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Topographic contrast of ultrathin cryo-sections for correlative super-resolution light and electron microscopy

机译:超薄冷冻切片的地形对比用于相关的超分辨率光学和电子显微镜

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摘要

Fluorescence microscopy reveals molecular expression at nanometer resolution but lacks ultrastructural context information. This deficit often hinders a clear interpretation of results. Electron microscopy provides this contextual subcellular detail, but protein identification can often be problematic. Correlative light and electron microscopy produces complimentary information that expands our knowledge of protein expression in cells and tissue. Inherent methodological difficulties are however encountered when combining these two very different microscopy technologies. We present a quick, simple and reproducible method for protein localization by conventional and super-resolution light microscopy combined with platinum shadowing and scanning electron microscopy to obtain topographic contrast from the surface of ultrathin cryo-sections. We demonstrate protein distribution at nuclear pores and at mitochondrial and plasma membranes in the extended topographical landscape of tissue.
机译:荧光显微镜揭示了纳米级的分子表达,但缺乏超微结构背景信息。这种缺陷常常妨碍对结果的清晰解释。电子显微镜提供了这种背景下的亚细胞细节,但是蛋白质鉴定常常是有问题的。相关的光镜和电子显微镜可产生互补信息,从而扩展了我们在细胞和组织中蛋白质表达的知识。但是,当将这两种截然不同的显微镜技术结合在一起时会遇到固有的方法上的困难。我们提供了一种快速,简单和可重现的蛋白质定位方法,该方法通过常规和超高分辨率光学显微镜结合铂金阴影和扫描电子显微镜从超薄冷冻切片的表面获得地形对比度。我们展示了在组织的扩展地形景观中核孔以及线粒体和质膜上的蛋白质分布。

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