Abstract
The three-dimensional positions of atoms in protein molecules define their structure and their roles in biological processes. The more precisely atomic coordinates are determined, the more chemical information can be derived and the more mechanistic insights into protein function may be inferred. Electron cryo-microscopy (cryo-EM) single-particle analysis has yielded protein structures with increasing levels of detail in recent years1,2. However, it has proved difficult to obtain cryo-EM reconstructions with sufficient resolution to visualize individual atoms in proteins. Here we use a new electron source, energy filter and camera to obtain a 1.7Å resolution cryo-EM reconstruction for a human membrane protein, the β3 GABAA receptor homopentamer3. Such maps allow a detailed understanding of small-molecule coordination, visualization of solvent molecules and alternative conformations for multiple amino acids, and unambiguous building of ordered acidic side chains and glycans. Applied to mouse apoferritin, our strategy led to a 1.22Å resolution reconstruction that offers a genuine atomic-resolution view of a protein molecule using single-particle cryo-EM. Moreover, the scattering potential from many hydrogen atoms can be visualized in difference maps, allowing a direct analysis of hydrogen-bonding networks. Our technological advances, combined with further approaches to accelerate data acquisition and improve sample quality, provide a route towards routine application of cryo-EM in high-throughput screening of small molecule modulators and structure-based drug discovery.
Highlights
Multiple factors determine the attainable resolution of reconstructions from cryo-EM images of individual biological macromolecules and their complexes[4]
By performing tip flashing every 6-10 hours, based on automated monitoring of the beam current in the data acquisition program EPU, we found that the cold" FEG (CFEG) beam current remains stable over multiple days (Extended Data Figure 1)
Application to a human GABAA receptor sample To evaluate the impact of the technological advances described above in a systematic manner and on a challenging sample, we focused on a ~200 kDa human membrane protein, a prototypical GABAA receptor (GABAAR) β3 homopentameric construct bound to its small molecule agonist, histamine[3,24]
Summary
Multiple factors determine the attainable resolution of reconstructions from cryo-EM images of individual biological macromolecules and their complexes[4]. We adapted our image processing software RELION22 (see Methods) to be able to read the new data format, allowing motion correction by the Bayesian polishing algorithm[23] and reconstructions of movie frames with the original 248 Hz time resolution of the camera.
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