triCLEM: Combining high-precision, room temperature CLEM with cryo-fluorescence microscopy to identify very rare events
- PMID: 28528638
- DOI: 10.1016/bs.mcb.2017.03.009
triCLEM: Combining high-precision, room temperature CLEM with cryo-fluorescence microscopy to identify very rare events
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.
Keywords: CLEM; Cryo-fluorescence microscopy; Electron tomography; Fiducials; Fluorescent proteins; High-pressure freezing; Sapphire disks; triCLEM.
Copyright © 2017 Elsevier Inc. All rights reserved.
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