4.5 Article

High-speed high-resolution data collection on a 200 keV cryo-TEM

Journal

IUCRJ
Volume 9, Issue -, Pages 243-252

Publisher

INT UNION CRYSTALLOGRAPHY
DOI: 10.1107/S2052252522000069

Keywords

cryo-electron microscopy; 200 keV cryo-TEM; beam image shift; direct-electron detector

Funding

  1. National Cancer Institute of the National Institute of Health [P30CA016086]
  2. Core Facility Advocacy Committee and Office of Research Technologies, UNC Chapel Hill School of Medicine

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This study tested key parameters to increase the data collection speed in single-particle cryo-EM and successfully obtained high-resolution EM maps of mouse apoferritin. By using specific methods and operating procedures, rapid determination of single-particle cryo-EM structures can be achieved.
Limitations to successful single-particle cryo-electron microscopy (cryo-EM) projects include stable sample generation, production of quality cryo-EM grids with randomly oriented particles embedded in thin vitreous ice and access to microscope time. To address the limitation of microscope time, methodologies to more efficiently collect data on a 200 keV Talos Arctica cryo-transmission electron microscope at speeds as fast as 720 movies per hour (similar to 17 000 per day) were tested. In this study, key parameters were explored to increase data collection speed including: (1) using the beam-image shift method to acquire multiple images per stage position, (2) employing UltrAufoil TEM grids with R0.6/1 hole spacing, (3) collecting hardware-binned data and (4) adjusting the image shift delay factor in SerialEM. Here, eight EM maps of mouse apoferritin at 1.8-1.9 angstrom resolution were obtained in the analysis with data collection times for each dataset ranging from 56 min to 2 h. An EM map of mouse apoferritin at 1.78 angstrom was obtained from an overnight data collection at a speed of 500 movies per hour and subgroup analysis performed, with no significant variation observed in data quality by image shift distance and image shift delay. The findings and operating procedures detailed herein allow for rapid turnover of single-particle cryo-EM structure determination.

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