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P-糖蛋白在人肠道Caco-2细胞顶膜中的功能表达。长春碱分泌动力学及其与调节剂的相互作用。

Functional expression of P-glycoprotein in apical membranes of human intestinal Caco-2 cells. Kinetics of vinblastine secretion and interaction with modulators.

作者信息

Hunter J, Jepson M A, Tsuruo T, Simmons N L, Hirst B H

机构信息

Gastrointestinal Drug Delivery Research Centre, University of Newcastle upon Tyne, Medical School, United Kingdom.

出版信息

J Biol Chem. 1993 Jul 15;268(20):14991-7.

PMID:8100817
Abstract

The functional expression of P-glycoprotein has been studied in confluent epithelial layers of human Caco-2 cells, a polarized, highly differentiated cell line demonstrating an intestinal absorptive cell phenotype. Expression of P-glycoprotein was localized, by indirect immunofluorescence with monoclonal antibody MRK16, to the apical brush-border, approximately 20 microns above the base of the cells. Functional, high capacity expression of P-glycoprotein in Caco-2 cell layers was demonstrated by the saturable secretion of vinblastine, a typical substrate, from basolateral to apical surfaces: Km 18.99 +/- 5.55 microM, Vmax 1285.9 +/- 281.2 pmol.cm-2 h-1. The direct correlation of apical P-glycoprotein expression with vinblastine net secretory flux was demonstrated by the reduction of this flux after treatment with MRK16 antibodies. Vinblastine secretory flux was also reduced by treatment with verapamil (R- and S-isomers with equal affinity), nifedipine, taxotere, and 1,9-dideoxyforskolin. Kinetic analyses suggest that the inhibition of vinblastine secretory flux by verapamil and nifedipine was competitive, while that by dideoxyforskolin was non-competitive, in nature. The polarized expression and activity of P-glycoprotein in Caco-2 cells is direct evidence for its secretory detoxifying function in the intestine, subserving at least one role of the gastrointestinal epithelial barrier.

摘要

已在人Caco-2细胞的汇合上皮层中研究了P-糖蛋白的功能表达,Caco-2细胞是一种极化的、高度分化的细胞系,表现出肠吸收细胞表型。用单克隆抗体MRK16进行间接免疫荧光定位显示,P-糖蛋白表达定位于细胞基部上方约20微米处的顶端刷状缘。通过典型底物长春碱从基底外侧向顶端表面的饱和分泌,证明了Caco-2细胞层中P-糖蛋白具有功能性高容量表达:米氏常数(Km)为18.99±5.55微摩尔,最大反应速度(Vmax)为1285.9±281.2皮摩尔·厘米-2·小时-1。用MRK16抗体处理后,顶端P-糖蛋白表达与长春碱净分泌通量的直接相关性得以证明,该通量降低。用维拉帕米(R-和S-异构体具有同等亲和力)、硝苯地平、多西他赛和1,9-二脱氧佛司可林处理也可降低长春碱分泌通量。动力学分析表明,维拉帕米和硝苯地平对长春碱分泌通量的抑制本质上是竞争性的,而二脱氧佛司可林的抑制是非竞争性的。Caco-2细胞中P-糖蛋白的极化表达和活性直接证明了其在肠道中的分泌解毒功能,这至少是胃肠道上皮屏障的一种作用。

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