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triCLEM:将高精度室温细胞光镜电镜关联技术与低温荧光显微镜相结合以识别极其罕见的事件。

triCLEM: Combining high-precision, room temperature CLEM with cryo-fluorescence microscopy to identify very rare events.

作者信息

Ader Nicholas R, Kukulski Wanda

机构信息

MRC Laboratory of Molecular Biology, Cambridge, United Kingdom; National Institutes of Health, Bethesda, MD, United States.

MRC Laboratory of Molecular Biology, Cambridge, United Kingdom.

出版信息

Methods Cell Biol. 2017;140:303-320. doi: 10.1016/bs.mcb.2017.03.009. Epub 2017 Apr 18.

DOI:10.1016/bs.mcb.2017.03.009
PMID:28528638
Abstract

Fiducial-based correlation of fluorescence and electron microscopy data from high-pressure frozen and resin-embedded samples allows for high-precision localization of fluorescent signals to subcellular ultrastructure. Here we introduce the triCLEM procedure to facilitate the identification of very rare events for high-precision correlation. We present a detailed protocol to screen high-pressure frozen cell monolayers on sapphire disks for very rare signals by cryo-fluorescence microscopy, relocate the cells of interest after freeze substitution and Lowicryl embedding, and perform fiducial-based correlation of the identified fluorescent signals to high-magnification electron tomograms. We show the applicability of the protocol to localize and image damaged mitochondria marked by the presence of Parkin, a protein involved in initiating mitophagy. We discuss how this extension to previously published fiducial-based correlation procedures has potential to both allow identifying very rare events and assess the quality of preservation in high-pressure frozen samples.

摘要

基于标记点的高压冷冻和树脂包埋样本荧光与电子显微镜数据的相关性分析,可实现荧光信号在亚细胞超微结构中的高精度定位。在此,我们介绍了triCLEM程序,以促进对非常罕见事件的识别,实现高精度相关性分析。我们提供了一个详细方案,用于通过低温荧光显微镜筛选蓝宝石盘上高压冷冻的细胞单层中的非常罕见信号,在冷冻置换和Lowicryl包埋后重新定位感兴趣的细胞,并将识别出的荧光信号与高倍电子断层扫描进行基于标记点的相关性分析。我们展示了该方案在定位和成像由参与启动线粒体自噬的蛋白质Parkin标记的受损线粒体方面的适用性。我们讨论了这种对先前发表的基于标记点的相关性程序的扩展如何既有潜力识别非常罕见的事件,又能评估高压冷冻样本的保存质量。

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