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用于电子显微镜观察的非洲爪蟾卵母细胞生发泡的阴影核膜制备。

Preparation of shadowed nuclear envelopes from Xenopus oocyte germinal vesicles for electron microscopy.

作者信息

Whytock S, Stewart M

机构信息

MRC Laboratory of Molecular Biology, Cambridge.

出版信息

J Microsc. 1988 Aug;151(Pt 2):115-26. doi: 10.1111/j.1365-2818.1988.tb04618.x.

DOI:10.1111/j.1365-2818.1988.tb04618.x
PMID:3216383
Abstract

Methods for examining the structure of the nuclear envelope of oocytes of Xenopus laevis by electron microscopy using metal shadowing have been developed and evaluated. Minor modifications were made to existing methods for preparing specimens by freeze drying, mainly to eliminate unnecessary steps and a rapid method for examining the structure and arrangement of nuclear envelope components, based on dehydration in an ethanol series followed by amyl acetate and then air drying, was also developed. The preservation of the lamina and connections between the nuclear pore complexes using the rapid air drying method was satisfactory for observing the fibrous components of the envelope and their attachment to the pores. Furthermore, air drying required only simple laboratory apparatus and, moreover, offered several advantages compared to freeze drying when assessing the effect of various disruptive treatments on the nuclear envelope or examining the connections between its components. In specimens prepared by either the more rapid air drying method or by freeze drying, the lamina meshwork beneath the nuclear face of the envelope was clear, but the fine structure of the nuclear pore complexes was superior in freeze dried preparations. In views of the nucleoplasmic face of the envelope, the lamina meshwork was suspended above the support film in freeze dried preparations, but collapsed in most air dried specimens. This collapse was not without its advantages, however, as it facilitated observation of the connections between nuclear pore complexes and lamina fibres, which were often masked in freeze dried preparations.

摘要

已经开发并评估了使用金属阴影法通过电子显微镜检查非洲爪蟾卵母细胞核膜结构的方法。对现有的冷冻干燥标本制备方法进行了细微修改,主要是为了消除不必要的步骤,还开发了一种基于乙醇系列脱水、然后乙酸戊酯脱水并随后空气干燥的快速方法,用于检查核膜成分的结构和排列。使用快速空气干燥法对核纤层和核孔复合体之间连接的保存,对于观察核膜的纤维成分及其与孔的附着情况来说是令人满意的。此外,空气干燥只需要简单的实验室设备,而且在评估各种破坏处理对核膜的影响或检查其成分之间的连接时,与冷冻干燥相比具有几个优点。在通过更快速的空气干燥法或冷冻干燥法制备的标本中,核膜核面下方的核纤层网络清晰可见,但核孔复合体的精细结构在冷冻干燥的制剂中更优。从核膜的核质面来看,在冷冻干燥的制剂中,核纤层网络悬浮在支持膜上方,但在大多数空气干燥的标本中会塌陷。然而,这种塌陷并非没有优点,因为它便于观察核孔复合体与核纤层纤维之间的连接,而这些连接在冷冻干燥的制剂中常常被掩盖。

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Preparation of shadowed nuclear envelopes from Xenopus oocyte germinal vesicles for electron microscopy.用于电子显微镜观察的非洲爪蟾卵母细胞生发泡的阴影核膜制备。
J Microsc. 1988 Aug;151(Pt 2):115-26. doi: 10.1111/j.1365-2818.1988.tb04618.x.
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