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在水相条件下使用去顶技术对细胞内细胞骨架进行原子力显微镜成像。

Use of the unroofing technique for atomic force microscopic imaging of the intra-cellular cytoskeleton under aqueous conditions.

作者信息

Usukura Jiro, Yoshimura Azumi, Minakata Shiho, Youn Daehwan, Ahn Jeonghun, Cho Sang-Joon

机构信息

EcoTopia Science Institute, Nagoya University, Nagoya, Japan.

出版信息

J Electron Microsc (Tokyo). 2012;61(5):321-6. doi: 10.1093/jmicro/dfs055. Epub 2012 Aug 7.

Abstract

Atomic force microscopy (AFM) combined with unroofing techniques enabled clear imaging of the intracellular cytoskeleton and the cytoplasmic surface of the cell membrane under aqueous condition. Many actin filaments were found to form a complex meshwork on the cytoplasmic surface of the membrane, as observed in freeze-etching electron microscopy. Characteristic periodic striations of about 5 nm formed by the assembly of G-actin were detected along actin filaments at higher magnification. Actin filaments aggregated and dispersed at several points, thereby dividing the cytoplasmic surface of the membrane into several large domains. Microtubules were also easily detected and were often tethered to the membrane surface by fine filaments. Furthermore, clathrin coats on the membrane were clearly visualized for the first time in water by AFM. Although the resolution of these images is lower than electron micrographs of freeze-etched samples processed similarly, the measurement capabilities of the AFM in a more biologically relevant conditions demonstrate that it is an important tool for imaging intracellular structures and cell surfaces in the native, aqueous state.

摘要

原子力显微镜(AFM)与去顶技术相结合,能够在水性条件下清晰成像细胞内细胞骨架和细胞膜的细胞质表面。如在冷冻蚀刻电子显微镜中观察到的那样,发现许多肌动蛋白丝在膜的细胞质表面形成复杂的网络。在更高放大倍数下,沿着肌动蛋白丝检测到由G-肌动蛋白组装形成的约5纳米的特征性周期性条纹。肌动蛋白丝在几个点聚集和分散,从而将膜的细胞质表面分成几个大区域。微管也很容易被检测到,并且经常通过细丝系在膜表面。此外,AFM首次在水中清晰地观察到膜上的网格蛋白包被。尽管这些图像的分辨率低于以类似方式处理的冷冻蚀刻样品的电子显微照片,但AFM在更具生物学相关性的条件下的测量能力表明,它是在天然水性状态下对细胞内结构和细胞表面进行成像的重要工具。

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