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Quantitation of Cellular Receptors by a New Immunocytochemical Flow Cytometry Technique

机译:一种新的免疫细胞化学流式细胞仪技术对细胞受体的定量

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摘要

Flow cytometry provides a rapid qualitative method for analyzing the binding oj a fluorescent probe to a cell. To quantitate the binding of a probe using flow cytometry, one must be able to first calibrate the fluorescent signal with some known standard We have compared a new one-step method with a previous two-step method for determining the number of binding sites (receptors) on the surface of cells using immunofluorescent staining of the cells and analysis by flow cytometry. Experimentally, recombinant Chinese hamster ovary cells, expressing cell surface glycoprotein receptors, lib/Ilia or Mac-1, were assayed using specific mouse monoclonal antibodies against these receptors. The two methods yielded comparable results and, depending on the cell type, detected anywhere from 100000 to 300000 antibody-binding sites per cell, respectively.
机译:流式细胞术为分析荧光探针与细胞的结合提供了一种快速的定性方法。要使用流式细胞仪定量探针的结合,必须首先能够使用一些已知的标准品校准荧光信号。我们已经将一种新的一步法与先前的一种两步法进行了比较,以确定结合位点(受体)的数量。使用细胞的免疫荧光染色并通过流式细胞仪进行分析)。实验上,使用针对这些受体的特异性小鼠单克隆抗体对表达细胞表面糖蛋白受体,lib / Ilia或Mac-1的重组中国仓鼠卵巢细胞进行了分析。两种方法产生的结果相当,并且取决于细胞类型,每个细胞分别检测到100000至300000个抗体结合位点。

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