Spatial redistribution of traction forces as a function of time. NIH3T3 cells were plated onto mPADs for 2–24 h. (A–C) Traction force maps (upper), actin epifluorescence (middle), and fibronectin immunofluorescence (lower) from representative cells at 2 h (A), 9 h (B), and 18 h (C), respectively, after plating. Traction forces were initially large at the cell periphery (black vectors) and small toward the cell center (red vectors), but progressed toward a pattern with smaller peripheral vectors and larger interior vectors. Scale bars in immunofluorescence images, 20 μm. Scale vectors in traction force maps, 20 nN. (D) The percentage of total cell force generated away from the cell periphery (black) increased with time over the first 10 h of plating and then oscillated with continued time in culture. Fibronectin fibril size (gray) fluctuated in accordance with the changes in the percentage of interior force. Each time point is an average of data from N = 9–20 cells. Bars represent the mean ± SE. (E) Interior force percentage was plotted against cell size for cells plated onto mPADs for 4.5, 6, 7.5, 9, and 12 h (gray arrows). Data indicate that cell size remained constant during this period of largest increase in interior force percentage (6–9 h).