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WANG Jing-ge, YU Xiao-qin, WEN Ji-rui, et al. Screening of the Optimum Medium for Rat Mesenchymal Stem Cells[J]. Journal of Sichuan University (Medical Sciences), 2019, 50(6): 891-895.
Citation: WANG Jing-ge, YU Xiao-qin, WEN Ji-rui, et al. Screening of the Optimum Medium for Rat Mesenchymal Stem Cells[J]. Journal of Sichuan University (Medical Sciences), 2019, 50(6): 891-895.

Screening of the Optimum Medium for Rat Mesenchymal Stem Cells

  •   Objective  To investigate the effect of three different cell culture mediums, DMEM-LG, α-MEM and DMEM/F12, on the growth of rat bone marrow mesenchymal stem cells (BMSCs) in vitro, and so that to screen out the most suitable medium for in vitro culturing the rat BMSCs.
      Methods  BMSCS were isolated from the femur and tibia of SD rats by whole bone marrow differential adherence method. The isolated cells were then cultured with three culture mediums, DMEM-LG, α-MEM and DMEM/F12. The rat BMSCs morphology, adhesion, proliferation, the time of passage and the number the colony at day 14 in three mediums respectively were observed with inverted phase contrast microscopy and compared. Flow cytometry was used to identify and observe the effects of different mediums on the surface antigen expression of rats BMSCs.
      Results  Compared with the other two groups of media, BMSCs cultured in DMEM-LG had shorter colony formation time, shorter first passage time, more clone formation (14±2) and showed uniform morphology and the highest attachment efficiency (47.0±2.8)%. Meanwhile, BMSCs cultured with DMEM-LG entered logarithmic growth phase after only 4 days of culturing and showed the highest average specific growth rate and the largest average number of propagations per unit time. The total number of cells reached about (2.2-2.7)×105 mL-1 within three days. The cells cultured with 3 mediums were all identified as rat BMSCs, and the expression of surface antigen in BMSCs was not significantly affected by different media.
      Conclusion  DMEM-LG is more suitable for proliferation of rat BMSCs in vitro.
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