Nitric Oxide Activation of Guanylate Cyclase Pushes the α1 Signaling Helix and the β1 Heme-binding Domain Closer to the Substrate-binding Site*

Background: NO-induced conformational changes of guanylate cyclase were analyzed. Results: FRET experiments show a movement of two tryptophans toward a fluorescent substrate. Conclusion: Activation is transmitted to the catalytic domain by direct interaction of the heme binding domain and through the coiled-coil helix. Significance: The results help to advance understanding of the molecular events associated with activation of NOsGC. The complete structure of the assembled domains of nitric oxide-sensitive guanylate cyclase (NOsGC) remains to be determined. It is also unknown how binding of NO to heme in guanylate cyclase is communicated to the catalytic domain. In the current study the conformational change of guanylate cyclase on activation by NO was studied using FRET. Endogenous tryptophan residues were used as donors, the substrate analog 2′-Mant-3′-dGTP as acceptor. The enzyme contains five tryptophan residues distributed evenly over all four functional domains. This provides a unique opportunity to detect the movement of the functional domains relative to the substrate-binding catalytic region. FRET measurements indicate that NO brings tryptophan 22 in the αB helix of the β1 heme NO binding domain and tryptophan 466 in the second short helix of the α1 coiled-coil domain closer to the catalytic domain. We propose that the respective domains act as a pair of tongs forcing the catalytic domain into the nitric oxide-activated conformation.

There are two pharmacologically important classes of guanylate cyclases that catalyze the reaction from GTP to cGMP; some are transmembrane receptors for extracellular peptides and others are intracellular receptors for the gaseous ligand NO (for reviews, see Refs. 1 and 2). Transmembrane and NO-sensitive guanylate cyclases (NOsGC) 2 show significant homology not only in their dimeric catalytic domain but also in the directly preceding helices forming a dimeric coiled-coil. In transmembrane forms similar to GC-A, the extracellular binding of the ligand ANP to preformed homodimers is transmitted across the transmembrane helices and reorients the two intracellular domains into the active conformation (3). By analogy, it was assumed that binding of NO to the amino-terminal heme NO binding (HNOX) domain is communicated to the carboxylterminal catalytic domain through the coiled-coil domain (4). This linear model of NO activation has been questioned by findings that the isolated HNOX domain can directly interact with the isolated catalytic region of NOsGC (5). In support of this, we have shown that the amino termini of NOsGC are in close proximity to the carboxyl termini based on fluorescence resonance energy transfer using fluorescent fusion proteins (6). Fusion of the fluorescent protein to the critical HNOX domain of the ␤ 1 subunit led to a heme-free NO unresponsive enzyme. This proved to be a serious obstacle for the detection of conformational changes during NO activation. In the current paper, we have overcome this challenge by using naturally occurring tryptophans as FRET donors and the substrate analog 2Ј-Mant-3Ј-dGTP as FRET acceptor.
(N-Methyl)anthraniloyl-substituted nucleotides (Mant-NTPs) are fluorescently labeled nucleotides that compete with GTP or ATP for the substrate binding site of adenylate and guanylate cyclases (7,8). Mant-GTP can be converted to Mant-cGMP and has been used to develop an assay of NOsGC activity based on direct fluorescence (9). In contrast, 3Ј-deoxy forms are competitive inhibitors of adenylate and guanylate cyclases (7,8). When tryptophan residues are excited and a sufficient proximity to the Mant group is provided by the conformation of the enzyme, Mant-deoxynucleotides can act as FRET acceptors (10 -12). This energy transfer can then be used to analyze the topical relationship of tryptophans to the substrate-binding site. Under optimal conditions, where a tryptophan moves during ligandinduced activation, conformational changes can be detected.
In the present work, we analyzed conformational changes of full-length NOsGC upon NO-activation using 2Ј-Mant-3Ј-dGTP as a FRET partner of naturally occurring tryptophan residues. NOsGC contains five tryptophan residues, which are evenly distributed over the four functional domains: one is located in the heme NO binding (HNOX) domain of the ␤ 1 subunit (␤ 1 , Trp-22), another resides in the Per-Arnt-Sim (PAS) domain of ␣ 1 (␣ 1 , Trp-352), one is in the coiled-coil domain of the ␣ 1 subunit (␣ 1 , Trp-466) and the last two tryptophan residues are located in the catalytic domain (␣ 1 , Trp-669; ␤ 1 , Trp-602) (Fig. 1). Based on our results, NO occupancy of the amino-terminal HNOX domain is communicated to the catalytic domain both through the coiled-coil helix and by direct interaction between the HNOX and catalytic domain.
