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Single Molecule Localization Microscopy of Mammalian Cell Nuclei on the Nanoscale

机译:哺乳动物细胞核在纳米尺度上的单分子定位显微镜。

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摘要

Nuclear texture analysis is a well-established method of cellular pathology. It is hampered, however, by the limits of conventional light microscopy (ca. 200 nm). These limits have been overcome by a variety of super-resolution approaches. An especially promising approach to chromatin texture analysis is single molecule localization microscopy (SMLM) as it provides the highest resolution using fluorescent based methods. At the present state of the art, using fixed whole cell samples and standard DNA dyes, a structural resolution of chromatin in the 50–100 nm range is obtained using SMLM. We highlight how the combination of localization microscopy with standard fluorophores opens the avenue to a plethora of studies including the spatial distribution of DNA and associated proteins in eukaryotic cell nuclei with the potential to elucidate the functional organization of chromatin. These views are based on our experience as well as on recently published research in this field.
机译:核纹理分析是一种公认​​的细胞病理学方法。但是,它受到常规光学显微镜(约200 nm)的限制。这些限制已通过各种超分辨率方法克服。染色质纹理分析的一种特别有前途的方法是单分子定位显微镜(SMLM),因为它可以使用基于荧光的方法提供最高的分辨率。在目前的技术水平下,使用固定的全细胞样品和标准DNA染料,使用SMLM可获得50-100 nm范围内染色质的结构分辨率。我们着重介绍定位显微镜与标准荧光团的结合如何为大量研究提供途径,包括真核细胞核中DNA和相关蛋白的空间分布,并有可能阐明染色质的功能组织。这些观点基于我们的经验以及该领域最近发表的研究。

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