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A Comparative Analysis of Mesenchymal Stem-Cell Lines Derived from Bone Marrow and Limb Muscle of Early Human Embryos

机译:人体早期胚胎的骨髓和四肢肌肉间充质干细胞系的比较分析

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The properties of mesenchymal stem-cell (MSC) lines derived from bone marrow (FetMSC) and limb muscle (M-FetMSC) of 5- to 6-week human embryos were assayed. The main cell-line characteristics were obtained at the sixth passage. The average cell-population doubling time was 33.0 ± 1.4 h for FetMSC and 25.0 ± 0.1 h for M-FetMSC. Growth curves indicated active cell proliferation. Numerical and structural karyotypic analysis showed that these lines have normal karyotype, 46, XY. Cell surface markers were analyzed by flow cytometry. It was found that the cells express CD44, CD73, CD90, CD 105, and HLA-ABC surface antigens and vimentin; which are common for human MSC beings, and lack CD34 and HLA-DR. The cells were capable of osteogenic, chondrogenic, and adipogenic differentiation. Immunofluorescence and flow-cytometry assays reveled a lack of surface antigen TRA-1-60, high expression of surface antigen SSEA-4, and low expression of transcription factor Oct-4 attributed to human embryonic stem cells.Immunofluorescence analysis showed the presence of early differentiation markers, three germ-layer derivatives for human embryonic stem cells. This makes MSCs useful for repair of damaged tissue in the corresponding microenvironment. Despite their sharedMSC status, the FetMSC and M-FetMSC lines displayed some interlinear differences related to growth characteristics and differentiation potential. The MFetMSC line exhibited reduced potential for adipogenic differentiation compared to the FetMSC line. Immunofluorescence analysis revealed Z-disks in M-FetMSC, but not in FetMSC, during skeletal-muscle differentiation. These findings suggest that the different microenvironment has an influence when cells are in an organism before their transplantation in vitro.
机译:分析了5至6周人类胚胎的骨髓(FetMSC)和肢体肌肉(M-FetMSC)来源的间充质干细胞(MSC)的特性。在第六代获得主要细胞系特性。 FetMSC的平均细胞群体倍增时间为33.0±1.4 h,M-FetMSC的平均细胞群体倍增时间为25.0±0.1 h。生长曲线表明活跃的细胞增殖。数值和结构核型分析表明,这些品系具有正常的核型,46,XY。通过流式细胞仪分析细胞表面标志物。发现细胞表达CD44,CD73,CD90,CD 105和HLA-ABC表面抗原和波形蛋白。它们是人类MSC常见的,并且缺乏CD34和HLA-DR。这些细胞具有成骨性,成软骨性和成脂性的能力。免疫荧光和流式细胞仪检测发现缺乏表面抗原TRA-1-60,表面抗原SSEA-4高表达和归因于人类胚胎干细胞的转录因子Oct-4低表达。免疫荧光分析显示早期存在分化标志物,人类胚胎干细胞的三种胚层衍生物。这使得MSC可用于修复相应微环境中的受损组织。尽管它们具有共享的MSC状态,但FetMSC和M-FetMSC品系显示出一些与生长特性和分化潜能有关的线性差异。与FetMSC系相比,MFetMSC系显示出成脂分化潜力降低。免疫荧光分析显示,骨骼肌分化过程中M-FetMSC中存在Z盘,而FetMSC中没有Z盘。这些发现表明,当细胞在体外移植之前处于生物体内时,不同的微环境会产生影响。

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