Cloning and Site-directed Mutagenesis of Tryptophan Residues-The ␤ 1 subunit of human guanylate cyclase was cloned into the pFASTBAC vector as described by Koglin and Behrends (13). Cloning of the ␣ 1 subunit with Strep-tag II (S) (␣ 1 S) into the pFASTBAC vector was described in Ref. 14. They served as template for site-directed mutagenesis with the QuikChange Lightning mutagenesis kit (Agilent Technologies, Böblingen, Germany).
Expression and Purification of NOsGC-NOsGC subunits were recombinantly co-expressed using the baculovirus/Sf9 system. Recombinant baculoviruses of the respective subunits were generated according to the Bac-To-Bac baculovirus expression system manual (Invitrogen). For cultivation of Sf9 insect cells (Invitrogen catalog no. 11496-015), Sf-900 II serumfree medium was supplemented with 1% penicillin/streptomycin and 10% fetal calf serum. Spinner cultures were grown at 27°C at 140 rpm on a shaking incubator and diluted to 2 ϫ 10 6 cells/ml for infection. 500 ml of cell suspension were co-infected with the recombinant baculovirus stock of the carboxylterminally Strep-tagged ␣ 1 subunit or a corresponding mutant and with either the wild-type or a mutant ␤ 1 subunit. Afterward, the enzyme was purified to apparent homogeneity as described previously (15).
Spectrofluorimetric Measurements-FRET was measured with a Varian spectrofluorometer at 37°C using a quartz UV microcuvette from Hellma (Mühlheim, Germany) in a volume of 50 l. Purified NOsGC and 2Ј-Mant-3Ј-dGTP were used at equimolar concentrations of 3 M. First, spectra of NOsGC were detected, and then 2Ј-Mant-3Ј-dGTP was added. The measurements were performed in a buffer containing 50 mM triethanolamine/HCl, 1 mM EDTA, and 5 mM MnCl 2 (pH 7.4). Previous studies with adenylate cyclase showed that FRET signals were much larger in the presence of Mn 2ϩ than in the presence of Mg 2ϩ (11). The sensitized emission method with three channels was used for the determination of FRET (16). The excitation slit for all excitation wavelengths was 5 nm. In the donor channel, NOsGC was excited at 280 nm and at 295 nm as the tryptophan-specific excitation (17). The emission was detected at 335 nm. In the acceptor channel, 2Ј-Mant-3Ј-dGTP was excited at 335 nm, and the emission wavelength was 430 nm. Therefore, the FRET channel was selected with an excitation wavelength of 335 nm and an emission wavelength of 430 nm. FRET efficiencies were calculated according to Wallrabe and Periasamy (18). In addition, spectra for both excitation wavelengths were recorded for an emission from 300 to 500 nm. Experiments with purified NOsGC were performed in the presence and absence of DEA/NO (100 M).
Photometric Measurements-Absorption measurements were carried out on a Varian photometer at 37°C. The same buffer and concentration of purified NOsGC were used as for the spectrofluorometric measurements. Absorption was recorded from 200 -600 nm.
NOsGC Activity Assay-NOsGC activity was quantified by the formation of [␣-32 P]cGMP from [␣-32 P]GTP, as described by Ref. 19. The activity of 50 ng of purified enzyme was determined in a total volume of 100 l in the presence of 50 mM triethanolamine/HCl buffer, pH 7.4, 1 mM 3-isobutyl-1-methylxanthine, 3 mM MgCl 2 , 3 mM dithiothreitol, 5 mM creatine phosphate, 1 mM cyclic GMP, 500 M GTP, [␣-32 P]GTP, and 0.025 mg creatine phosphokinase. The reaction was started by the incubation at 37°C and was stopped after 10 min by adding 500 l of 125 mM zinc acetate and 500 l of 120 mM sodium carbonate leading to co-precipitation of zinc carbonate and 5Јnucleotides. The purification of the enzyme-formed cGMP was performed on short alumina columns as described by Ref. 19. Stimulated measurements were performed in the presence of BAY 41-8543 (100 M) and DEA/NO (100 M). For the dose-response curves, DEA/NO was used at a concentration ranging from 1 nM to 100 M. BAY 41-8543 was used at concentrations ranging from 1 nM to 100 M in the presence of DEA/NO (100 M).
