Neutralizing a Surface Charge on the FMN Subdomain Increases the Activity of Neuronal Nitric-oxide Synthase by Enhancing the Oxygen Reactivity of the Enzyme Heme-Nitric Oxide Complex |
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Authors: | Mohammad Mahfuzul Haque Mohammed Fadlalla Zhi-Qiang Wang Sougata Sinha Ray Koustubh Panda Dennis J. Stuehr |
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Affiliation: | From the ‡Department of Pathobiology, Lerner Research Institute, The Cleveland Clinic, Cleveland, Ohio 44195, ;the §Department of Chemistry, Kent State University-Tuscarawas, New Philadelphia, Ohio 44663, and ;the ¶Center for Genetic Engineering and Biotechnology, University of Calcutta, Kolkata 700019, India |
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Abstract: | Nitric-oxide synthases (NOSs) are calmodulin-dependent flavoheme enzymes that oxidize l-Arg to nitric oxide (NO) and l-citrulline. Their catalytic behaviors are complex and are determined by their rates of heme reduction (kr), ferric heme-NO dissociation (kd), and ferrous heme-NO oxidation (kox). We found that point mutation (E762N) of a conserved residue on the enzyme''s FMN subdomain caused the NO synthesis activity to double compared with wild type nNOS. However, in the absence of l-Arg, NADPH oxidation rates suggested that electron flux through the heme was slower in E762N nNOS, and this correlated with the mutant having a 60% slower kr. During NO synthesis, little heme-NO complex accumulated in the mutant, compared with ∼50–70% of the wild-type nNOS accumulating as this complex. This suggested that the E762N nNOS is hyperactive because it minimizes buildup of an inactive ferrous heme-NO complex during NO synthesis. Indeed, we found that kox was 2 times faster in the E762N mutant than in wild-type nNOS. The mutational effect on kox was independent of calmodulin. Computer simulation and experimental measures both indicated that the slower kr and faster kox of E762N nNOS combine to lower its apparent Km,O2 for NO synthesis by at least 5-fold, which in turn increases its V/Km value and enables it to be hyperactive in steady-state NO synthesis. Our work underscores how sensitive nNOS activity is to changes in the kox and reveals a novel means for the FMN module or protein-protein interactions to alter nNOS activity.Nitric oxide (NO)2 is a biological mediator that is produced in animals by three NO synthase isozymes (NOS, EC 1.14.13.39): inducible NOS (iNOS), neuronal NOS (nNOS), and endothelial NOS (eNOS) (1, 2). The NOS are modular enzymes composed of an N-terminal oxygenase domain and a C-terminal flavoprotein domain, with a calmodulin (CaM)-binding site connecting the two domains (3). During NO synthesis, the flavoprotein domain transfers NADPH-derived electrons through its FAD and FMN cofactors to a heme located in the oxygenase domain. The FMN-to-heme electron transfer enables heme-dependent oxygen activation and a stepwise conversion of l-Arg to NO and citrulline (4, 5). Heme reduction also requires that CaM be bound to NOS and is rate-limiting for NO biosynthesis (6–9).NOS enzymes operate under the constraint of having their newly made NO bind to the ferric heme before it can exit the enzyme (10). How this intrinsic heme-NO binding event impacts NOS catalytic cycling is shown in and has previously been discussed in detail (10–13). The l-Arg to NO biosynthetic reaction (FeIII to FeIIINO in ) is limited by the rate of ferric heme reduction (kr), because all biosynthetic steps downstream are faster than kr. However, once the ferric heme-NO complex forms at the end of each catalytic cycle, it can either dissociate to release NO into the medium (at a rate kd as shown in ) or become reduced by the flavoprotein domain (at a rate k′r in ; equal to kr) to form the enzyme ferrous heme-NO species (FeIINO), which releases NO very slowly (11, 12). Consequently, two cycles compete during steady-state NO synthesis (); NO dissociation from the ferric heme (kd) is part of a “productive cycle” that releases NO and is essential for NOS bioactivity, whereas reduction of the ferric heme-NO complex (kr′) channels the enzyme into a “futile cycle” that actually represents a NO dioxygenase activity. The rate of futile cycling is also determined by the rate of O2 reaction with the ferrous heme-NO complex (at a rate kox in ), which regenerates the ferric enzyme. Surprisingly, NOS enzymes have evolved to have a broad range of kr (varies 40×), kox (varies 15×), and kd (varies 30×) values (Table S1) (12). This causes each NOS to distribute quite differently during steady-state NO synthesis and gives each NOS a unique catalytic profile (12).Open in a separate windowGlobal kinetic model for NOS catalysis. Ferric enzyme reduction (kr) is rate-limiting for the biosynthetic reactions (central linear portion). kcat1 and kcat2 are the conversion rates of the enzyme FeIIO2 species to products in the l-Arg and Nω-hydroxy-l-arginine (NOHA) reactions, respectively. The ferric heme-NO product complex (FeIIINO) can either release NO (kd) or become reduced (k′r) to a ferrous heme-NO complex (FeIINO), which reacts with O2 (kox) to regenerate ferric enzyme. Enzyme partitioning and NO release are determined by the relative rates of kr, kox, and kd. This figure is adapted from Ref. 12.The enzyme physical and electronic factors that may set and regulate each of the three kinetic parameters (kr, kox, and kd) in NOS enzymes remain to be fully described. At present, the composition of the NOS flavoprotein domain and CaM appear to be primarily responsible for determining the kr (14–17), whereas the composition of the NOS oxygenase domain is presumed to determine the kd and kox (18, 19). Indeed, our recent point mutagenesis study identified a patch of electronegative residues on the FMN subdomain that are required to maintain a normal kr and NO synthesis activity in nNOS, suggesting that subdomain electrostatic interactions are important in the process (20). We found particularly large effects when the negative charge at Glu762 was neutralized via mutation to Asn. Remarkably, the NO synthesis activity of E762N nNOS was double that of wild-type nNOS, despite the mutant displaying a slow kr that was half of wild type. In the current report, we show that the E762N mutation has an additional, unsuspected effect on the kox kinetic parameter of nNOS. How this effect alters distribution of the nNOS enzyme during steady-state catalysis, impacts the apparent Km,O2, and leads to hyperactive NO synthesis is described. Our finding that the nNOS flavoprotein domain can tune a key kinetic parameter that defines the rate of a heme-based reaction in the nNOS oxygenase domain is unusual and suggests a means by which protein-protein interactions could regulate the catalytic behavior of nNOS. |
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