首页> 外文期刊>Mutation Research: International Journal on Mutagenesis, Chromosome Breakage and Related Subjects >Quantification of CD59- mutants in human-hamster hybrid (A(L)) cells by flow cytometry.
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Quantification of CD59- mutants in human-hamster hybrid (A(L)) cells by flow cytometry.

机译:通过流式细胞仪对人-仓鼠杂种(A(L))细胞中的CD59突变体进行定量。

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摘要

Mutation assay is an important approach in evaluating the genotoxic risk of potentially harmful environmental chemicals. The human-hamster hybrid (A(L)) cell mutagenesis system, based on the complement/antibody-mediated cytotoxicity principle, has been used successfully to evaluate the mutagenic potential of a variety of environmental toxicants. The A(L) cells contain a standard set of CHO chromosomes and a single human chromosome 11, which expresses several cell surface proteins including CD59 encoded by the CD59 gene at 11p13.5. A modified mutation assay by flow cytometry was developed to determine the yield of CD59- mutants after either radiation or chemical treatment. After incubation with phycoerythrin-conjugated mouse monoclonal anti-CD59 antibody, the CD59- mutant yields were determined by quantifying the fluorescence of the cells using flow cytometry. This method is faster and eliminates the commonly encountered toxicity problems of the complements with the traditional complement/antibody assay. By comparing the mutant fractions of radiation or chemically treated A(L) cultures using the two methods, we show here that the flow cytometry assay is an excellent substitute in providing an efficient and highly sensitive method in mutant detection for the traditional complement/antibody assay.
机译:突变测定法是评估潜在有害环境化学品的遗传毒性风险的重要方法。基于补体/抗体介导的细胞毒性原理的人-仓鼠杂种(A(L))细胞诱变系统已成功用于评估多种环境毒物的诱变潜力。 A(L)细胞包含一组标准的CHO染色体和一条人类染色体11,该染色体表达11p13.5处的几种细胞表面蛋白,包括CD59基因编码的CD59。开发了通过流式细胞术的改进的突变测定法,以确定放射或化学处理后CD59-突变体的产量。与藻红蛋白缀合的小鼠单克隆抗CD59抗体孵育后,通过使用流式细胞仪定量细胞的荧光来确定CD59突变体的产量。该方法更快,并且消除了传统补体/抗体测定法中补体常见的毒性问题。通过比较使用两种方法的放射线或化学处理过的A(L)培养物的突变级分,我们在这里表明,流式细胞术检测是一种出色的替代品,可为传统补体/抗体检测提供有效且高度灵敏的突变检测方法。

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