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通过单颗粒冷冻电镜从无序二维晶体中获取高分辨率信息。

Retrieving high-resolution information from disordered 2D crystals by single-particle cryo-EM.

作者信息

Righetto Ricardo D, Biyani Nikhil, Kowal Julia, Chami Mohamed, Stahlberg Henning

机构信息

Center for Cellular Imaging and NanoAnalytics, Biozentrum, University of Basel, Mattenstrasse 26, CH-4058, Basel, Switzerland.

Institute for Molecular Biology and Biophysics, ETH Zürich, Otto-Stern-Weg 5, CH-8093, Zürich, Switzerland.

出版信息

Nat Commun. 2019 Apr 12;10(1):1722. doi: 10.1038/s41467-019-09661-5.

Abstract

Electron crystallography can reveal the structure of membrane proteins within 2D crystals under close-to-native conditions. High-resolution structural information can only be reached if crystals are perfectly flat and highly ordered. In practice, such crystals are difficult to obtain. Available image unbending algorithms correct for disorder, but only perform well on images of non-tilted, flat crystals, while out-of-plane distortions are not addressed. Here, we present an approach that employs single-particle refinement procedures to locally unbend crystals in 3D. With this method, density maps of the MloK1 potassium channel with a resolution of 4 Å were obtained from images of 2D crystals that do not diffract beyond 10 Å. Furthermore, 3D classification allowed multiple structures to be resolved, revealing a series of MloK1 conformations within a single 2D crystal. This conformational heterogeneity explains the poor diffraction observed and is related to channel function. The approach is implemented in the FOCUS package.

摘要

电子晶体学能够在接近天然的条件下揭示二维晶体中膜蛋白的结构。只有当晶体完美平整且高度有序时,才能获得高分辨率的结构信息。实际上,这样的晶体很难获得。现有的图像矫正算法可以校正无序情况,但仅在非倾斜、平整晶体的图像上表现良好,而面外畸变问题并未得到解决。在此,我们提出一种方法,该方法采用单颗粒精修程序在三维空间中对晶体进行局部矫正。通过这种方法,从衍射极限不超过10 Å的二维晶体图像中获得了分辨率为4 Å的MloK1钾通道密度图。此外,三维分类使多种结构得以解析,揭示了单个二维晶体内一系列MloK1构象。这种构象异质性解释了所观察到的衍射不佳现象,并与通道功能相关。该方法已在FOCUS软件包中实现。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d0c2/6461647/e23bc3da5bbf/41467_2019_9661_Fig1_HTML.jpg

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