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原位薄片的平行冷冻电子断层扫描术

Parallel cryo electron tomography on in situ lamellae.

作者信息

Eisenstein Fabian, Yanagisawa Haruaki, Kashihara Hiroka, Kikkawa Masahide, Tsukita Sachiko, Danev Radostin

机构信息

Graduate School of Medicine, University of Tokyo, Tokyo, Japan.

Advanced Comprehensive Research Organization, Teikyo University, Tokyo, Japan.

出版信息

Nat Methods. 2023 Jan;20(1):131-138. doi: 10.1038/s41592-022-01690-1. Epub 2022 Dec 1.

Abstract

In situ cryo electron tomography of cryo focused ion beam milled samples has emerged in recent years as a powerful technique for structural studies of macromolecular complexes in their native cellular environment. However, the possibilities for recording tomographic tilt series in a high-throughput manner are limited, in part by the lamella-shaped samples. Here we utilize a geometrical sample model and optical image shift to record tens of tilt series in parallel, thereby saving time and gaining access to sample areas conventionally used for tracking specimen movement. The parallel cryo electron tomography (PACE-tomo) method achieves a throughput faster than 5 min per tilt series and allows for the collection of sample areas that were previously unreachable, thus maximizing the amount of data from each lamella. Performance testing with ribosomes in vitro and in situ on state-of-the-art and general-purpose microscopes demonstrated the high throughput and quality of PACE-tomo.

摘要

近年来,冷冻聚焦离子束研磨样品的原位冷冻电子断层扫描已成为一种强大的技术,用于在天然细胞环境中对大分子复合物进行结构研究。然而,以高通量方式记录断层倾斜系列的可能性有限,部分原因是薄片形状的样品。在这里,我们利用几何样品模型和光学图像移位来并行记录数十个倾斜系列,从而节省时间并能够获取传统上用于跟踪样品移动的样品区域。并行冷冻电子断层扫描(PACE-tomo)方法实现了每个倾斜系列快于5分钟的通量,并允许收集以前无法到达的样品区域,从而最大化每个薄片的数据量。在最先进的通用显微镜上对核糖体进行体外和原位性能测试,证明了PACE-tomo的高通量和高质量。

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