OBJECTIVES: The aim of this study was to determine an optimal culture method for porcine bone marrow-derived endothelial progenitor cells (EPCs). MATERIALS AND METHODS: Mononuclear cells (MNCs) were isolated by density centrifugation and differentiated into EPCs in in vitro. At first-passage, EPCs were cultured at different cell densities (5 x 10(3), 1 x 10(4), 2 x 10(4) or 5 x 10(4)/cm(2)) and in basic medium (EGM, medium 199, DMEM or 1640) supplemented with FBS (2%, 5%, 10% or 20%) and different combinations of cytokines (VEGF, VEGF + bFGF, VEGF + bFGF + EGF, or VEGF + bFGF + EGF + IGF), the experiment being based on L(64) (4(21)) orthogonal design. RESULTS AND CONCLUSIONS: This demonstrated that the optimal culture method for our EPCs displayed higher expansion and migration rates as compared to other groups, by analysis of variance; that is, cultured at 1 x 10(4)/cm(2) in M199 supplemented with 10% FBS and VEGF + bFGF + IGF + EGF. Furthermore, percentage of positive cells stained by Dil-ac-LDL and FITC-UEA-1 was more than 65%, and as shown by immunohistochemistry, these cells also stained positively for CD133, CD34 and KDR. The present study indicates that the number and function of porcine EPCs significantly increased when using our optimized culture parameters.
展开▼
机译:目的:本研究的目的是确定猪骨髓源性内皮祖细胞(EPC)的最佳培养方法。材料与方法:通过密度离心分离单核细胞,并在体外分化为EPC。首次传代时,将EPC以不同的细胞密度(5 x 10(3),1 x 10(4),2 x 10(4)或5 x 10(4)/ cm(2))和基本培养基进行培养(EGM,培养基199,DMEM或1640)补充了FBS(2%,5%,10%或20%)和不同的细胞因子组合(VEGF,VEGF + bFGF,VEGF + bFGF + EGF或VEGF + bFGF + EGF + IGF),该实验基于L(64)(4(21))正交设计。结果与结论:通过方差分析表明,与其他组相比,我们EPC的最佳培养方法显示出更高的扩增和迁移速率。也就是说,在添加了10%FBS和VEGF + bFGF + IGF + EGF的M199中以1 x 10(4)/ cm(2)培养。此外,Dil-ac-LDL和FITC-UEA-1染色的阳性细胞百分比超过65%,并且如免疫组织化学所示,这些细胞的CD133,CD34和KDR也呈阳性染色。本研究表明,当使用我们优化的培养参数时,猪EPC的数量和功能显着增加。
展开▼
