de Campos Nebel Marcelo, Palmitelli Micaela, González-Cid Marcela
Laboratorio de Mutagénesis, Instituto de Medicina Experimental (IMEX), Academia Nacional de Medicina, CONICET. Ciudad Autónoma de Buenos Aires, Argentina.
Curr Protoc Cytom. 2017 Jul 5;81:7.48.1-7.48.8. doi: 10.1002/cpcy.21.
The poisoning of Topoisomerase II (Top2) has been found to be useful as a therapeutic strategy for the treatment of several tumors. The mechanism of Top2 poisons involves a drug-mediated stabilization of a Top2-DNA complex, termed Top2 cleavage complex (Top2cc), which maintains a 5' end of DNA covalently bound to a tyrosine from Top2 through a phosphodiester group. Drug-stabilized Top2cc leads to Top2-linked-DNA breaks, which are believed to mediate their cytotoxicity. Several time-consuming or cell type-limiting assays have been used in the past to study drug-stabilized Top2cc. Here, we describe a flow cytometry-based method that allows a rapid assessment of drug-induced Top2cc, which is suitable for high throughput analysis in almost any kind of human cell. The analyses of the drug-induced Top2cc in the cell cycle context and the possibility to track its removal are additional benefits from this methodology. © 2017 by John Wiley & Sons, Inc.
拓扑异构酶II(Top2)中毒已被证明是治疗多种肿瘤的一种有效治疗策略。Top2中毒机制涉及药物介导的拓扑异构酶II-DNA复合物(称为Top2切割复合物,Top2cc)的稳定,该复合物使DNA的5'末端通过磷酸二酯基团与Top2的酪氨酸共价结合。药物稳定的Top2cc会导致与Top2相关的DNA断裂,据信这介导了它们的细胞毒性。过去曾使用几种耗时或受细胞类型限制的试验来研究药物稳定的Top2cc。在此,我们描述了一种基于流式细胞术的方法,该方法可快速评估药物诱导的Top2cc,适用于几乎任何类型人类细胞的高通量分析。在细胞周期背景下分析药物诱导的Top2cc以及追踪其清除的可能性是该方法的额外优势。© 2017约翰威立父子公司版权所有
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