黄体酮对体外糖蛋白- p活性影响的研究

P. Erokhina, Y. Abalenikhina, A. Shchulkin, I. V. Chernykh, N. M. Popova, A. A. Slepnev, E. Yakusheva
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引用次数: 6

摘要

背景。糖蛋白- p (Glycoprotein-P, Pgp, АВСВ1)是一种参与药物药代动力学的转运蛋白,也参与肿瘤细胞对化疗的耐药发展。的目标。目的:研究黄体酮对体外人小肠上皮细胞模型Pgp活性的影响。材料与方法。这项工作是在Caco-2细胞上进行的。Pgp的活性是通过非索非那定在一个特殊的转运系统中的转运来评价的。采用高效液相色谱法测定非索非那定的浓度。采用EIA法测定Pgp的含量。进行了四组实验:对照细胞用不添加任何物质的干净运输介质预孵育;利福平浓度为10µmol/l预孵育3 d时对Pgp活性和合成的影响(诱导对照);孕酮浓度分别为1、10和100µmol/l,预孵育30 min后对Pgp活性的影响;孕酮浓度分别为1、10和100µmol/l,预孵育3 d时对Pgp活性和合成的影响。结果。孕酮浓度为1和10µM,与细胞孵育30分钟内,对Pgp的活性没有任何可靠的影响,但浓度为100µM时,它降低了转运蛋白的活性。Caco-2细胞与浓度分别为1、10和100µM的黄体酮孵育3天后,Pgp的活性保持不变。孕酮浓度为100µM,孵育3天内,与对照组相比,孕酮显著增加肠细胞中Pgp的合成114.3%,而在其他使用浓度(1µM和10µM)下,孕酮没有产生可靠的效果。结论。体外实验中,浓度为100µM的黄体酮对Caco-2细胞的Pgp活性有直接抑制作用;然而,在3天的孵育中,它增加了转运蛋白的合成,这抵消了它的抑制活性。
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A study of influence of progesterone on activity of Glycoprotein-P in vitro
Background . Glycoprotein-P (Pgp, АВСВ1) is a transporter protein participating in pharmacokinetics of medical drugs, and also in development of resistance of tumor cells to chemotherapy. Aim . To study the influence of progesterone on the activity of Pgp in vitro on a cell model of human small intestinal epithelium. Materials and Methods . The work was conducted on Caco-2 cells. The activity of Pgp was eva-luated by transport of fexofenadine in a special transwell-system. Concentration of fexofenadine was analyzed by HPLC method. The amount of Pgp was determined by EIA method. Four series of experiments were conducted: control – cells preincubated with clean transport medium without addition of any substances; influence of rifampicin on the activity and synthesis of Pgp in the concentration 10 µmol/l in preincubation for 3 days (induction control); influence of progesterone on the activity of Pgp in concentrations 1, 10 and 100 µmol/l in preincubation for 30 min; influence of progesterone on the activity and synthesis of Pgp in concentrations 1, 10 and 100 µmol/l in preincubation for 3 days. Results . Progesterone in the concentrations 1 and 10 µM in incubation with cells within 30 minutes did not show any reliable influence on the activity of Pgp, however, in concentration 100 µM it reduced the activity of the transporter protein. In incubation of Caco-2 cells with progesterone in concentrations 1, 10 and 100 µM within 3 days the activity of Pgp remained unchanged. Progesterone in concentration 100 µM in incubation within 3 days significantly increased synthesis of Pgp in enterocytes by 114.3% as compared to control, and in other used concentrations (1 and 10 µM) it produced no reliable effect. Conclusion . In in vitro experiments on Caco-2 cells progesterone in concentration 100 µM produces a direct inhibiting effect on the activity of Pgp; however, in incubation within 3 days it increases synthesis of the transporter protein, which cancels out its inhibitory activity.
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