SDS-PAGE Analysis-The SDS-PAGE analysis was performed as described in Ref. 15.
Statistical Analysis-The results are expressed as means Ϯ S.E. of at least three independent experiments. All results were controlled for their statistical significance by Student's t test. A value of p Ͻ 0.05 was considered to be statistically significant.

Fluorescence Resonance Energy Transfer between Wild-type
NOsGC and Mant-To confirm that 2Ј-Mant-3Ј-dGTP binds to NOsGC and can be used as a conformation-sensitive detector, purified NOsGC (␣ 1 S/␤ 1 , 3 M) was excited at 280 nm ( Fig.  2A) and 295 nm, which represents the tryptophan-specific . The appearance of this new maximum at 430 nm indicates that tyrosine and tryptophan residues are able to serve as FRET donors, whereas 2Ј-Mant-3Ј-dGTP acts as FRET acceptor. The resulting basal FRET efficiency reached 12.1 Ϯ 1.0% for an excitation at 280 nm and 5.0 Ϯ 0.4% for the tryptophanspecific excitation at 295 nm. NOsGC contains only five tryptophan residues. They are distributed over the four functional domains, providing the opportunity to study FRET between the substrate analog 2Ј-Mant-3Ј-dGTP and the specific tryptophan residues of the HNOX, PAS, coiled-coil, and catalytic region. Therefore, we decided to use tryptophan-specific excitation at 295 nm in all further FRET experiments.
Increase in FRET Efficiency between Tryptophans and the Mant Group upon Addition of DEA/NO-The addition of the NO-donor DEA/NO to NOsGC and 2Ј-Mant-3Ј-dGTP increased FRET efficiency by 2.7 Ϯ 0.1% (Fig. 3). The increase in FRET efficiency was significant. As a negative control, we used a mutant isoform of the ␤ 1 subunit (␣ 1 S/␤ 1 H105A), which does not increase its catalytic activity in the presence of NO (20). This catalytically NO-insensitive mutant was also NO-insensitive with respect to the observed increase in FRET efficiency (see Fig. 3). The data indicate that binding of NO to NOsGC leads to a conformational change that increases FRET efficiency between the substrate analog 2Ј-Mant-3Ј-dGTP and endogenous tryptophans. FRET efficiency increases when the distance between the donor fluorophore and the acceptor fluorophore decreases (21). Therefore, we hypothesized that one or more tryptophan residues move toward the substrate binding site upon activation by NO.  Mutations of Tryptophan-There are five tryptophan residues within rat NOsGC, and each could contribute to FRET under basal and NO-stimulated conditions (see Fig. 1). For purification purposes, each mutant contains a Strep-tag carboxylterminally to the ␣ 1 subunit that has an additional tryptophan residue. To identify the tryptophan residues involved in FRET, we mutated each of them to either the amino acids alanine (Ala) or phenylalanine (Phe).
Comparison of FRET Efficiency of Wild-type NOsGC and Mutants-Each of the generated five mutants lacked a single tryptophan and therefore a potential donor for FRET. Without this FRET donor, the basal FRET efficiency should be reduced if the corresponding tryptophan takes part in basal FRET. As expected, the FRET efficiency under basal conditions decreased in some tryptophan mutants (Fig. 4A).
The increase in FRET efficiency of the mutants after activation by NO should be considerably reduced if the correspond-ing tryptophan is responsible for the increase in FRET efficiency seen for the wild-type enzyme. The mutant of Trp-22 (W22F) of the ␤ 1 subunit and the mutants of Trp-669 (W669A) and Trp-352 (W352F) of the ␣ 1 subunit showed no significant difference, whereas two mutants stood out in comparison with the wild-type (Fig. 4B): the substitution of a phenylalanine for Trp-466 (W466F) of the ␣ 1 subunit led to a significant reduction in the presence of DEA/NO. This indicates that Trp-466 is likely responsible for the observed increase in FRET efficiency of the wild-type enzyme. The substitution of a phenylalanine for Trp-602 (W602F) in the ␤ 1 subunit led to a significant increase in FRET under NO-stimulated conditions. This was unexpected and will be discussed after the following paragraph.
