Figure 2
Figure 2. Mks form podosomes on different substrata. Cells were spread for 3 hours on 100 μg/mL fibrinogen or fibronectin-coated surfaces or on glass, and then fixed and stained for F-actin (red, phalloidin) and WASp (A, C, D) or vinculin (B) (green). The right panel of pictures shows the merge of both channels. Mks were spread for 3 hours on 100 μg/mL Horm collagen-coated surface ±250 ng/mL SDF. Cells were analyzed for (E) the number of podosomes, (F) cell surface area, and (G) podosomes per μm2. Scale bars represent 10 μm. Red square indicates enlarged area to highlight podosomes. Data are representative of at least 3 experiments.

Mks form podosomes on different substrata. Cells were spread for 3 hours on 100 μg/mL fibrinogen or fibronectin-coated surfaces or on glass, and then fixed and stained for F-actin (red, phalloidin) and WASp (A, C, D) or vinculin (B) (green). The right panel of pictures shows the merge of both channels. Mks were spread for 3 hours on 100 μg/mL Horm collagen-coated surface ±250 ng/mL SDF. Cells were analyzed for (E) the number of podosomes, (F) cell surface area, and (G) podosomes per μm2. Scale bars represent 10 μm. Red square indicates enlarged area to highlight podosomes. Data are representative of at least 3 experiments.

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