Figure 7.
Figure 7. Effect of MVs from healthy and diabetic individuals on differentiation of K562 cells. (A-D) Cells were treated for 72 hours with medium (control, gray) or in vivo circulating MVs from healthy (2 μg/mL; A-B) or diabetic individuals (5 μg/mL; C-D) respectively, in the absence (blue trace) or presence of 30 μM cyclopamine (red trace). (E-H) Cells were treated for 72 hours with medium (gray) or 5 μg/mL MVs generated from PHA/PMA/act D-treated lymphocytes from healthy (E-F) or diabetic individuals (G-H) in the absence (blue trace) or presence of 30 μM cyclopamine (red trace). Detection of αIIbβ3 and CD42b expression was performed by flow cytometry after labeling by the corresponding antibody. Fluorescence (FL2, red fluorescence channel intensity) is expressed in arbitrary units (au). Data are representative of 4 experiments yielding similar results. (I-J) Histograms representing the increase of mean fluorescence intensity (± SEM) reflecting the expression level of αIIbβ3 (I) and CD42b (J), in control cells, or in cells treated with circulating MVs from healthy (2 μg/mL, white bars) or diabetic individuals (5 μg/mL, black bars) or 5 μg/mL MVs generated from PHA/PMA/act D–treated lymphocytes from healthy (hatched bars) or diabetic individuals (dotted bars) in the absence or presence of 30 μM cyclopamine (cycl). *P < .05, **P < .01, ***P < .001, significantly different from nontreated control cells; †P < .05, ††P < .01, significantly different from MV-treated cells.

Effect of MVs from healthy and diabetic individuals on differentiation of K562 cells. (A-D) Cells were treated for 72 hours with medium (control, gray) or in vivo circulating MVs from healthy (2 μg/mL; A-B) or diabetic individuals (5 μg/mL; C-D) respectively, in the absence (blue trace) or presence of 30 μM cyclopamine (red trace). (E-H) Cells were treated for 72 hours with medium (gray) or 5 μg/mL MVs generated from PHA/PMA/act D-treated lymphocytes from healthy (E-F) or diabetic individuals (G-H) in the absence (blue trace) or presence of 30 μM cyclopamine (red trace). Detection of αIIbβ3 and CD42b expression was performed by flow cytometry after labeling by the corresponding antibody. Fluorescence (FL2, red fluorescence channel intensity) is expressed in arbitrary units (au). Data are representative of 4 experiments yielding similar results. (I-J) Histograms representing the increase of mean fluorescence intensity (± SEM) reflecting the expression level of αIIbβ3 (I) and CD42b (J), in control cells, or in cells treated with circulating MVs from healthy (2 μg/mL, white bars) or diabetic individuals (5 μg/mL, black bars) or 5 μg/mL MVs generated from PHA/PMA/act D–treated lymphocytes from healthy (hatched bars) or diabetic individuals (dotted bars) in the absence or presence of 30 μM cyclopamine (cycl). *P < .05, **P < .01, ***P < .001, significantly different from nontreated control cells; †P < .05, ††P < .01, significantly different from MV-treated cells.

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