Tryptophan 466 Is Necessary and Sufficient for NO-induced FRET Increase of Wild-type NOsGC-The previous experiments show that substitution of a phenylalanine for Trp-466 (W466F) leads to a significant loss of the NO-induced increase in FRET efficiency between tryptophans and 2Ј-Mant-3Ј-dGTP. To positively identify Trp-466 as the tryptophan responsible for the NO-induced increase in FRET efficiency, we left Trp-466 intact and mutated all other endogenous NOsGC tryptophan residues to either the amino acids alanine or phenylalanine (␣ 1 S-W352F,W669A/␤ 1 -W22F,W602F). After adding DEA/NO to the quadruple mutant, we were able to detect an increase in FRET efficiency, which equals the increase of the wild-type enzyme (see Fig. 4). Because Trp-466 is the only endogenous tryptophan in the quadruple mutant, the visible increase in FRET efficiency of this mutant and the wild-type enzyme can likely be traced back to Trp-466. A considerable participation and movement of the tryptophan in the Strep-tag after NO stimulation cannot be completely ruled out but is unlikely: the mutation of ␣ 1 Trp-669 only 23 amino acids upstream of the tryptophan in the Strep-tag does not show significant differences in FRET efficiency under basal or under NO-stimulated conditions. The data resulting from analysis of the quadruple mutant indicate that Trp-466 is not only required but is also sufficient for the visible increase in FRET efficiency. Because FRET efficiency increases, when the distance between the participating fluorophores decreases (21), it follows that Trp-466 of the ␣ 1 subunit moves toward the substrate binding site upon NO stimulation.
Interaction between Tryptophan 602 and Tryptophan 22-Even though the substitution of Trp-602 led to a decrease of FRET efficiency in comparison with the wild-type enzyme under basal conditions (see Fig. 4A), FRET efficiency increased under NO-stimulated conditions, much to our surprise. We therefore postulated that Trp-602 masks the movement of a tryptophan other than Trp-466 toward the Mant group. A candidate for this act is Trp-22 of ␤ 1 HNOX. We and others (5, 6) recently reported a spatial proximity of the catalytic domain and the HNOX domain, suggesting that Trp-22 in the ␤ 1 HNOX and Trp-602 in the ␤ 1 catalytic domain could indeed be close enough for an interaction. To positively identify Trp-22 as the tryptophan masked by Trp-602, we left Trp-466 and Trp-22 intact and mutated all other endogenous tryptophan residues to the amino acids alanine or phenylalanine (␣ 1 S-W352F,W669A/ ␤ 1 -W602F). In the presence of NO, the FRET efficiency of this triple mutant exceeded the value of the wild-type enzyme and reached the value of ␣ 1 S/␤ 1 -W602F. These results indicate that in the triple mutant, Trp-22 and Trp-466 move toward the substrate binding site upon activation by NO and cause an increase in FRET efficiency by 3.9 Ϯ 0.3% (see Fig. 4).
Comparison of the tryptophan emission maxima under basal conditions showed a shift to shorter wavelengths in the triple mutant containing only Trp-22 and Trp-466 (336.7 Ϯ 0.8 nm) opposed to the wild-type enzyme (340.5 Ϯ 1.0 nm). The emission of the quadruple mutant containing only Trp-466 revealed a small shift in the opposite direction to a maximum at 342.5 Ϯ 1.5 nm. From this, it follows that the tryptophan emission maximum of Trp-22 is significantly blueshifted in comparison with the other tryptophans. This is an important prerequisite for homo-FRET and provides a likely explanation for the observed interaction between Trp-22 and Trp-602 (see "Discussion").
