Correlative single molecule lattice light sheet imaging reveals the dynamic relationship between nucleosomes and the local chromatin environment

Timothy A. Daugird, Yu Shi, Katie L. Holland, Hosein Rostamian, Zhe Liu, Luke D. Lavis, Joseph Rodriguez, Brian D. Strahl, Wesley R. Legant
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Abstract

In the nucleus, biological processes are driven by proteins that diffuse through and bind to a meshwork of nucleic acid polymers. To better understand this interplay, we developed an imaging platform to simultaneously visualize single protein dynamics together with the local chromatin environment in live cells. Together with super-resolution imaging, new fluorescent probes, and biophysical modeling, we demonstrated that nucleosomes display differential diffusion and packing arrangements as chromatin density increases whereas the viscoelastic properties and accessibility of the interchromatin space remain constant. Perturbing nuclear functions impacted nucleosome diffusive properties in a manner that was dependent on local chromatin density and supportive of a model wherein transcription locally stabilizes nucleosomes while simultaneously allowing for the free exchange of nuclear proteins. Our results reveal that nuclear heterogeneity arises from both active and passive process and highlights the need to account for different organizational principals when modeling different chromatin environments.
相关的单分子点阵光片成像揭示了核小体与局部染色质环境之间的动态关系
在细胞核中,生物过程是由蛋白质驱动的,这些蛋白质通过核酸聚合物网络扩散并结合在一起。为了更好地理解这种相互作用,我们开发了一个成像平台,可以同时可视化活细胞中单个蛋白质动力学和局部染色质环境。结合超分辨率成像、新型荧光探针和生物物理模型,我们证明了核小体随着染色质密度的增加而表现出不同的扩散和堆积排列,而粘弹性和染色质间空间的可及性保持不变。干扰核功能以依赖于局部染色质密度的方式影响核小体的扩散特性,并支持转录在局部稳定核小体的同时允许核蛋白自由交换的模型。我们的研究结果表明,核异质性源于主动和被动过程,并强调在建模不同的染色质环境时需要考虑不同的组织原则。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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