OLIGOMERIZATION OF ENDOTHELIAL NITRIC-OXIDE SYNTHASE - EVIDENCE FOR A DOMINANT-NEGATIVE EFFECT OF TRUNCATION MUTANTS

Nitric oxide produced by the endothelial isoform of nitric oxide synthase (ecNOS) is a key determinant of vascular tone, In contrast to other nitric oxide synthase (NOS) isoforms, which have been characterized as soluble homodimeric enzymes, ecNOS is predominantly membrane-associated, a feature that has hindered direct biochemical analyses of its oligomeric structure, We investigated ecNOS oligomerization using co immunoprecipitation experiments in transiently transfected COS-7 cells. When COS-7 cells co transfected with constructs encoding wild-type ecNOS and an epitope-tagged myristoylation-deficient mutant were biosynthetically labeled with [H-3]myristate, the antibody to the epitope tag specifically immunoprecipitated H-3-labeled ecNOS, reflecting enzyme oligomerization, In COS-7 cells transfected with cDNAs encoding epitope-tagged truncation mutants and untagged full-length ecNOS, the wild-type enzyme could be immunoprecipitated by the antibody to the epitope tag, Co-immunoprecipitation of ecNOS with truncation mutants documented that both N- and C-terminal domains are involved in ecNOS oligomerization, When these truncation mutants are coexpressed with wild-type ecNOS, they exert a marked dominant negative effect on enzyme activity. Since NOS oligomerization itself may be subject to dynamic modulation, the regulation of ecNOS assembly may have implications for NO signaling in the vascular wall.