Preserved NO Heme Binding in All Tryptophan Mutants, Including W22F and W466F Mutants-The heme absorbance spectra for the enzyme lacking Trp-22 (␣ 1 S/␤ 1 -W22F) or lacking Trp-466 (␣ 1 S-W466F/␤ 1 ) were measured in the absence and also in the presence of DEA/NO (Fig. 5A). The Soret peak of heme undergoes the typical shift from 430 nm under basal conditions to 399 nm under NO-stimulated conditions (BAY 41-8543). Thus, the absence or presence of Trp-22 or Trp-466 neither influences the binding of heme to NOsGC nor interferes with the binding of NO to the heme group. The same is true for all other tryptophan mutants used in this study (data not shown). Fig. 5B shows SDS-PAGE analysis of the W22F and W466F mutants. There were no apparent differences in purity between the wild-type enzyme and all other enzyme mutants used in this study (data not shown). Table 1 provides information on enzyme activity measurements under basal, NO-stimulated and NO plus ciguat-stimulated conditions. All tryptophan mutants used in this study showed significant activation by NO and significant activation in the presence of ciguat plus NO. Activity per mg protein under basal and NO-stimulated conditions was lowest for the W466F mutant. This was not due to lower purity of the enzyme preparations as controlled by SDS-PAGE analysis (see Fig. 5B). Much to our surprise, the addition of BAY 41-8543 in addition to DEA/NO had the greatest effect on the W466F mutant. As seen in Fig. 6A, NO activated both the ␣ 1 S-W352F,W669A/␤ 1 -W22F,W602F mutant and wild-type NOsGC by 80 -100-fold, whereas the   (Fig. 6B), increased enzyme activity 2-fold in the wild-type enzyme and in the ␣ 1 S-W352F,W669A/␤ 1 -W22F,W602F mutant, whereas BAY 41-8543 increased the activity of ␣ 1 S-W466F/␤ 1 Ͼ6-fold over NO-stimulated activity. This approaches the level of activation elicited by DEA/NO in the wild-type enzyme.

DISCUSSION
In the current study, we measured fluorescence resonance energy transfer from tryptophan residues of full-length guanylate cyclase to the substrate analog 2Ј-Mant-3Ј-dGTP under basal and NO-stimulated conditions. Our results indicate that NO binding to the amino-terminal ␤ 1 HNOX domain is transmitted to the carboxyl-terminal catalytic domain both through the coiled-coil helices and by direct interdomain signal transmission between the ␤ 1 HNOX domain and the catalytic domain.
The Role of Trp-22 in the ␤ 1 HNOX Domain-Trp-22 of the ␤ 1 subunit is located in the ␣B helix of the HNOX domain according to the crystal structure of Nostoc sp. PCC 7120, a cyanobacterial HNOX homolog (22). The authors show that the binding of NO initially leads to a six-coordinated NO-heme state, which finally passes into a five-coordinated NO-heme state. This is accompanied by a severe distortion of the heme leading to an extensive conformational change of the amino terminus. In this process, helix ␣B containing Trp-22 rotates for ϳ20° (22). In the crystal structure of the HNOX domain derived from Thermoanaerobacter tengcongenesis, Olea et al. (23) show an NO-induced shift of the ␣B helix of 4.9 Å. Our data indicate that this very movement of the helix containing Trp-22 brings it closer to the catalytic domain and the Mant group. This is consistent with the idea first suggested by Winger and Marletta that the NO activation signal is transmitted via a direct interaction between the ␤ 1 HNOX domain and the catalytic domain (5).

TABLE 1 Activity data of NOsGC mutants
The first three columns of the table present the specific activity mol ϫ min Ϫ1 ϫ mg Ϫ1 of NOsGC wild-type enzyme and the mutants under basal conditions and in the presence of DEA/NO (100 M) or BAY 41-8543 and DEA/NO (both 100 M). The results are expressed as means Ϯ S.E. of at least three independent experiments. The next two columns give the values for the x-fold stimulation of basal activity by DEA/NO or BAY 41-8543 plus DEA/NO. Additionally, the x-fold activation of NO-stimulated activity by BAY 41-8543 is shown. The last three columns present percent activity of the mutants compared with wild-type enzyme.

Nature of the Trp-22 and Trp-602
Interaction-The movement of Trp-22 in the wild-type enzyme as detected by FRET is masked by an interaction with Trp-602. A likely explanation for the quenching effect is the occurrence of homo-FRET (17). Homo-FRET occurs when there is considerable overlap between the emission and absorbance of the same type of fluorophore. This is generally not the case for tryptophans unless the microenvironment of one tryptophan causes a shift in the emission spectrum. Our data confirm that Trp-22 shows a blueshifted emission in comparison with the other tryptophan residues (see "Results"). This is consistent with a more unpolar microenvironment within the heme-binding HNOX domain. The blueshift leads to greater overlap of the respective spectra that is a prerequisite for homo-FRET of tryptophans. This strongly supports the idea that homo-FRET occurs between tryptophans 22 and 602. The homo-FRET interaction between Trp-602 of the catalytic region and Trp-22 of the HNOX domain provides additional evidence for an interaction between the ␤ 1 HNOX domain and the catalytic domain.
