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Primary cultures of human hepatocytes but not HepG2 hepatoblastoma cells are suitable for the study of glycosidic conjugation of bile acids

机译:人肝细胞的原代培养物而不是HepG2肝母细胞瘤细胞的原代培养物适合于胆汁酸的糖苷结合研究

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摘要

To define the role of glycosidic conjugation of bile acids in humans, an in vitro model system is desirable. We studied the formation of glycosidic conjugates of bile acids in primary cultures of human hepatocytes, isolated from organ donor liver, and the human hepatoblastoma cell line, HepG2. Cells were incubated with 100 μM bile acids (chenodeoxycholic, CDCA; hyodeoxycholic, HDCA; and isoursodeoxycholic acids, isoUDCA) and 1-2 mM uridine diphosphoglycosides (UDP-glucose, UDP-Glc., UDP-glucuronic acid, UDP-GlcA, and UDP-N-acetylglucosamine, UDP-GlcNAc), and octyl glucoside. Media were analysed by electrospray-/gas chromatography-mass spectrometry and electrospray with collision induced dissociation. Primary cultures of human hepatocytes formed glycosidic bile acid conjugates with UDP-sugars (6α-Glc-HDCA, 6α-GlcA-HDCA, and 7β-GlcNAc-isoUDCA) and octyl glucoside as sugar donors (3α-Glc-CDCA). HDCA was completely metabolised to either Glc-HDCA, a compound yet not found in vivo, or GlcA-HDCA. No glycosidic bile acid conjugate was found in media from experiments with HepG2. Thus, primary cultures of human hepatocytes, but not HepG2, are suitable in vitro systems for the study of glycosidic bile acid conjugation reactions.
机译:为了定义胆汁酸在人体内的糖苷结合作用,需要体外模型系统。我们研究了从器官供体肝脏和人肝母细胞瘤细胞系HepG2中分离出来的人肝细胞原代培养物中胆汁酸的糖苷结合物的形成。将细胞与100μM胆汁酸(chenodeoxycholic,CDCA; hyodeoxycholic,HDCA; and isoursodeoxycholic acid,isoUDCA)和1-2 mM尿苷二磷酸糖苷(UDP-葡萄糖,UDP-Glc。,UDP-葡萄糖醛酸,UDP-GlcA和UDP-N-乙酰氨基葡萄糖,UDP-GlcNAc)和辛基葡萄糖苷。通过电喷雾/气相色谱-质谱法分析培养基,并通过碰撞诱导解离进行电喷雾。人肝细胞的原代培养物与UDP糖(6α-Glc-HDCA,6α-GlcA-HDCA和7β-GlcNAc-isoUDCA)和辛基葡糖苷作为糖供体(3α-Glc-CDCA)形成了糖苷胆酸共轭物。 HDCA完全代谢为体内尚未发现的Glc-HDCA或GlcA-HDCA。在用HepG2进行的实验培养基中未发现糖苷胆酸结合物。因此,人肝细胞的原代培养物,而不是HepG2,是适合于糖苷胆汁酸结合反应研究的体外系统。

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