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优化一种有效的定向分化培养基,用于在体外将小鼠骨髓间充质干细胞分化为肝细胞。

Optimization of an effective directed differentiation medium for differentiating mouse bone marrow mesenchymal stem cells into hepatocytes in vitro.

作者信息

Shi Xiao-Lei, Mao Liang, Xu Bi-Yun, Xie Ting, Zhu Zhang-Hua, Chen Jun-Hao, Li Lei, Ding Yi-Tao

机构信息

Department of Hepatobiliary Surgery, Affiliated Drum Tower Hospital, Medical College of Nanjing University, No. 321 Zhongshan Road, Nanjing 210008, PR China.

出版信息

Cell Biol Int. 2008 Aug;32(8):959-65. doi: 10.1016/j.cellbi.2008.04.013. Epub 2008 Apr 10.

Abstract

We have used a uniform design to explore the most effective directed differentiation medium (MEDDM) for differentiating mouse bone marrow mesenchymal stem cells (mMSCs) into hepatocytes. Our methods involved arranging eight differentiation medium groups following uniform design. Flow cytometry was used to evaluate the percentage of ALB+ and CK18+ cells in each group. Factors and their concentrations in the MEDDMs were then identified. The MEDDMs were evaluated by their ability to differentiate mMSCs into hepatocytes by RNA and protein expressions and synthesis functions. FGF at 35 ng/ml and OSM at 30 ng/ml in the medium yielded the highest percentage of ALB+ and CK18+ cells. During directed differentiation using MEDDMs, ALB, CK18, TTR, AFP mRNAs were expressed. ALB and CK18 proteins were detected in the cells. The differentiated cells produced albumin and urea in a time dependent manner. Uniform design was adequate for choosing the MEDDM of mMSCs. MEDDM containing 35 ng/ml FGF and 30 ng/ml OSM was effective in differentiating mMSCs into hepatocytes.

摘要

我们采用均匀设计法来探索将小鼠骨髓间充质干细胞(mMSCs)分化为肝细胞的最有效定向分化培养基(MEDDM)。我们的方法包括按照均匀设计安排八个分化培养基组。使用流式细胞术评估每组中ALB+和CK18+细胞的百分比。然后确定MEDDMs中的因子及其浓度。通过RNA和蛋白质表达以及合成功能,根据MEDDMs将mMSCs分化为肝细胞的能力对其进行评估。培养基中35 ng/ml的FGF和30 ng/ml的OSM产生的ALB+和CK18+细胞百分比最高。在使用MEDDMs进行定向分化过程中,ALB、CK18、TTR、AFP mRNA表达。在细胞中检测到ALB和CK18蛋白。分化后的细胞以时间依赖性方式产生白蛋白和尿素。均匀设计足以选择mMSCs的MEDDM。含有35 ng/ml FGF和30 ng/ml OSM的MEDDM在将mMSCs分化为肝细胞方面是有效的。

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