Figure 3.
Figure 3. Mobilization and differentiation of mesenchymal stem cells (CMG cells) into cardiomyocytes in vitro and in vivo. (A) The experimental protocol is shown. The CMG-ME cells are CMG cells that have been permanently transfected with a plasmid-encoding EGFP driven by the myosin light chain promoter (pMLC2v-EGFP). (B,C) Cultured CMG-ME cells were treated with 5-azacytidine and immunoassayed with anti-GATA4 (red) antibody on the seventh day of culture. GATA4 was expressed in the CMG-ME cells. Some of the CMG-ME cells became EGFP+ (green). (D,E) At 3 weeks, CMG-ME cells that were positive for both EGFP and actinin were observed, indicating that the cells had differentiated into cardiomyocytes. (F) The engraftment of CMG-ME cells into the recipients' BM was confirmed by PCR. Representative results using BM samples collected from recipient mice (samples 1 and 2) are shown. The transgene was clearly detected in the 2 samples. P indicates positive control (CMG-ME cells); N, negative control (CMG cells); M, marker. P:N controls are shown as the percentage with respect to the positive control. (G,H) The myocardium of infarcted mice that received transplants of CMG-ME cells was analyzed using immunofluorescent microscopy. The green, red, and blue signals indicate EGFP, actinin, and nuclei, respectively. EGFP+ actinin+ CMG-ME cells were observed in the myocardium, indicating that the CMG-ME cells had been mobilized into the ischemic myocardium. Actinin and EGFP expression, driven by the MLC-2v promoter, was detected, indicating that the cells had differentiated into cardiomyocytes. Bars indicate 10 μm.

Mobilization and differentiation of mesenchymal stem cells (CMG cells) into cardiomyocytes in vitro and in vivo. (A) The experimental protocol is shown. The CMG-ME cells are CMG cells that have been permanently transfected with a plasmid-encoding EGFP driven by the myosin light chain promoter (pMLC2v-EGFP). (B,C) Cultured CMG-ME cells were treated with 5-azacytidine and immunoassayed with anti-GATA4 (red) antibody on the seventh day of culture. GATA4 was expressed in the CMG-ME cells. Some of the CMG-ME cells became EGFP+ (green). (D,E) At 3 weeks, CMG-ME cells that were positive for both EGFP and actinin were observed, indicating that the cells had differentiated into cardiomyocytes. (F) The engraftment of CMG-ME cells into the recipients' BM was confirmed by PCR. Representative results using BM samples collected from recipient mice (samples 1 and 2) are shown. The transgene was clearly detected in the 2 samples. P indicates positive control (CMG-ME cells); N, negative control (CMG cells); M, marker. P:N controls are shown as the percentage with respect to the positive control. (G,H) The myocardium of infarcted mice that received transplants of CMG-ME cells was analyzed using immunofluorescent microscopy. The green, red, and blue signals indicate EGFP, actinin, and nuclei, respectively. EGFP+ actinin+ CMG-ME cells were observed in the myocardium, indicating that the CMG-ME cells had been mobilized into the ischemic myocardium. Actinin and EGFP expression, driven by the MLC-2v promoter, was detected, indicating that the cells had differentiated into cardiomyocytes. Bars indicate 10 μm.

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