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改进的FACS-Gal:对表达报告基因构建体的活真核细胞进行流式细胞术分析和分选。

Improved FACS-Gal: flow cytometric analysis and sorting of viable eukaryotic cells expressing reporter gene constructs.

作者信息

Fiering S N, Roederer M, Nolan G P, Micklem D R, Parks D R, Herzenberg L A

机构信息

Department of Genetics, Stanford University, California.

出版信息

Cytometry. 1991;12(4):291-301. doi: 10.1002/cyto.990120402.

DOI:10.1002/cyto.990120402
PMID:1905992
Abstract

The previously reported FACS-Gal assay (Nolan et al., Proc Natl Acad Sci USA 85:2603-2607, 1988) measures E. coli lacZ-encoded beta-galactosidase activity in individual viable eukaryotic cells for a variety of molecular and cellular biological applications. Enzyme activity is measured by flow cytometry, using a fluorogenic substrate, which is hydrolyzed and retained intracellularly. In this system, lacZ serves both as a reporter gene to quantitate gene expression and as a selectable marker for the fluorescence-activated sorting of cells based on their lacZ expression level. This report details the following improvements of the original assay: 1) use of phenylethyl-beta-D-thiogalactoside, a competitive inhibitor, to inhibit beta-galactosidase activity; 2) reduction of false positives by two-color measurements; and 3) inhibition of interfering mammalian beta-galactosidases by the weak base chloroquine. We found an exponential relationship between fluorescence generated by beta-galactosidase in this assay and the intracellular concentration of beta-galactosidase molecules. Finally, we report conditions for optimal loading of the substrate (FDG) and retention of the product, fluorescein. Under these conditions, we found uniform loading of FDG in all cells of a clone in individual experiments. Together, these improvements make FACS-Gal an extremely powerful tool for investigation of gene expression in eukaryotic cells.

摘要

先前报道的FACS-Gal检测方法(Nolan等人,《美国国家科学院院刊》85:2603-2607,1988年)可在单个活真核细胞中测量大肠杆菌lacZ编码的β-半乳糖苷酶活性,用于多种分子和细胞生物学应用。酶活性通过流式细胞术测量,使用一种荧光底物,该底物被水解并保留在细胞内。在这个系统中,lacZ既作为报告基因来定量基因表达,又作为基于lacZ表达水平对细胞进行荧光激活分选的选择标记。本报告详细介绍了对原始检测方法的以下改进:1)使用竞争性抑制剂苯乙基-β-D-硫代半乳糖苷来抑制β-半乳糖苷酶活性;2)通过双色测量减少假阳性;3)用弱碱氯喹抑制干扰性的哺乳动物β-半乳糖苷酶。我们发现在该检测方法中β-半乳糖苷酶产生的荧光与β-半乳糖苷酶分子的细胞内浓度之间存在指数关系。最后,我们报告了底物(FDG)最佳加载和产物荧光素保留的条件。在这些条件下,我们发现在单个实验中克隆的所有细胞中FDG加载均匀。总之,这些改进使FACS-Gal成为研究真核细胞基因表达的极其强大的工具。

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