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活细胞中的超分辨率成像。

Super-resolution imaging in live cells.

作者信息

Cox Susan

机构信息

Randall Division of Cell and Molecular Biophysics, King׳s College London, SE1 1UL, UK.

出版信息

Dev Biol. 2015 May 1;401(1):175-81. doi: 10.1016/j.ydbio.2014.11.025. Epub 2014 Dec 10.

Abstract

Over the last twenty years super-resolution fluorescence microscopy has gone from proof-of-concept experiments to commercial systems being available in many labs, improving the resolution achievable by up to a factor of 10 or more. There are three major approaches to super-resolution, stimulated emission depletion microscopy, structured illumination microscopy, and localisation microscopy, which have all produced stunning images of cellular structures. A major current challenge is optimising performance of each technique so that the same sort of data can be routinely taken in live cells. There are several major challenges, particularly phototoxicity and the speed with which images of whole cells, or groups of cells, can be acquired. In this review we discuss the various approaches which can be successfully used in live cells, the tradeoffs in resolution, speed, and ease of implementation which one must make for each approach, and the quality of results that one might expect from each technique.

摘要

在过去二十年中,超分辨率荧光显微镜已从概念验证实验发展到许多实验室都可使用的商业系统,将可实现的分辨率提高了10倍或更多。超分辨率有三种主要方法,即受激发射损耗显微镜、结构照明显微镜和定位显微镜,它们都产生了令人惊叹的细胞结构图像。当前的一个主要挑战是优化每种技术的性能,以便能够在活细胞中常规获取同类数据。存在几个主要挑战,特别是光毒性以及获取整个细胞或细胞群图像的速度。在本综述中,我们讨论了可成功用于活细胞的各种方法、每种方法在分辨率、速度和实施难易程度方面必须做出的权衡,以及每种技术可能获得的结果质量。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8e34/4405210/6d33bebafe3e/gr1.jpg

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