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首页> 外文期刊>Journal of medicinal food >Transwell-grown HepG2 cell monolayers as in vitro permeability model to study drug-drug or drug-food interactions.
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Transwell-grown HepG2 cell monolayers as in vitro permeability model to study drug-drug or drug-food interactions.

机译:Transwell生长的HepG2细胞单层作为体外渗透性模型,用于研究药物-药物或药物-食物的相互作用。

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HepG2 cell monolayers, formed during cell growth on collagen-coated Transwell(R) (Corning(R) Inc., Corning, NY, USA) inserts, can be used for the evaluation of interactions between food supplements and drugs that are substrates for P-glycoprotein (Pgp) and/or multidrug resistance-associated protein 2 (MRP-2). Samples obtained during such permeability studies were relatively free of intracellular proteins or cell debris compared to usually performed uptake experiments with HepG2 cells; therefore no special preparation protocol prior to the analysis was needed. In the presence of aged garlic extract the activities of hepatic efflux transporters (Pgp, MRP-2) changed, which was observed as significant permeability changes of tested human immunodeficiency virus (HIV) protease inhibitors. Darunavir efflux significantly increased, whereas that of saquinavir significantly decreased. Because of the observed in vitro interactions between aged garlic extract and HIV protease inhibitors (darunavir, saquinavir), any alterations of in vivo liver transport in the presence of garlic phytochemicals could also significantly influence darunavir/saquinavir hepatocyte intracellular concentrations and hence their bioavailabilities. Therefore this aspect needs further in vivo animal evaluation.
机译:HepG2细胞单层形成于细胞生长过程中,该细胞在胶原蛋白涂层的Transwell(R)(Corning®,Inc.,Corning,NY,USA)插入物上形成,可用于评估食品补充剂与作为P底物的药物之间的相互作用-糖蛋白(Pgp)和/或多药耐药相关蛋白2(MRP-2)。与通常使用HepG2细胞进行的摄取实验相比,在此类渗透性研究中获得的样品相对不含细胞内蛋白质或细胞碎片。因此,在分析之前不需要特殊的制备方案。在存在老化大蒜提取物的情况下,肝外排转运蛋白(Pgp,MRP-2)的活性发生了变化,这被观察为测试的人类免疫缺陷病毒(HIV)蛋白酶抑制剂的通透性显着变化。 Darunavir外排显着增加,而沙奎那韦则明显减少。由于观察到了老年大蒜提取物和HIV蛋白酶抑制剂(darunavir,saquinavir)之间的体外相互作用,因此在存在大蒜植物化学物质的情况下体内肝脏运输的任何变化也可能显着影响darunavir / saquinavir肝细胞的细胞内浓度并因此影响其生物利用度。因此,这方面需要进一步的体内动物评估。

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