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FEK 自组装肽水凝胶促进原代肝细胞培养和药代动力学筛选。

FEK self-assembled peptide hydrogels facilitate primary hepatocytes culture and pharmacokinetics screening.

机构信息

School of Pharmaceutical Sciences, Nanjing Tech University, Nanjing, China.

Shanghai Institute of Materia Medica, Chinese Academy of Sciences, Shanghai, China.

出版信息

J Biomed Mater Res B Appl Biomater. 2022 Sep;110(9):2015-2027. doi: 10.1002/jbm.b.35056. Epub 2022 Mar 18.

DOI:10.1002/jbm.b.35056
PMID:35301798
Abstract

A FEFEFKFK (FEK, F, phenylalaninyl; E, glutamyl; K, lysinyl)-based self-assembling peptide hydrogel (FEK-SAPH) was developed to replace sandwich culture (SC) for improved culture of primary hepatocytes in vitro. Under neutral conditions, FEK self-assembles to form β-sheet nanofibers, which in turn form FEK-SAPH. For the culture of rat primary hepatocytes (RPH), the use of FEK-SAPH simplified operation steps and promoted excellent cell-cell interactions while maintaining the SC-related RPH polarity trend. Compared with SC, FEK-SAPH cultured RPH for 14 days, the bile duct network was formed, the secretion of albumin and urea was improved, and the metabolic clearance rate based on cytochrome P450 (CYPs) was comparable. In FEK-SAPH culture, the expression level of the biliary efflux transporter bile salt export pump increased by 230.7%, while the biliary excretion index value of deuterium-labeled sodium taurocholate (d8-TCA) differed slightly from the SC value (72% and 77%, respectively, p = .0195). The inhibitory effect of cholestasis drugs on FEK-SAPH was significantly higher than that of SC. In FEK-SAPH, hepatoprotective drugs were more effective in antagonizing hepatotoxicity induced by lithocholic acid (LCA). FEK-SAPH cultured RPH with hepatoprotective drugs can better recover from LCA-induced damage. In summary, FEK-SAPH can be used as a substitute for SC for pharmacokinetic screening to evaluate the drug absorption, disposition, metabolism, excretion, and toxicity (ADMET) in hepatocytes.

摘要

一种基于 FEFEFKFK(FEK、F、苯丙氨酸;E、谷氨酸;K、赖氨酸)的自组装肽水凝胶(FEK-SAPH)被开发出来,以替代三明治培养(SC),从而提高原代肝细胞的体外培养效果。在中性条件下,FEK 自组装形成β-折叠纳米纤维,进而形成 FEK-SAPH。对于大鼠原代肝细胞(RPH)的培养,FEK-SAPH 的使用简化了操作步骤,促进了优异的细胞间相互作用,同时保持了与 SC 相关的 RPH 极性趋势。与 SC 相比,FEK-SAPH 培养的 RPH 可在 14 天内形成胆管网络,提高白蛋白和尿素的分泌,并具有可比较的基于细胞色素 P450(CYPs)的代谢清除率。在 FEK-SAPH 培养中,胆汁流出转运体胆盐输出泵的表达水平增加了 230.7%,而氘标记的牛磺胆酸钠(d8-TCA)的胆汁排泄指数值与 SC 值略有不同(分别为 72%和 77%,p=0.0195)。在 FEK-SAPH 中,胆汁淤积药物对其的抑制作用明显高于 SC。在 FEK-SAPH 中,保肝药物在拮抗石胆酸(LCA)诱导的肝毒性方面更有效。用保肝药物培养的 FEK-SAPH 能更好地从 LCA 诱导的损伤中恢复。总之,FEK-SAPH 可替代 SC 用于药代动力学筛选,以评估肝细胞的药物吸收、分布、代谢、排泄和毒性(ADMET)。

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