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低温荧光显微镜有助于光学显微镜与低温电子显微镜之间的关联,并降低光漂白速率。

Cryo-fluorescence microscopy facilitates correlations between light and cryo-electron microscopy and reduces the rate of photobleaching.

作者信息

Schwartz Cindi L, Sarbash Vasily I, Ataullakhanov Fazoil I, McIntosh J Richard, Nicastro Daniela

机构信息

Boulder Laboratory for 3D Electron Microscopy of Cells, University of Colorado, Department of Molecular, Cellular, and Developmental Biology, Boulder, CO, USA.

出版信息

J Microsc. 2007 Aug;227(Pt 2):98-109. doi: 10.1111/j.1365-2818.2007.01794.x.

Abstract

Fluorescence light microscopy (LM) has many advantages for the study of cell organization. Specimen preparation is easy and relatively inexpensive, and the use of appropriate tags gives scientists the ability to visualize specific proteins of interest. LM is, however, limited in resolution, so when one is interested in ultrastructure, one must turn to electron microscopy (EM), even though this method presents problems of its own. The biggest difficulty with cellular EM is its limited utility in localizing macromolecules of interest while retaining good structural preservation. We have built a cryo-light microscope stage that allows us to generate LM images of vitreous samples prepared for cryo-EM. Correlative LM and EM allows one to find areas of particular interest by using fluorescent proteins or vital dyes as markers within vitrified samples. Once located, the sample can be placed in the EM for further study at higher resolution. An additional benefit of the cryo-LM stage is that photobleaching is slower at cryogenic temperatures (-140 degrees C) than at room temperature.

摘要

荧光光学显微镜(LM)在细胞组织研究方面具有诸多优势。样本制备简便且成本相对较低,使用合适的标记物能使科学家可视化感兴趣的特定蛋白质。然而,LM的分辨率有限,因此当人们对超微结构感兴趣时,就必须借助电子显微镜(EM),即便这种方法自身也存在问题。细胞EM最大的困难在于,在保留良好结构保存的同时,其在定位感兴趣的大分子方面实用性有限。我们构建了一个低温光学显微镜载物台,它能让我们生成用于低温EM的玻璃态样本的LM图像。相关的LM和EM使人们能够通过使用荧光蛋白或活性染料作为玻璃化样本中的标记物来找到特别感兴趣的区域。一旦找到,样本就可以放入EM中以更高分辨率进行进一步研究。低温LM载物台的另一个好处是,在低温(-140摄氏度)下光漂白比在室温下更慢。

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