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一种提高超薄冷冻切片质量的新方法;其在免疫胶体金电镜和电子冷冻断层相关技术中的应用。

A new approach to improve the quality of ultrathin cryo-sections; its use for immunogold EM and correlative electron cryo-tomography.

机构信息

Netherlands Cancer Institute, Antoni van Leeuwenhoek Hospital, Amsterdam, The Netherlands.

出版信息

J Struct Biol. 2011 Jul;175(1):62-72. doi: 10.1016/j.jsb.2011.03.022. Epub 2011 Apr 5.

Abstract

Cryo-ultramicrotomy can be used to obtain ultrathin cryo-sections from cryo-fixed or aldehyde-fixed cryo-protected vitreous biologic samples. For immuno-gold EM, cryo-sections are retrieved from the cryo-chamber on a droplet of a pick-up solution (paste-like and almost frozen) to which the sections attach. The sections are then placed on an EM specimen grid at room temperature. This procedure compromises the ultrastructure, resulting in folds, holes, and loss of the original material. In this paper we show the critical influence of humidity, stretching, and relief of compression during thawing of the sections. We show a new lift-up hinge device for semi-automated retrieval of cryo-sections that results in significantly improved section quality. This approach was also applied successfully to vitreous sections from high pressure frozen samples. An important advance is that these vitreous cryo-sections can now successfully be post-fixed and immunolabelled after thawing; this allows cryo-EM comparison with adjacent ribbons of sections still in the frozen hydrated state. These findings call for technical innovations aiming at automated cryo-ultramicrotomy in a fully controlled environment for improved localization of proteins within their 'close to native' cellular context and correlative electron cryo-tomography of consecutive ribbons of sections of one frozen hydrated sample.

摘要

低温超微切割技术可用于从低温固定或醛固定的低温保护玻璃体液生物样本中获得超薄的低温切片。对于免疫金电镜,低温切片从低温室中转移到一小滴(糊状且几乎冻结)的拾取溶液上,切片会附着在溶液上。然后将切片放在室温下的 EM 标本网格上。这个过程会影响超微结构,导致折叠、孔和原始材料的丢失。在本文中,我们展示了在切片解冻过程中湿度、拉伸和压缩缓解对超微结构的关键影响。我们展示了一种新的提升铰链装置,用于半自动检索低温切片,这显著提高了切片质量。这种方法也成功应用于高压冷冻样本的玻璃体液切片。一个重要的进展是,这些玻璃体液低温切片现在可以在解冻后进行后固定和免疫标记;这允许在解冻的水合状态下对相邻的切片进行冷冻电镜比较。这些发现呼吁针对在完全控制的环境中进行自动化低温超微切割的技术创新,以提高蛋白质在其“接近天然”细胞环境中的定位,并对一个冷冻水合样本的连续切片的电镜断层扫描进行相关研究。

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