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Keratinocyte serum-free medium maintains long-term liver gene expression and function in cultured rat hepatocytes by preventing the loss of liver-enriched transcription factors

机译:角质形成细胞无血清培养基可防止肝富集的转录因子的丢失,从而在培养的大鼠肝细胞中长期维持肝脏基因的表达和功能

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摘要

Freshly isolated hepatocytes rapidly lose their differentiated properties when placed in culture. Therefore, production of a simple culture system for maintaining the phenotype of hepatocytes in culture would greatly facilitate their study. Our aim was to identify conditions that could maintain the differentiated properties of hepatocytes for up to 28 days of culture. Adult rat hepatocytes were isolated and attached in Williams’ medium E containing 10% serum. The medium was changed to either fresh Williams’ medium E or keratinocyte serum-free medium supplemented with dexamethasone, epidermal growth factor and pituitary gland extract. The hepatic phenotype was then analysed using RT-PCR, immunohistochemistry, Western blotting and assays of liver function. Cells cultured in keratinocyte serum-free medium supplemented with dexamethasone, epidermal growth factor and pituitary gland extract maintained their phenotype for 3–4 weeks, based on expression of liver proteins, ureagensis and response to xenobiotics. In contrast, hepatocytes cultured in Williams’ medium E rapidly lost the expression of liver proteins after 3 days. Cells cultured in keratinocyte serum-free medium supplemented with dexamethasone, epidermal growth factor and pituitary gland extract maintained their expression of liver-enriched transcription factors (C/EBPα and β, HNF4α and RXRα) while expression was either lost or reduced in cells cultured in Williams’ medium E. These results suggest that keratinocyte serum-free medium supplemented with dexamethasone, epidermal growth factor and pituitary gland extract can maintain the hepatic phenotype for a prolonged period and that this is probably related to the continued expression of the liver-enriched transcription factors.
机译:新鲜分离的肝细胞在培养时会迅速失去其分化特性。因此,生产用于维持培养中肝细胞表型的简单培养系统将极大地促进其研究。我们的目标是确定可以在长达28天的培养中维持肝细胞分化特性的条件。分离成年大鼠肝细胞并将其附着在含有10%血清的Williams培养基E中。将培养基改为新鲜的Williams培养基E或补充了地塞米松,表皮生长因子和垂体提取物的无角质形成细胞血清培养基。然后使用RT-PCR,免疫组织化学,Western印迹和肝功能测定分析肝表型。在补充了地塞米松,表皮生长因子和垂体提取物的无角质形成细胞的无血清培养基中培养的细胞,根据肝脏蛋白,尿素的表达和对异种生物的反应,保持其表型3-4周。相反,在威廉姆斯培养基E中培养的肝细胞在3天后迅速丧失了肝蛋白的表达。在补充了地塞米松,表皮生长因子和垂体提取物的无角质形成细胞的无血清培养基中培养的细胞保持了肝脏富集的转录因子(C /EBPα和β,HNF4α和RXRα)的表达,而在培养的细胞中表达则丢失或减少。 Williams培养基E。这些结果表明,补充了地塞米松,表皮生长因子和垂体提取物的无角质形成细胞血清培养基可以长期维持肝表型,这可能与富肝转录的持续表达有关。因素。

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