Abstract
Protein-protein interactions represent an important post-translational mechanism for endothelial nitric-oxide synthase (eNOS) regulation. We have previously reported that beta-actin is associated with eNOS oxygenase domain and that association of eNOS with beta-actin increases eNOS activity and nitric oxide (NO) production. In the present study, we found that beta-actin-induced increase in NO production was accompanied by decrease in superoxide formation. A synthetic actin-binding sequence (ABS) peptide 326 with amino acid sequence corresponding to residues 326-333 of human eNOS, one of the putative ABSs, specifically bound to beta-actin and prevented eNOS association with beta-actin in vitro. Peptide 326 also prevented beta-actin-induced decrease in superoxide formation and increase in NO and L-citrulline production. A modified peptide 326 replacing hydrophobic amino acids leucine and tryptophan with neutral alanine was unable to interfere with eNOS-beta-actin binding and to prevent beta-actin-induced changes in NO and superoxide formation. Site-directed mutagenesis of the actin-binding domain of eNOS replacing leucine and tryptophan with alanine yielded an eNOS mutant that exhibited reduced eNOS-beta-actin association, decreased NO production, and increased superoxide formation in COS-7 cells. Disruption of eNOS-beta-actin interaction in endothelial cells using ABS peptide 326 resulted in decreased NO production, increased superoxide formation, and decreased endothelial monolayer wound repair, which was prevented by PEG-SOD and NO donor NOC-18. Taken together, this novel finding indicates that beta-actin binding to eNOS through residues 326-333 in the eNOS protein results in shifting the enzymatic activity from superoxide formation toward NO production. Modulation of NO and superoxide formation from eNOS by beta-actin plays an important role in endothelial function.
Highlights
Nitric oxide (NO) generated by endothelial NO synthase2 plays an important role in a number of physiological and pathophysiological processes including regulation of vascular tone, smooth muscle cell proliferation, and angiogenesis [1,2,3,4]
We have found that endothelial NO synthase (eNOS) localized to the plasma membrane is colocalized with cortical filamentous polymerized actin (F-actin). eNOS that is located in the perinuclear area is colocalized with globular actin (G-actin) [5,6,7,8]. eNOS and actin in endothelial cells can be co-immunoprecipitated, suggesting that eNOS is associated with -actin protein [8]
Using a yeast two-hybrid experiment, we have reported that the eNOS oxygenase domain rather than the reductase domain or the middle part of the eNOS molecule has direct interaction with -actin, suggesting that the actin-binding site is in the oxygenase domain of the eNOS protein [7]
Summary
Nitric oxide (NO) generated by endothelial NO synthase (eNOS)2 plays an important role in a number of physiological and pathophysiological processes including regulation of vascular tone, smooth muscle cell proliferation, and angiogenesis [1,2,3,4]. Site-directed mutagenesis of the actin-binding domain of eNOS replacing leucine and tryptophan with alanine yielded an eNOS mutant that exhibited reduced eNOS--actin association, decreased NO production, and increased superoxide formation in COS-7 cells. Disruption of eNOS--actin interaction in endothelial cells using ABS peptide 326 resulted in decreased NO production, increased superoxide formation, and decreased endothelial monolayer wound repair, which was prevented by PEG-SOD and NO donor NOC-18.
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