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细胞培养条件对原代大鼠肝细胞的影响——细胞形态和差异基因表达

Effects of cell culture conditions on primary rat hepatocytes-cell morphology and differential gene expression.

作者信息

Tuschl Gregor, Mueller Stefan O

机构信息

Institute of Toxicology, Molecular Toxicology, Merck KGaA, 64271 Darmstadt, Germany.

出版信息

Toxicology. 2006 Feb 1;218(2-3):205-15. doi: 10.1016/j.tox.2005.10.017. Epub 2005 Dec 6.

Abstract

We incubated primary rat hepatocytes on collagen monolayer as well as in collagen sandwich cultures with serum-containing or serum-free medium formulations. Morphological monitoring of hepatocytes revealed that hepatocytes cultured on collagen monolayer adopted their polygonal shape and started to create aggregates earlier than sandwich-cultured cells. Bile canaliculi-like structures were observed in every cell culture system but were more prominent in serum-free cultures. Hepatocytes in collagen-sandwich configuration and serum-free medium were the most viable after 72 h of culture, still displaying polygonal shape, clear cytoplasm and stable canaliculi-like structures. Differential gene expression patterns were determined for each cell culture condition using quantitative TaqMan Low Density Arrays (LDA). Gene expression analysis revealed distinct profiles in monolayer versus sandwich cultures and in particular in serum-free versus serum-containing culture medium. The hepatocytes cultured in the collagen-sandwich with serum-free medium showed the least variation in expression values over time. Importantly, stress markers were not induced in the serum-free sandwich culture, in contrast to the monolayer and the serum-containing sandwich cultures. Additionally, expression of the investigated cytochrome P450 genes was maintained in the serum-free monolayer and the sandwich cultures. In conclusion, culturing primary rat hepatocytes in a sandwich between two layers of gelled collagen and in a serum-free medium formulation, appears to be most suitable for long-term in vitro hepatotoxicity screening.

摘要

我们将原代大鼠肝细胞在胶原蛋白单层以及胶原蛋白夹心培养体系中进行培养,使用含血清或无血清培养基配方。对肝细胞的形态学监测显示,在胶原蛋白单层上培养的肝细胞呈现多边形形状,且比夹心培养的细胞更早开始形成聚集体。在每个细胞培养体系中均观察到胆小管样结构,但在无血清培养中更为明显。在培养72小时后,处于胶原蛋白夹心结构且使用无血清培养基培养的肝细胞活力最强,仍呈现多边形形状,细胞质清晰,胆小管样结构稳定。使用定量TaqMan低密度阵列(LDA)确定了每种细胞培养条件下的差异基因表达模式。基因表达分析显示,单层培养与夹心培养之间,尤其是无血清培养基与含血清培养基培养之间,存在明显不同的表达谱。在胶原蛋白夹心结构中使用无血清培养基培养的肝细胞,其表达值随时间的变化最小。重要的是,与单层培养和含血清的夹心培养不同,在无血清夹心培养中未诱导应激标志物。此外,在无血清单层培养和夹心培养中,所研究的细胞色素P450基因的表达得以维持。总之,将原代大鼠肝细胞培养在两层胶凝胶原蛋白之间并使用无血清培养基配方,似乎最适合用于长期体外肝毒性筛选。

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