首页> 外文期刊>Journal of Pharmacological and Toxicological Methods >A reporter gene assay for evaluation of tissue-specific responses to estrogens based on the differential use of promoters A to F of the human estrogen receptor alpha gene.
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A reporter gene assay for evaluation of tissue-specific responses to estrogens based on the differential use of promoters A to F of the human estrogen receptor alpha gene.

机译:基于人雌激素受体α基因启动子A至F的差异使用,用于评估对雌激素的组织特异性反应的记者基因检测。

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INTRODUCTION: Reporter gene assays are useful means for monitoring cellular responses. We report here a reporter gene assay for evaluating and monitoring estrogen activities by estrogen-like compounds and xenoestrogens, which is based on the promoters from the human estrogen receptor alpha (ERalpha) gene. METHODS: The reporter gene constructs contained a proximal promoter region (containing promoters A and B: ProAB) or either of promoters C to F (ProC, ProD, ProE, and ProF) or fused minor promoters (ProCDEF). These constructs were first used to evaluate promoter activity in cell lines derived from breast (MCF-7 and T-47D cells), ovary (SK-OV-3 cells), endometrium (Ishikawa cells), and stomach (MKN-28 cells). RESULTS: Besides very high levels of activity by ProAB in all of the cell lines tested, moderate levels were detected for ProD in the breast and endometrium cell lines and for ProF in the ovary and endometrium cell lines. A moderate level of activity by ProE was detected only in the stomach cells. Differences in estrogen-like activity between ProAB and ProD were observed for tamoxifen and bisphenol A (BPA) in MCF-7 cells. DISCUSSION: The assay proposed here might provide expression profiles of cancer cells of various origins for evaluating the estrogen responsiveness and for identifying tissue- or cancer cell-specific transcription factors.
机译:简介:报告基因检测是监测细胞反应的有用手段。我们在这里报告一种记者基因检测方法,用于评估和监测雌激素样化合物和异种雌激素的雌激素活性,这是基于人类雌激素受体α(ERalpha)基因的启动子。方法:报告基因构建体包含一个近端启动子区域(包含启动子A和B:ProAB)或启动子C至F(ProC,ProD,ProE和ProF)或融合的次要启动子(ProCDEF)。这些构建体首先用于评估源自乳腺(MCF-7和T-47D细胞),卵巢(SK-OV-3细胞),子宫内膜(石川细胞)和胃(MKN-28细胞)的细胞系中的启动子活性。 。结果:除了在所有测试的细胞系中ProAB的活性很高外,在乳腺癌和子宫内膜细胞系中的ProD以及在卵巢和子宫内膜细胞系中的ProF均检测到中等水平。 ProE仅在胃细胞中检测到中等水平的活性。对于他莫昔芬和双酚A(BPA),在MCF-7细胞中观察到ProAB和ProD之间的雌激素样活性不同。讨论:此处提出的测定法可能会提供各种来源的癌细胞的表达谱,以评估雌激素的反应性并鉴定组织或癌细胞特异性的转录因子。

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