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Published November 20, 2020 | Published
Journal Article Open

Serial Cryomicrotomy of Saccharomyces cerevisiae for Serial Electron Cryotomography

Abstract

Electron cryotomography (cryo-ET) is an increasingly popular technique to study cellular structures and macromolecules in situ. Due to poor penetration of electrons through thick biological samples, the vitreously frozen samples for cryo-ET need to be thin. For frozen-hydrated cells, such samples can be produced either by cryomicrotomy or cryo-FIB-milling. As a result, a tomogram of such a sample contains information of a small fraction of the entire cell volume, making it challenging to image rare structures in the cell or to determine the distribution of scattered structures. Here, we describe the tools and workflow that we designed to facilitate serial cryomicrotomy, which makes possible the exploration of a larger volume of individual cells at molecular resolution. We successfully used serial cryomicrotomy to locate and image the Dam1/DASH complex located at microtubule plus ends inside mitotic Saccharomyces cerevisiae cells.

Additional Information

© 2020 The Authors; exclusive licensee Bio-protocol LLC. We thank Chen Chen for the initial cryomicrotomy set up in the lab, Gemma An for suggesting the use of parallel-bar EM grids, and Olivia Ma for her help in preparation of figures and feedback on the manuscript. We also thank members of the Gan lab for feedback and tips on cryomicrotomy. We thank Satoru Chomabayashi (Narishige) for help in modifying the MN-151 to increase the joystick travel and Eddie Lee (JEG Engineering Supplies) for fabricating the other custom tools. This protocol was used in Ng et al., 2019. C.T. Ng and L. Gan were funded by Singapore Ministry of Education grant MOE2018-T2-2-146. M.S. Ladinsky was funded by National Institutes of Health grant (2 P50 GM082545-08) to Pamela J. Bjorkman. The authors declare no competing financial interests.

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August 20, 2023
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