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通过荧光原位杂交检测核仁组织区和细胞核糖体RNA的光镜与荧光显微镜联合成像。

Combined light and fluorescent microscopical imaging of nucleolar organizer regions and cellular rRNA as detected by fluorescent in situ hybridization.

作者信息

Pajor L, Honeyman T W

机构信息

Department of Surgery, University of Massachusetts Medical Center, Worcester, USA.

出版信息

Cytometry. 1995 Feb 1;19(2):171-6. doi: 10.1002/cyto.990190212.

Abstract

A method for combined light and fluorescent microscopic imaging of nucleolar organizer regions and cellular rRNA is described. Nucleolar organizer regions were detected by silver staining (Ag-NOR), and rRNA was detected by fluorescent in situ hybridization (FISH). MG-63 human fibrosarcoma cells were silver stained prior to in situ hybridization. To quantitate Ag-NOR within individual cells, brightfield images were digitized, and the total Ag-NOR area/nucleus was determined. Fluorescent images were digitized, and the total cellular fluorescence was calculated after correction for nonuniformity of illumination. By using this method, it was shown that the Ag-NOR procedure did not significantly affect the fluorescence intensity related to FISH. Furthermore, the hybridization procedure did not interfere with quantitation of Ag-NOR. With this method, both Ag-NOR and rRNA product can be quantitated within the same cell. Because the relationship of rRNA content to cell proliferation is well established, correlation to quantitative Ag-NOR parameters within individual cells will contribute to the better definition of the relationship of quantitative Ag-NOR indices with cellular proliferation.

摘要

本文描述了一种用于核仁组织区和细胞rRNA的光镜与荧光显微镜联合成像方法。核仁组织区通过银染法(Ag-NOR)检测,rRNA通过荧光原位杂交(FISH)检测。MG-63人纤维肉瘤细胞在原位杂交前进行银染。为了对单个细胞内的Ag-NOR进行定量,将明场图像数字化,并确定每个细胞核的Ag-NOR总面积。将荧光图像数字化,并在对光照不均匀性进行校正后计算细胞总荧光强度。通过使用该方法,结果表明Ag-NOR程序不会显著影响与FISH相关的荧光强度。此外,杂交程序不会干扰Ag-NOR的定量。使用该方法,可以在同一个细胞内对Ag-NOR和rRNA产物进行定量。由于rRNA含量与细胞增殖之间的关系已得到充分确立,因此单个细胞内Ag-NOR定量参数的相关性将有助于更好地定义定量Ag-NOR指标与细胞增殖之间的关系。

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