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Optimized sample preparation for single-molecule localization-based superresolution microscopy in yeast

机译:用于酵母中基于单分子定位的超分辨率显微镜的优化样品制备

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摘要

Single-molecule localization-based superresolution microscopy methods allow the resolution of cellular structures in the range of tens of nanometers. However, these techniques are of limited use in current yeast labeling protocols, owing to problems with structural preservation. Here we describe an optimized sample preparation protocol that enables single-molecule localization microscopy at high resolution combined with improved structural preservation in Saccharomyces cerevisiae. The protocol uses small binders called nanobodies and an enzymatic labeling strategy to deliver organic dyes to the target protein. These small binders readily penetrate through the yeast cell wall and thus eliminate the requirement for its prior degradation, and they allow structural preservation. In addition, the small size of the binders reduces the distance of the dye to the target protein, and thus it reduces the localization error. The preparation of S. cerevisiae cells for superresolution imaging takes 2-4 h to perform. Researchers should have skills in yeast molecular biology, immunolabeling techniques and access to a microscope equipped for single-molecule imaging.
机译:基于单分子定位的超分辨率显微镜方法可使细胞结构的分辨率在数十纳米的范围内。然而,由于结构保存的问题,这些技术在当前的酵母标记方案中用途有限。在这里,我们描述了一种优化的样品制备方案,该方案可实现高分辨率的单分子定位显微镜检查以及酿酒酵母中改善的结构保存。该协议使用称为纳米抗体的小结合剂和酶标记策略将有机染料递送至目标蛋白。这些小的粘合剂很容易穿透酵母细胞壁,因此消除了对其先前降解的要求,并且它们可以保留结构。另外,粘合剂的小尺寸减小了染料到靶蛋白的距离,因此减小了定位误差。用于超分辨率成像的酿酒酵母细胞的制备需要2-4小时才能完成。研究人员应具有酵母分子生物学,免疫标记技术的技能,并应具备配备用于单分子成像的显微镜的能力。

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