在 rSlco2b1 基因敲除和 SLCO2B1 基因敲除大鼠体内研究 OATP2B1 对阿托伐他汀药代动力学的影响。

IF 4.4 3区 医学 Q1 PHARMACOLOGY & PHARMACY Drug Metabolism and Disposition Pub Date : 2024-08-14 DOI:10.1124/dmd.124.001686
Jonny Kinzi, Janine Hussner, Isabell Seibert, Mirubagini Vythilingam, Celina Vonwyl, Clarisse Gherardi, Pascal Detampel, Oliver Schwardt, Daniel Ricklin, Henriette E Meyer Zu Schwabedissen
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引用次数: 0

摘要

有机阴离子转运多肽(OATP)2B1 被认为是一种新兴的药物转运体,在肝脏、小肠和肾脏等药物动力学相关器官中均有表达。尽管它与多种底物药物存在相互作用,但人们对其体内相关性的了解仍然有限。在本研究中,我们首先利用瞬时转染的 HeLa 细胞验证了阿托伐他汀与大鼠 OATP2B1 的相互作用。此外,我们还鉴定了 rSlco2b1 基因敲除大鼠和 SLCO2B1 基因敲除大鼠的 mRNA、蛋白质表达以及 OATP2B1 在肝脏、小肠和肾脏的定位。该转运体在肝脏的表达量最高,其次是小肠。在人源化大鼠中,人 OATP2B1 定位于肝细胞的窦状膜上。在野生型大鼠和人源化大鼠的肠细胞中,转运体在管腔膜上被检测到,绝大多数位于顶端下。随后,我们评估了雄性野生型大鼠、R Slco2b1 基因敲除大鼠和 SLCO2B1 基因敲除大鼠单剂量给药(口服和静脉注射)后阿托伐他汀的药代动力学。研究大鼠 OATP2B1 或人类 OATP2B1 对口服阿托伐他汀药代动力学的影响发现,两者的浓度-时间曲线和药代动力学参数均无差异。然而,在比较人源化 SLCO2B1 大鼠和基因敲除动物静脉注射阿托伐他汀后的药代动力学时,观察到了明显的差异。特别是,人源化动物的全身暴露量(AUC)降低了约 40%,而表达人 OATP2B1 的动物的清除率(CL)则高出 57%。这些研究结果表明,人源 OATP2B1 会影响阿托伐他汀静脉注射后的药代动力学,很可能是通过促进肝脏摄取来实现的。意义声明 野生型、rSlco2b1-剔除型和 SLCO2B1-人源化 Wistar 大鼠是大鼠和人 SLCO2B1/OATP2B1 的表达特征。在雄性野生型大鼠、rSlco2b1-基因敲除大鼠和 SLCO2B1-人源化大鼠中进行了阿托伐他汀 24 小时的药代动力学研究。单剂量静脉注射后,与基因敲除动物相比,SLCO2B1-人源化大鼠的全身暴露量更低,清除率更高,这表明 OATP2B1 对肝脏清除率有贡献。
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Impact of OATP2B1 on Pharmacokinetics of Atorvastatin Investigated in rSlco2b1-Knockout and SLCO2B1-Knockin Rats.

The organic anion transporting polypeptide (OATP) 2B1 is considered an emerging drug transporter that is found expressed in pharmacokinetically relevant organs such as the liver, small intestine, and kidney. Despite its interaction with various substrate drugs, the understanding of its in vivo relevance is still limited. In this study, we first validated the interaction of atorvastatin with rat OATP2B1 using transiently transfected HeLa cells. Moreover, we characterized our rSlco2b1-knockout and SLCO2B1-knockin rats for mRNA, protein expression, and localization of OATP2B1 in the liver, small intestine, and kidney. The transporter showed the highest expression in the liver followed by the small intestine. In humanized rats, human OATP2B1 is localized on the sinusoidal membrane of hepatocytes. In enterocytes of wild-type and humanized rats, the transporter was detected in the luminal membrane with the vast majority being localized subapical. Subsequently, we assessed atorvastatin pharmacokinetics in male wild-type, rSlco2b1-knockout, and SLCO2B1-knockin rats after a single-dose administration (orally and intravenously). Investigating the contribution of rat OATP2B1 or human OATP2B1 to oral atorvastatin pharmacokinetics revealed no differences in concentration-time profiles or pharmacokinetic parameters. However, when comparing the pharmacokinetics of atorvastatin after intravenous administration in SLCO2B1-humanized rats and knockout animals, notable differences were observed. In particular, the systemic exposure (area under the curve) decreased by approximately 40% in humanized animals, whereas the clearance was 57% higher in animals expressing human OATP2B1. These findings indicate that human OATP2B1 influences pharmacokinetics of atorvastatin after intravenous administration, most likely by contributing to the hepatic uptake. SIGNIFICANCE STATEMENT: Wild-type, rSlco2b1-knockout, and SLCO2B1-humanized Wistar rats were characterized for the expression of rat and human SLCO2B1/OATP2B1. Pharmacokinetic studies of atorvastatin over 24 hours were conducted in male wild-type, rSlco2b1-knockout, and SLCO2B1-humanized rats. After a single-dose intravenous administration, a lower systemic exposure and an increase in clearance were observed in SLCO2B1-humanized rats compared with knockout animals indicating a contribution of OATP2B1 to the hepatic clearance.

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期刊介绍: An important reference for all pharmacology and toxicology departments, DMD is also a valuable resource for medicinal chemists involved in drug design and biochemists with an interest in drug metabolism, expression of drug metabolizing enzymes, and regulation of drug metabolizing enzyme gene expression. Articles provide experimental results from in vitro and in vivo systems that bring you significant and original information on metabolism and disposition of endogenous and exogenous compounds, including pharmacologic agents and environmental chemicals.
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