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Published October 28, 2022 | Published
Journal Article Open

A cryogenic, coincident fluorescence, electron, and ion beam microscope

Boltje, Daan B. ORCID icon
Hoogenboom, Jacob P. ORCID icon
Jakobi, Arjen J. ORCID icon
Jensen, Grant J. ORCID icon
Jonker, Caspar T. H.
Kaag, Max J.
Koster, Abraham J. ORCID icon
Last, Mart G. F. ORCID icon
de Agrela Pinto, Cecilia
Plitzko, Jürgen M. ORCID icon
Raunser, Stefan ORCID icon
Tacke, Sebastian ORCID icon
Wang, Zhexin ORCID icon
van der Wee, Ernest B. ORCID icon
Wepf, Roger ORCID icon
den Hoedt, Sander

Abstract

Cryogenic electron tomography (cryo-ET) combined with subtomogram averaging, allows in situ visualization and structure determination of macromolecular complexes at subnanometre resolution. Cryogenic focused ion beam (cryo-FIB) micromachining is used to prepare a thin lamella-shaped sample out of a frozen-hydrated cell for cryo-ET imaging, but standard cryo-FIB fabrication is blind to the precise location of the structure or proteins of interest. Fluorescence-guided focused ion beam (FIB) milling at target locations requires multiple sample transfers prone to contamination, and relocation and registration accuracy is often insufficient for 3D targeting. Here, we present in situ fluorescence microscopy-guided FIB fabrication of a frozen-hydrated lamella to address this problem: we built a coincident three-beam cryogenic correlative microscope by retrofitting a compact cryogenic microcooler, custom positioning stage, and an inverted widefield fluorescence microscope (FM) on an existing FIB scanning electron microscope. We show FM controlled targeting at every milling step in the lamella fabrication process, validated with transmission electron microscope tomogram reconstructions of the target regions. The ability to check the lamella during and after the milling process results in a higher success rate in the fabrication process and will increase the throughput of fabrication for lamellae suitable for high-resolution imaging.

Additional Information

© 2022, Boltje et al. This article is distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use and redistribution provided that the original author and source are credited. Drosophila flight muscle myofibrils were kindly provided by EH Chan and F Schnorrer (Institut de Biologie du Développement de Marseille), and zebrafish myofibrils by Y Hinits and M Gautel (King's College London). We express our gratitude to Fulvio Reggiori (University of Groningen, Netherlands) for providing the HeLa cells and are thankful to Mingjun Xu for help during sample preparation. We thank Andries Effting (Delmic BV) for helpful discussions, and we would like to thank Ryan Lane (TU Delft) for his contribution in various Python developments. The majority of the 3D CAD design was done by Thomas van der Heijden (Delmic BV), for which we are grateful. This work was financially supported by NWO-TTW project no. 17152 to JPH, NIH grant RO1 AI127401 to GJJ, European SME2 grant no. 879673 to Delmic BV, Eurostars grant no. E13008 to SH & SR, and ERC grant ERC-StG-852880 to AJJ. The funders had no role in study design, data collection, and interpretation, or the decision to submit the work for publication.

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Identifiers Related works Funding Dates Caltech Custom Metadata
Created:
August 22, 2023
Modified:
December 22, 2023