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EF5[2-(2-硝基-1H-咪唑-1-基)-N-(2,2,3,3,3-五氟丙基)乙酰胺]细胞摄取的氧依赖性:通过荧光抗体与结合放射性分析药物加合物。

Oxygen dependence of cellular uptake of EF5 [2-(2-nitro-1H-imidazol-1-yl)-N-(2,2,3,3,3-pentafluoropropyl)a cet amide] : analysis of drug adducts by fluorescent antibodies vs bound radioactivity.

作者信息

Koch C J, Evans S M, Lord E M

机构信息

University of Pennsylvania, Philadelphia 19104-6072, USA.

出版信息

Br J Cancer. 1995 Oct;72(4):869-74. doi: 10.1038/bjc.1995.426.

Abstract

The present studies were initiated to quantitate the oxygen dependence of bioreductive metabolism-induced binding of EF5, a pentafluorinated derivative of the 2-nitroimidazole, etanidazole. Two different assays were compared: first, radioactive drug incorporation into cell lysates, which provides a direct measure of drug metabolism or uptake; second, monoclonal antibody detection of cellular macromolecular adducts of EF5 after whole cell permeabilisation and fixing. The antibodies (a single clone designated ELK3-51) were conjugated with the fluorescent dye Cy3, with fluorescence determined by fluorescence microscopy and flow cytometry. For the two cell lines tested (V79 Chinese hamster fibroblasts and 9L rat glioma), the oxygen dependence of binding was found to be the same for the two techniques. Using the antibody binding technique, the fluorescence signal was highly reproducible between experiments, resistant to light or chemical bleaching and stable over time following cell or tissue staining. Flow cytometric analysis of cells from rat 9L tumours treated with EF5 in vivo or in vitro showed a distribution of fluorescent signal which was very compatible, on both a relative and absolute basis, with the in vitro results. Our results indicate that immunofluorescent techniques provide a quantitative assay for bioreductive drug adducts, and therefore may be able to measure the absolute oxygen concentration distribution in cell populations and tissues of interest.

摘要

开展本研究是为了对生物还原代谢诱导的2-硝基咪唑类五氟衍生物依他硝唑(etanidazole)的EF5结合的氧依赖性进行定量分析。比较了两种不同的检测方法:第一种是将放射性药物掺入细胞裂解物中,这可直接测量药物代谢或摄取情况;第二种是在全细胞通透化和固定后,通过单克隆抗体检测EF5的细胞大分子加合物。抗体(指定克隆ELK3 - 51)与荧光染料Cy3偶联,通过荧光显微镜和流式细胞术测定荧光。对于所测试的两种细胞系(V79中国仓鼠成纤维细胞和9L大鼠胶质瘤细胞),发现两种技术检测到的结合的氧依赖性相同。使用抗体结合技术,实验之间荧光信号具有高度可重复性,抗光或化学漂白,并且在细胞或组织染色后随时间保持稳定。对体内或体外经EF5处理的大鼠9L肿瘤细胞进行流式细胞术分析,结果显示荧光信号分布在相对和绝对水平上都与体外结果非常相符。我们的结果表明,免疫荧光技术可为生物还原药物加合物提供定量检测方法,因此可能能够测量感兴趣的细胞群体和组织中的绝对氧浓度分布。

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