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A basic introduction to single particles cryo-electron microscopy

机译:单颗粒冷冻电子显微镜的基本介绍

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摘要

In the last years, cryogenic-electron microscopy (cryo-EM) underwent the most impressive improvement compared to other techniques used in structural biology, such as X-ray crystallography and NMR. Electron microscopy was invented nearly one century ago but, up to the beginning of the last decades, the 3D maps produced through this technique were poorly detailed, justifying the term "blobbology" to appeal to cryo-EM. Recently, thanks to a new generation of microscopes and detectors, more efficient algorithms, and easier access to computational power, single particles cryo-EM can routinely produce 3D structures at resolutions comparable to those obtained with X-ray crystallography. However, unlike X-ray crystallography, which needs crystallized proteins, cryo-EM exploits purified samples in solution, allowing the study of proteins and protein complexes that are hard or even impossible to crystallize. For these reasons, single-particle cryo-EM is often the first choice of structural biologists today. Nevertheless, before starting a cryo-EM experiment, many drawbacks and limitations must be considered. Moreover, in practice, the process between the purified sample and the final structure could be trickier than initially expected. Based on these observations, this review aims to offer an overview of the principal technical aspects and setups to be considered while planning and performing a cryo-EM experiment.
机译:在过去的几年里,与结构生物学中使用的其他技术(如X射线晶体学和核磁共振)相比,低温电子显微镜(cryo-EM)经历了最令人印象深刻的改进。电子显微镜是在近一个世纪前发明的,但直到最近几十年的开始,通过这种技术产生的3D图谱的细节都很差,这证明了“斑点学”一词对冷冻电镜的吸引力是合理的。最近,由于新一代显微镜和探测器、更高效的算法以及更容易获得计算能力,单粒子冷冻电镜可以通常以与X射线晶体学相当的分辨率产生3D结构。然而,与需要结晶蛋白质的 X 射线晶体学不同,冷冻电镜利用溶液中的纯化样品,可以研究难以甚至不可能结晶的蛋白质和蛋白质复合物。由于这些原因,单颗粒冷冻电镜通常是当今结构生物学家的首选。然而,在开始冷冻电镜实验之前,必须考虑许多缺点和局限性。此外,在实践中,纯化样品和最终结构之间的过程可能比最初预期的要棘手。基于这些观察结果,本综述旨在概述在规划和执行冷冻电镜实验时要考虑的主要技术方面和设置。

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