Li A P, Jurima-Romet M
In Vitro Technologies, Inc., Baltimore, Maryland, USA.
Cell Biol Toxicol. 1997 Jul;13(4-5):365-74. doi: 10.1023/a:1007451911843.
The utility of primary human hepatocytes in the evaluation of drug-drug interactions is being investigated in our laboratories. Our initial approach was to investigate whether drug-drug interactions observed in humans in vivo could be reproduced in vitro using human hepatocytes. Two model drugs were studied: terfenadine and rifampin, representing compounds subjected to drug-drug interactions via inhibitory and induction mechanisms, respectively. Terfenadine was found to be metabolized by human hepatocytes to C-oxidation and N-dealkylation products as observed in humans in vivo. Metabolism by human hepatocytes was found to be inhibited by drugs which are known to be inhibitory in vivo. Ki values for the various inhibitors were derived from the in vitro metabolism data, resulting in the following ranking of inhibitory potency: For the inhibition of C-oxidation, ketoconazole > itraconazole > cyclosporin approximately troleandomycin > erythromycin > naringenin. For the inhibition of N-dealkylation, itraconazole > or = ketoconazole > cyclosporin > or = naringenin > or = erythromycin > or = troleandomycin. Rifampin induction of CYP3A, a known effect of rifampin in vivo, was also reproduced in primary human hepatocytes. Induction of CYP3A4, measured as testosterone 6 beta-hydroxylation, was found to be dose-dependent, treatment duration-dependent, and reversible. The induction effect of rifampin was observed in hepatocytes isolated from all 7 human donors studied, with ages ranging from 1.7 to 78 years. To demonstrate that the rifampin-induction of testosterone 6 beta-hydroxylation could be generalized to other CYP3A4 substrates, we evaluated the metabolism of another known substrate of CYP3A4, lidocaine. Dose-dependent induction of lidocaine metabolism by rifampin is observed. Our results suggest that primary human hepatocytes may be a useful experimental system for preclinical evaluation of drug-drug interaction potential during drug development, and as a tool to evaluate the mechanism of clinically observed drug-drug interactions.
我们实验室正在研究原代人肝细胞在药物相互作用评估中的效用。我们最初的方法是研究在人体中观察到的药物相互作用是否可以在体外用人肝细胞重现。研究了两种模型药物:特非那定和利福平,分别代表通过抑制和诱导机制发生药物相互作用的化合物。发现特非那定在人肝细胞中代谢为C-氧化和N-脱烷基产物,这与在人体中观察到的情况一致。已知在体内具有抑制作用的药物会抑制人肝细胞的代谢。各种抑制剂的Ki值来自体外代谢数据,得出以下抑制效力排名:对于C-氧化的抑制,酮康唑>伊曲康唑>环孢素≈三乙酰竹桃霉素>红霉素>柚皮苷。对于N-脱烷基的抑制,伊曲康唑≥酮康唑>环孢素≥柚皮苷≥红霉素≥三乙酰竹桃霉素。利福平对CYP3A的诱导作用,这是利福平在体内的已知作用,在原代人肝细胞中也得到了重现。以睾酮6β-羟化来衡量,CYP3A4的诱导呈剂量依赖性、治疗持续时间依赖性且可逆。在研究的所有7名年龄从1.7岁到78岁的人类供体分离的肝细胞中均观察到利福平的诱导作用。为了证明利福平对睾酮6β-羟化的诱导作用可以推广到其他CYP3A4底物,我们评估了另一种已知的CYP3A4底物利多卡因的代谢。观察到利福平对利多卡因代谢的剂量依赖性诱导作用。我们的结果表明,原代人肝细胞可能是药物开发过程中临床前评估药物相互作用潜力的有用实验系统,并且作为评估临床观察到的药物相互作用机制的工具。
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