A tridimensional view of the organization of actin filaments in the central nervous system by use of fluorescent photooxidation.

F. Capani, E. Saraceno, V. Boti, Laura Aon-Bertolino, J. C. Fernández, Fernándo Gato, M. Kruse, L. Giraldez, Mark Ellisman, H. Coirini
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引用次数: 9

Abstract

Cellular and subcellular organization and distribution of actin filaments have been studied with various techniques. The use of fluorescence photo-oxidation combined with phalloidin conjugates with eosin has allowed the examination of the precise cellular and subcellular location of F-actin. Correlative fluorescence light microscopy and transmission electron microscopy studies of F-actin distribution are facilitated with this method for morphological and physiological studies. Because phalloidin-eosin is smaller than other markers, this method allows the analysis of the three-dimensional location of F-actin with high-resolution light microscopy, three-d serial sections reconstructions, and electron tomography. The combination of selective staining and three-dimensional reconstructions provide a valuable tool for revealing aspects of the synaptic morphology that are not available when conventional electron microscopy is used. By applying this selective staining technique and three-dimensional imaging, we uncovered the structural organization of actin in the postsynaptic densities in physiological and pathological conditions.
用荧光光氧化法观察中枢神经系统中肌动蛋白丝的三维结构。
肌动蛋白丝的细胞和亚细胞组织和分布已经用各种技术进行了研究。使用荧光光氧化结合与伊红结合的phalloidin已经允许检查精确的细胞和亚细胞位置的f -肌动蛋白。该方法可用于相关的荧光显微镜和透射电镜对f -肌动蛋白分布进行形态学和生理学研究。由于phalloidin-eosin比其他标记物更小,该方法允许使用高分辨率光学显微镜、三维连续切片重建和电子断层扫描分析F-actin的三维位置。选择性染色和三维重建的结合提供了一个有价值的工具来揭示突触形态的各个方面,当使用传统的电子显微镜时是不可用的。通过这种选择性染色技术和三维成像,我们揭示了生理和病理条件下肌动蛋白在突触后密度中的结构组织。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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