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The Contribution of 17beta-Hydroxysteroid Dehydrogenase Type 1 to the Estradiol-Estrone Ratio in Estrogen-Sensitive Breast Cancer Cells

机译:雌激素敏感性乳腺癌细胞中17β-羟基类固醇脱氢酶1型对雌二醇-雌激素比的贡献。

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摘要

Estrone and estradiol are both estrogens with estrone being the less potent form and estradiol being the most potent estrogen. The binding of the latter to cellular regulatory elements stimulates the proliferation of breast cancer cells. A high ratio of estradiol/estrone is related to increased cell proliferation, and is of great importance to understanding of breast cancer mechanisms. 17beta-hydroxysteroid dehydrogenase type 1 and type 2 play important roles in the activation of estrone and inactivation of estradiol. Breast cancer cells T47D, MCF-7, BT 20, and JEG 3 as control cells, were chosen to evaluate the contribution of these two enzymes to the ratio. Twenty four hours after addition of different concentrations of estrone and estradiol, the ratio stabilized to around 9/1 in breast cancer cell lines with high expression of type 1 (T47D, BT 20, and JEG 3), whereas it approached 1/5 in cells with low expression of type 1 (MCF-7). The estradiol/estrone concentration ratio was modified to 9/1 in MCF-7 and HEK-293 cells over-expressing type 1. In T47D and BT 20, this ratio was decreased from 9/1 to nearly 1/5 (19/81 and 17/83 respectively) after type 1 knockdown by specific siRNAs. Type 2 is mainly involved in the conversion of estradiol into estrone. This ratio was decreased from 9/1 to 7/3 after over-expression of type 2 in MCF-7 cells already over-expressing type 1. The ratio was further decreased by the addition of the oxidative cofactor, NAD, to the cell culture to facilitate the estradiol to estrone conversion catalyzed by type 2. These results demonstrate that the estradiol/estrone ratio is controlled by both type 1 and type 2 with an additional contribution by NAD, although type 1 is the first determining factor in the cellular environment compared with type 2 and cofactors. Moreover, kinetic studies were carried out in intact cells as a new approach, using HEK-293 cells over-expressing type 1 and T47D breast cancer cells.
机译:雌酮和雌二醇都是雌激素,雌酮是效力较低的形式,雌二醇是最有效的雌激素。后者与细胞调节元件的结合刺激乳腺癌细胞的增殖。雌二醇/雌酮的高比例与细胞增殖的增加有关,并且对了解乳腺癌的机制非常重要。 17β-羟基类固醇脱氢酶1型和2型在雌酮的活化和雌二醇的失活中起重要作用。选择乳腺癌细胞T47D,MCF-7,BT 20和JEG 3作为对照细胞,以评估这两种酶对该比例的贡献。在添加不同浓度的雌酮和雌二醇后二十四小时,在具有高表达1型(T47D,BT 20和JEG 3)的乳腺癌细胞系中,该比率稳定在9/1左右,而在1型细胞中接近1/5。 1型低表达细胞(MCF-7)。在过度表达1型的MCF-7和HEK-293细胞中,雌二醇/雌酮的浓度比例已修改为9/1。在T47D和BT 20中,该比例从9/1降低至近1/5(19/81和17/83)分别通过特异性siRNA敲低1型。 2型主要涉及雌二醇向雌酮的转化。在已经过表达1型的MCF-7细胞中过表达2型后,该比例从9/1降低到7/3。通过向细胞培养物中添加氧化辅因子NAD,该比例进一步降低。促进由类型2催化的雌二醇向雌酮的转化。这些结果表明,雌二醇/雌酮比例受类型1和类型2的控制,而NAD的贡献更大,尽管类型1是比较细胞环境中的第一个决定性因素与2型和辅助因子。此外,使用完整表达1型HEK-293细胞和T47D乳腺癌细胞的新方法,在完整细胞中进行了动力学研究。

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