The Coiled-coil Functions as Signaling Helix-In analogy to the crystallized ␤ 1 coiled-coil, Trp-466 is located in a short helix (␣B) behind the long amphipathic helix (␣A) of the coiled-coil domain (24). Based on comparative genomics, this domain has been suggested to act as a signaling helix that transmits the flow of signals between modules in diverse multi-domain signaling proteins (25). Our experimental data fully support the prediction that the coiled-coil functions as a signaling helix.
Comparison with Existing Models of NOsGC-Fritz et al. (26) examined a carboxyl-terminally truncated NOsGC from Manduca sexta (tobacco hornworm) using analytical ultracentrifugation, small angle x-ray scattering, cross-linking, and tandem mass spectrometry. They found 20 intramolecular contacts and hypothesized a model with a central parallel coiled-coil domain upon which the HNOX and PAS domains are assembled. Our data are consistent with the model proposed by Fritz et al. Fig.  7 shows the resulting model where we fitted the catalytic domain beneath the central coiled-coil domain in close proximity to the ␤ 1 HNOX and the carboxyl terminus of ␣ 1 coiledcoil domain.
Model of NO Signal Transmission Based on our FRET Data-Based on the crystal structure of the free and NO-bound HNOX domain from a cyanobacterial homolog, it has been suggested that NO binding induces a rotational shift of the helix ␣B containing Trp-22 due to heme bending and a shift of the helix ␣F away from the heme due to breakage of the bond between its histidine residue 105 and the heme iron (22). The NO-induced movement of helix ␣B containing Trp-22 can easily be applied to our findings because we provide evidence for a direct approximation of Trp-22 in the ␣B helix to the catalytic domain. The NO-induced movement of the helix ␣F containing histidine 105 is likely transferred to the second short helix of the coiled-coil domain of the ␣ 1 subunit, which contains Trp-466. This transfer could be mediated via the ␣ 1 PAS domain. In agreement with this thought, Underbakke et al. (27) propose an interaction between the ␣F helix of the HNOX domain with the PAS domain, and Fritz et al. (26) found that the ␣ 1 PAS domain is in contact with the ␤ 1 HNOX domain. The central importance of the ␣ 1 PAS domain for the signal transmission of NO is also underlined by previous findings from our group that in contrast to the ␣ 1 HNOX domain, ␣ 1 PAS is necessary for the intramolecular transmission of the NO activation signal (28).
Ciguat Hypersensitivity of the ␣ 1 S-W466F/␤ 1 Mutant-In contrast to the deletion mutant of the ␣ 1 PAS domain that abrogates both stimulation by NO and ciguat stimulators (28), the ␣ 1 S-W466F mutation had a peculiar differential influence on NO versus NO plus ciguat stimulation. Yoo et al. (29) suggested that the influence of the ciguat stimulator, BAY 41-2272, is the same for full-length NOsGC and a truncated ␤ 1 (1-200) HNOX domain. Consequently, it was concluded that NOsGC stimulators bind to the HNOX domain of ␤ 1 . Recent evidence indicates that ciguat stimulators relieve allosteric inhibition of the HNOX domain of ␤ 1 by the ␣ 1 PAS domain thereby enhancing NO binding (26,30). The differential influence of the ␣ 1 S-W466F mutation on ciguat/NO stimulation can be accommodated in such an allostery model where signal transmission from the HNOX domain of ␤ 1 via the ␣ 1 PAS domain and the coiled-coil region of ␣ 1 to the catalytic domain is not unidirectional. This is consistent with data that argue in favor of reciprocal communication between the catalytic and NO-binding domain (31).
Summary-In summary, we propose a model of NO activation where the movement of the ␣B helix of the ␤ 1 HNOX domain containing Trp-22 interacts directly with the catalytic domain, whereas the movement of the signaling helix containing His-105 is indirectly transmitted to the catalytic domain via the ␣ 1 PAS domain and ␣ 1 coiled-coil domain. This is proposed to allow the short helix of the coiled-coil domain in ␣ 1 containing Trp-466 and the ␣B helix of the ␤ 1 HNOX domain containing Trp-22 to form a pair of tongs forcing the catalytic domain into the nitric oxide-activated conformation.