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在标准FACScan上使用异硫氰酸荧光素、别藻蓝蛋白和碘化丙啶同时测量两种细胞抗原和DNA。

Simultaneous measurement of two cellular antigens and DNA using fluorescein-isothiocyanate, R-phycoerythrin, and propidium iodide on a standard FACScan.

作者信息

Corver W E, Cornelisse C J, Fleuren G J

机构信息

Department of Pathology, University of Leiden, The Netherlands.

出版信息

Cytometry. 1994 Feb 1;15(2):117-28. doi: 10.1002/cyto.990150205.

DOI:10.1002/cyto.990150205
PMID:8168399
Abstract

Multiparameter flow cytometry is a powerful tool for analyzing the phenotypic, cell kinetic, and ploidy heterogeneity of tumor cell populations. Because of the substantial spectral overlap of propidium iodide (PI) and R-phycoerythrin (PE) fluorescence emission, this combined use of these fluorochromes has been thought not to be feasible on a standard flow cytometer for these kind of studies. Instead of PI, 7-amino-actinomycin D (7-AAD) is used as DNA stain. In this paper however, we show that PI can be used as a DNA stain in combination with fluorescein isothiocyanate (FITC) and R-phycoerythrin (PE) on a standard FACScan. Three established ovarian cancer cell lines (IGROV1, NIH: OVCAR-3, and COV362.c14) were used for these experiments. Cells were fixed with 1.0% paraformaldehyde and permeabilized with various concentrations of lysolecithin for the simultaneous detection of surface antigens by monoclonal antibodies MOv18, BMA180 or OV632, intermediate filament antigens (keratin 18 or vimentin), and DNA. A final concentration of 80 micrograms/ml lysolecithin was found to give optimal results. The emission spectrum overlap from PI into the orange fluorescence channel (FL2) used for PE fluorescence detection could be sufficiently compensated up to a photomultiplier tube potential of about 440 Volts (V) required at the FL2 channel. Using the same instrument settings, 5.10 x 10(4) PE equivalents were detectable. Under these conditions, CVs obtained for the DNA histograms ranged from 3.0-4.1. Application of the method on a mixture of activated peripheral blood lymphocytes and ovarian tumor cells resulted in a clear separation of the two populations both by surface and cytoplasmic antigen expression and DNA content.

摘要

多参数流式细胞术是分析肿瘤细胞群体的表型、细胞动力学和倍体异质性的有力工具。由于碘化丙啶(PI)和藻红蛋白(PE)荧光发射存在大量光谱重叠,人们一直认为在标准流式细胞仪上联合使用这两种荧光染料进行此类研究是不可行的。7-氨基放线菌素D(7-AAD)被用作DNA染色剂,而非PI。然而,在本文中,我们表明PI可在标准FACScan上与异硫氰酸荧光素(FITC)和藻红蛋白(PE)联合用作DNA染色剂。这些实验使用了三种已建立的卵巢癌细胞系(IGROV1、NIH:OVCAR-3和COV362.c14)。细胞用1.0%多聚甲醛固定,并用不同浓度的溶血卵磷脂进行通透处理,以便通过单克隆抗体MOv18、BMA180或OV632同时检测表面抗原、中间丝抗原(角蛋白18或波形蛋白)和DNA。发现最终浓度为80微克/毫升的溶血卵磷脂可产生最佳结果。PI进入用于PE荧光检测的橙色荧光通道(FL2)的发射光谱重叠在FL2通道所需的约440伏(V)光电倍增管电位下可得到充分补偿。使用相同的仪器设置,可检测到5.10×10⁴个PE当量。在这些条件下,DNA直方图的变异系数(CV)范围为3.0 - 4.1。将该方法应用于活化外周血淋巴细胞和卵巢肿瘤细胞的混合物,通过表面和细胞质抗原表达以及DNA含量可清晰分离这两种细胞群体。

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