Measurement of estrogen receptors in intact cells by flow cytometry.

Cytometry Pub Date : 2000-10-01
S Cao, S D Hudnall, F Kohen, L J Lu
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Abstract

Background: Estrogen receptor (ER) levels in tumor cells are important for determining the outcome of treatment and the prognosis of breast cancer patients. Flow cytometry is a convenient tool for quantifying the ER in cells, but a more sensitive, reproducible method for immunostaining the ER with anti-ER antibody is needed. Materials and Methods ER-positive human breast cancer cells MCF-7 and T47D, and ER-negative MDA-MBA-321 cells, were fixed and permeabilized by three different protocols. The cells were then stained by indirect immunofluorescence, using two commercial antibodies to ER (MA1-310 and DAKO 1D5), or by direct immunofluorescence using FITC-labeled anti-idiotypic antibody clone 1D(5). The stained cells were analyzed by flow cytometry.

Results: The fixation of cells with a mixture of 0.25% paraformaldehyde and 70% methanol, permeabilization with 0.05% Triton X-100, and increasing antibody and antigen reaction time led to 80-99% of cells being stained with anti-ER antibodies. The relative brightness of ER immunostaining was as follows: anti-idiotypic antibody ID5 > MA1-310 > DAKO 1D5.

Conclusions: Direct immunofluorescence with the FITC-labeled anti-idiotypic antibody of permeabilized cells resulted in improved specific staining of the ER, as compared to indirect immunofluorescence with anti-ER antibodies of fixed and permeabilized cells. Increasing the length of staining, and treatment of cells with Triton X-100, are both necessary to improve the staining of intracellular antigen for flow cytometric analysis.

流式细胞术检测完整细胞雌激素受体。
背景:肿瘤细胞中雌激素受体(ER)水平对乳腺癌患者的治疗效果和预后有重要影响。流式细胞术是一种方便的定量细胞内质网的工具,但需要一种更灵敏、可重复的方法来用抗内质网抗体对内质网进行免疫染色。材料和方法采用三种不同的方法固定和渗透er阳性的人乳腺癌细胞MCF-7和T47D,以及er阴性的MDA-MBA-321细胞。然后用间接免疫荧光染色细胞,使用两种商业ER抗体(MA1-310和DAKO 1D5),或直接免疫荧光染色使用fitc标记的抗独特型抗体克隆1D(5)。流式细胞术分析染色细胞。结果:用0.25%多聚甲醛和70%甲醇的混合物固定细胞,用0.05% Triton X-100渗透,增加抗体和抗原反应时间,80-99%的细胞被抗er抗体染色。ER免疫染色相对亮度为:抗独特型抗体ID5 > MA1-310 > DAKO 1D5。结论:与使用固定细胞和渗透细胞的抗ER抗体进行间接免疫荧光相比,使用fitc标记的渗透细胞抗独特型抗体进行直接免疫荧光可提高内质网的特异性染色。增加染色时间,并用Triton X-100处理细胞,都是改善流式细胞术分析中细胞内抗原染色的必要条件。
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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