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使用相关原子力显微镜/荧光显微镜对核膜进行成像

Imaging Nuclear Envelopes Using Correlative AFM/Fluorescence Microscopy.

作者信息

Costes Emilie, Vial Anthony, Doucet Christine, Milhiet Pierre-Emmanuel

机构信息

Centre de Biologie Structurale, INSERM, CNRS, University of Montpellier, Montpellier, France.

University of Bordeaux, CNRS, Bordeaux INP, CBMN, UMR 5248, F-33600, Pessac, France.

出版信息

Methods Mol Biol. 2025;2958:45-69. doi: 10.1007/978-1-0716-4714-1_4.

DOI:10.1007/978-1-0716-4714-1_4
PMID:40833566
Abstract

The nuclear envelope (NE) is the hallmark of eukaryotic cells. It is a complex structure composed of two concentric lipid bilayers separated by a 50 nm lumen. While the outer nuclear membrane is continuous with the endoplasmic reticulum, the inner nuclear membrane contains a unique set of proteins. Methods have been developed several decades ago to prepare NEs from Xenopus laevis oocytes, exposing inner and outer nuclear membranes, which makes them ideal samples for probe scanning methods such as atomic force microscopy (AFM). In addition, biochemical preparations of human NEs have been valuable tools to investigate the structure of their nuclear pore complexes (NPCs). However, recent data have highlighted that membrane tension loss during NE preparation changes the morphology of NPCs. In this chapter, we outline a novel approach to extract nuclei from cultured mammalian cells, affix them onto glass substrates, and gently open them, thereby maintaining membrane tension and preserving NPC structure for subsequent AFM imaging of both inner and outer nuclear membranes. Furthermore, we detail a protocol for immuno-labeling and correlative imaging by AFM/dSTORM (direct Stochastic Optical Reconstruction Microscopy). Additionally, we provide comprehensive guidance on data analysis, in particular for proper correlation of the optical and AFM images. Notably, the sample preparation steps only require basic materials. The procedures described here could be easily extended to other cellular models such as plant cells or cells isolated from animal tissues.

摘要

核膜(NE)是真核细胞的标志。它是一种复杂的结构,由两个同心脂质双层组成,中间隔着50纳米的腔隙。外核膜与内质网连续,而内核膜含有一组独特的蛋白质。几十年前就已开发出从非洲爪蟾卵母细胞制备核膜的方法,可暴露出内核膜和外核膜,这使其成为原子力显微镜(AFM)等探针扫描方法的理想样本。此外,人核膜的生化制备一直是研究其核孔复合体(NPC)结构的宝贵工具。然而,最近的数据表明,核膜制备过程中膜张力的丧失会改变NPC的形态。在本章中,我们概述了一种从培养的哺乳动物细胞中提取细胞核、将其固定在玻璃基板上并轻轻打开的新方法,从而保持膜张力并保留NPC结构,以便随后对内、外核膜进行AFM成像。此外,我们详细介绍了免疫标记和AFM/dSTORM(直接随机光学重建显微镜)相关成像的方案。此外,我们还提供了数据分析的全面指导,特别是关于光学图像和AFM图像的正确关联。值得注意的是,样品制备步骤仅需要基本材料。这里描述的程序可以很容易地扩展到其他细胞模型,如植物细胞或从动物组织分离的细胞。

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本文引用的文献

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Structure and mechanics of the human nuclear pore complex basket using correlative AFM-fluorescence superresolution microscopy.使用相关原子力显微镜-荧光超分辨率显微镜研究人类核孔复合体篮的结构和力学性质。
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Architecture of the linker-scaffold in the nuclear pore.核孔中连接体-支架的结构。
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Architecture of the cytoplasmic face of the nuclear pore.核孔胞质面的结构。
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Structure of the cytoplasmic ring of the nuclear pore complex.核孔复合体胞质环的结构
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