Fig. 3.
Fig. 3. Expression of c-kit and c-mpl in CD34+ BM cells and cultured mast cells grown by SCF + TPO. The expression of c-kit and c-mpl in CD34+ BM cells and 15-week-old cultured cells grown by SCF + TPO were examined using (a) flow cytometric analysis and (b) RT-PCR analysis. Day 10 megakaryocytic cells generated by TPO alone from CD34+ cord blood cells were used as positive controls. (a) Flow cytometric analysis: (A), CD34+ BM cells; (B), 15-week-old cultured cells grown by SCF + TPO; (C), Day 10 cultured CD41+ cells grown by TPO. (—), labeled with PE-conjugated anti–c-kit MoAb or anti–c-mpl MoAb followed by FITC-conjugated GAM. (---), labeled with PE-conjugated mouse IgG1 or control mouse IgG1 followed by FITC-conjugated GAM. The abscissa shows the fluorescence intensity of each surface marker, and the ordinate shows the number of cells. (b) RT-PCR analysis: lane 1, no RNA; lane 2, CD34+ BM cells; lane 3, cultured c-kit+ cells grown by SCF + TPO; lane 4, cultured CD41+ cells grown by TPO.

Expression of c-kit and c-mpl in CD34+ BM cells and cultured mast cells grown by SCF + TPO. The expression of c-kit and c-mpl in CD34+ BM cells and 15-week-old cultured cells grown by SCF + TPO were examined using (a) flow cytometric analysis and (b) RT-PCR analysis. Day 10 megakaryocytic cells generated by TPO alone from CD34+ cord blood cells were used as positive controls. (a) Flow cytometric analysis: (A), CD34+ BM cells; (B), 15-week-old cultured cells grown by SCF + TPO; (C), Day 10 cultured CD41+ cells grown by TPO. (—), labeled with PE-conjugated anti–c-kit MoAb or anti–c-mpl MoAb followed by FITC-conjugated GAM. (---), labeled with PE-conjugated mouse IgG1 or control mouse IgG1 followed by FITC-conjugated GAM. The abscissa shows the fluorescence intensity of each surface marker, and the ordinate shows the number of cells. (b) RT-PCR analysis: lane 1, no RNA; lane 2, CD34+ BM cells; lane 3, cultured c-kit+ cells grown by SCF + TPO; lane 4, cultured CD41+ cells grown by TPO.

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