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用于细胞冷冻电子断层成像的微纳加工工具及相关方法。

Micromachining tools and correlative approaches for cellular cryo-electron tomography.

机构信息

Max Planck Institute of Biochemistry, Department of Molecular Structural Biology, Am Klopferspitz 18, D-82152 Martinsried, Germany.

出版信息

J Struct Biol. 2010 Nov;172(2):169-79. doi: 10.1016/j.jsb.2010.02.011. Epub 2010 Feb 21.

Abstract

A principal limitation of cryo-transmission electron microscopy performed on cells or tissues is the accessible specimen thickness. This is exacerbated in tomography applications, where the aspect ratio (and thus the apparent specimen thickness) changes considerably during specimen tilting. Cryo-ultramicrotomy is the most obvious way of dealing with this problem; however, frozen-hydrated sections suffer from potentially inconsistent compression that cannot be corrected with certainty, and furthermore, yields of sections that satisfy all of the conditions necessary for tomographic imaging are poor. An alternative approach that avoids mechanical deformations is the use of focused ion beam (FIB) instrumentation, where thinning of the frozen-hydrated specimen occurs through the process of sputtering with heavy ions, typically gallium. Here, we use correlative cryo-fluorescence microscopy to navigate large cellular volumes and to localize specific cellular targets. We show that the selected targets in frozen-hydrated specimens can be accessed directly by focused ion beam milling. We also introduce a novel cryo-planing procedure as a method that could facilitate thinning of large areas of vitreous ice prior to cryo-fluorescence, FIB thinning, and cryo-electron tomography.

摘要

在细胞或组织上进行低温传输电子显微镜观察的主要限制因素是可接触的样本厚度。在断层扫描应用中,这个问题更加严重,因为在样本倾斜过程中,纵横比(因此,表观样本厚度)会发生很大变化。低温超薄切片是解决这个问题最明显的方法;然而,冷冻水合切片可能会受到无法确定的、不一致的压缩,并且无法满足断层成像所需的所有条件的切片产量也很差。避免机械变形的另一种方法是使用聚焦离子束(FIB)仪器,其中通过用重离子(通常是镓)溅射来使冷冻水合样本变薄。在这里,我们使用相关的低温荧光显微镜来导航大的细胞体积并定位特定的细胞目标。我们表明,可以通过聚焦离子束铣削直接访问冷冻水合样本中的选定目标。我们还引入了一种新的低温刨削程序,作为一种可以在低温荧光、FIB 变薄和低温电子断层扫描之前促进玻璃态冰大面积变薄的方法。

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