Figure 1. PKCδ activity inversely affects p190 activity.

Confluent LMVEC were treated with vehicle (DMSO) or 10μM rottlerin for 30min (panel a) or infected with adenoviral vectors encoding GFP or wild-type PKCδ cDNA (panel b). Cells were harvested and p190 activity determined. The level of active p190 relative to total p190 was determined by densitometry. In panel b, GFP and PKCδ overexpression was confirmed in the transfected endothelial cells by immunoblot analysis. Data are presented as the mean ± SE. Panel a, n = 4; *p<0.05 vs. vehicle. Panel b, n = 7, ^#p<0.05 vs. GFP.