number of unique features related to the efficiency of chromatin compaction by multivalent cations, the mechanism of compaction, and the character of partly compact chromatin structures. The observations may be relevant for how DNA accessibility in chromatin is maintained. Compaction of saturated chromatin, in turn, is accompanied by an intra-chain segregation at the level of single chromatin molecules, suggesting an intriguing scenario of selective activation/deactivation of DNA as a result of chromatin fiber heterogeneity due to the nucleosome positioning. We suggest that this chromatin, reconstituted on megabase-long DNA because of its large size, is a useful model of eukaryotic chromatin.
机译:为了深入了解兆碱基长的染色质分子的构象特性和紧密性,我们从T4噬菌体DNA(165 kb)和重组人组蛋白八聚体(HO)重构了染色质。通过单分子荧光显微镜(FM)和动态光散射(DLS)技术研究了由二价Mg 2 + 或四价精胺 4 + 阳离子引起的单分子压实,导致形成250–400 nm的染色质冷凝物。这种大小的DNA压缩与体内染色质拓扑相关域(TAD)的压缩相当。 HO负载的变化揭示了许多独特的特征,这些特征与多价阳离子对染色质的压实效率,压紧机理以及部分致密的染色质结构的特征有关。这些观察结果可能与如何保持染色质中的DNA可及性有关。饱和染色质的压实又伴随着单个染色质分子水平的链内分离,这表明由于核小体定位,染色质纤维异质性导致DNA选择性激活/失活的有趣情况。我们建议,由于其大尺寸而在兆碱基长的DNA上重建的这种染色质是真核染色质的有用模型。

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