There is evidence that endothelial nitric-oxide synthase (eNOS) is regulated by reciprocal dephosphorylation of Thr 497 and phosphorylation of Ser 1179 . To examine the interrelationship between these sites, cells were transfected with wild-type (WT), T497A, T497D, S1179D, and T497A/S1179D eNOS and activity, NO release and eNOS localization were assessed. Although eNOS T497A, S1179D and T497A/S1179D eNOS had greater enzymatic activity than did WT eNOS in lysates, basal production of NO from cells was markedly reduced in cells transfected with T497A and T497A/S1179D eNOS but augmented in cells transfected with S1179D eNOS. Stimulating cells with ATP or ionophore normalized the loss of function seen with T497A and T497A/S1179D eNOS to levels observed with WT and S1179D eNOS, respectively. Despite these functional differences, the localization of eNOS mutants were similar to WT. Because both T497A and T497A/S1179D eNOS exhibited higher enzyme activity but reduced production of NO, we examined whether these mutations were "uncoupling" NO synthesis. T497A and T497A/S1179D eNOS generated 2-3 times more superoxide anion than WT eNOS, and both basal and stimulated interactions of T497A/S1179D eNOS with hsp90 were reduced in co-immunoprecipitation experiments. Thus, the phosphorylation/dephosphorylation of Thr 497 may be an intrinsic switch mechanism that determines whether eNOS generates NO versus superoxide in cells.
Endothelial nitric-oxide synthase (eNOS)1 produces the free radical gas, nitric oxide, which has been implicated in the regulation of cardiovascular homeostasis. Due to its importance to overall cardiovascular health, nature has evolved multiple control mechanisms that tightly regulate the enzymatic function of eNOS. eNOS is a prototype for proteins regulated by spatial and temporal signals, namely subcellular targeting to the Golgi complex and lipid rafts/caveolae by protein-protein interactions and phosphorylation events (1). These complex post-translational mechanisms control the state of eNOS activation/inactivation and the fidelity of electron flux through the reductase domain of the protein to the oxygenase domain where the chemistry of NO synthesis occurs. Dysregulation of the synthesis of eNOS cofactors, protein-protein interactions, and phosphorylation could potentially "uncouple eNOS," i.e. electron transfer reactions result in the production of superoxide, instead of NO.eNOS can be phosphorylated on serines 116, 617, 635, and 1179 and phosphorylated on threonine 497 (bovine amino acids) (2-9). The phosphorylation of serines 617, 635, and 1179 all result in the activation of eNOS function, whereas the phosphorylation of serine 116 and threonine 497 may reduce eNOS function (3,4,7,10). There is a good correlation between threonine 497 (bovine)/threonine 495 (human) dephosphorylation and NO production (measured as cGMP) but not Ser 1179 phosphorylation when bradykinin is used as an agonist for NO production, suggesting that Thr 497 dephosphorylation is sufficient for eNOS activation (3, 4, 7). Usin...
