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在三维软骨细胞培养中获取细胞骨架和细胞核的四色共聚焦荧光图像的最佳处理方法。

Optimal processing method to obtain four-color confocal fluorescent images of the cytoskeleton and nucleus in three-dimensional chondrocyte cultures.

作者信息

Blanc Antoine, Tran-Khanh Nicolas, Filion Dominic, Buschmann Michael D

机构信息

Department of Chemical Engineering, Ecole Polytechnique, PO 6079, Station Centre-ville, Montreal, QC, Canada H3C 3A7.

出版信息

J Histochem Cytochem. 2005 Sep;53(9):1171-5. doi: 10.1369/jhc.5B6728.2005. Epub 2005 Jun 2.

Abstract

Tissue engineering of articular cartilage requires accurate imaging of the chondrocyte cytoskeleton. Past studies have applied various fixation and permeabilization protocols without optimization of parameters. In this study, we have examined procedures using glutaraldehyde and paraformaldehyde as fixatives and Triton X-100 and Octyl-POE as permeabilizing detergents. A four-color fluorescence confocal method was developed to simultaneously image actin, tubulin, vimentin, and the nucleus. We found optimal preservation and morphology of the chondrocyte cytoskeleton after simultaneous fixation and permeabilization with glutaraldehyde and Triton X-100. These images displayed less cellular shrinkage and higher-resolution filamentous structures than with paraformaldehyde or when permeabilization followed fixation.

摘要

关节软骨组织工程需要对软骨细胞细胞骨架进行精确成像。过去的研究应用了各种固定和通透方案,但未对参数进行优化。在本研究中,我们研究了使用戊二醛和多聚甲醛作为固定剂以及 Triton X-100 和辛基 - POE 作为通透去污剂的程序。开发了一种四色荧光共聚焦方法来同时对肌动蛋白、微管蛋白、波形蛋白和细胞核进行成像。我们发现,在用戊二醛和 Triton X-100 同时进行固定和通透处理后,软骨细胞细胞骨架得到了最佳保存且形态良好。与使用多聚甲醛时或先固定后通透相比,这些图像显示出更少的细胞收缩和更高分辨率的丝状结构。

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