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多粒子冷冻电镜重构技术 M 成功解析了细胞内 3.5Å 分辨率的核糖体-抗生素复合物。

Multi-particle cryo-EM refinement with M visualizes ribosome-antibiotic complex at 3.5 Å in cells.

机构信息

Department of Molecular Biology, Max Planck Institute for Biophysical Chemistry, Göttingen, Germany.

Structural and Computational Biology Unit, European Molecular Biology Laboratory (EMBL), Heidelberg, Germany.

出版信息

Nat Methods. 2021 Feb;18(2):186-193. doi: 10.1038/s41592-020-01054-7. Epub 2021 Feb 4.

Abstract

Cryo-electron microscopy (cryo-EM) enables macromolecular structure determination in vitro and inside cells. In addition to aligning individual particles, accurate registration of sample motion and three-dimensional deformation during exposures are crucial for achieving high-resolution reconstructions. Here we describe M, a software tool that establishes a reference-based, multi-particle refinement framework for cryo-EM data and couples a comprehensive spatial deformation model to in silico correction of electron-optical aberrations. M provides a unified optimization framework for both frame-series and tomographic tilt-series data. We show that tilt-series data can provide the same resolution as frame-series data on a purified protein specimen, indicating that the alignment step no longer limits the resolution obtainable from tomographic data. In combination with Warp and RELION, M resolves to residue level a 70S ribosome bound to an antibiotic inside intact bacterial cells. Our work provides a computational tool that facilitates structural biology in cells.

摘要

低温电子显微镜(cryo-EM)可实现体外和细胞内的大分子结构测定。除了对准单个粒子外,在曝光过程中准确记录样品运动和三维变形对于实现高分辨率重构至关重要。在这里,我们描述了 M,这是一个软件工具,它为 cryo-EM 数据建立了基于参考的多粒子精修框架,并将全面的空间变形模型与电子光学像差的计算机校正相结合。M 为帧系列和断层倾斜系列数据提供了统一的优化框架。我们表明,倾斜系列数据可以在纯化蛋白样品上提供与帧系列数据相同的分辨率,这表明对准步骤不再限制从断层数据获得的分辨率。与 Warp 和 RELION 结合使用,M 可以解析到残基水平,解析出与完整细菌细胞内抗生素结合的 70S 核糖体。我们的工作提供了一种计算工具,有助于细胞内的结构生物学。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/70b4/7611018/93c5af9632ae/EMS114919-f008.jpg

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