(Received for publication, August 26, 1996)
From the Vascular Biology Center, Departments of Pediatrics and of Pharmacology and Toxicology, Medical College of Georgia, Augusta, Georgia 30912
Endothelial nitric-oxide synthase (eNOS) is comprised of two identical subunits. Each subunit has a bidomain structure consisting of an N-terminal oxygenase domain containing heme and tetrahydrobiopterin (BH4) and a C-terminal reductase domain containing binding sites for FAD, FMN, and NADPH. Each subunit is also myristoylated and contains a calmodulin (CaM)-binding site located between the oxygenase and reductase domains. In this study, wild-type and mutant forms of eNOS have been expressed in a baculovirus system, and the quaternary structure of the purified enzymes has been analyzed by low temperature SDS-PAGE. eNOS dimer formation requires incorporation of the heme prosthetic group but does not require myristoylation or CaM or BH4 binding. In order to identify domains of eNOS involved in subunit interactions, we have also expressed eNOS oxygenase and reductase domain fusion proteins in a yeast two-hybrid system. Corresponding human neuronal NOS (nNOS) and murine inducible NOS (iNOS) fusion proteins have also been expressed. Comparative analysis of NOS domain interactions shows that subunit association of eNOS and nNOS involves not only head to head interactions of oxygenase domains but also tail to tail interactions of reductase domains and head to tail interactions between oxygenase and reductase domains. In contrast, iNOS subunit association involves only oxygenase domain interactions.
Three distinct isoforms of nitric-oxide synthase
(NOS)1 have been identified in mammalian
tissues. Although none of these enzymes has an absolutely
tissue-specific pattern of expression, they are commonly referred to as
endothelial NOS (eNOS), neuronal NOS (nNOS), and macrophage or
inducible NOS (iNOS). eNOS, nNOS, and iNOS catalyze the oxidation of
L-arginine to produce NO and L-citrulline via a
similar or identical reaction mechanism involving several cofactors or
prosthetic groups (1). In accord with their common catalytic function,
the NOS enzymes possess many common features including 50-60% amino
acid sequence identity and an 2 quaternary structure
(2). In addition, all three types of NOS monomers have a bidomain
structure consisting of an N-terminal oxygenase domain that contains
iron protoporphyrin IX (heme) and tetrahydrobiopterin (BH4)
and binds L-arginine and a C-terminal reductase domain that contains binding sites for FAD, FMN, and NADPH (3, 4, 5, 6). Each domain can
exist and function independently. The isolated oxygenase domain of iNOS
can thus form dimers while the isolated reductase domain catalyzes
cytochrome c reduction at a rate equivalent to that of
native dimeric iNOS (4). The isolated oxygenase and reductase domains
of eNOS can be reconstituted in vitro to catalyze production
of NO and L-citrulline from L-arginine (6). The
three NOS enzymes, therefore, have many similarities in structure and
catalytic function. However, because each of the enzymes has a
different physiological role and tissue distribution, the molecular mechanisms for regulation of eNOS, nNOS, and iNOS can differ
significantly (7).
All three NOS isoforms are dimeric enzymes comprised of two identical subunits. iNOS and nNOS are catalytically active only in dimeric form (8, 9, 10, 11, 12, 13, 14, 15). Regulation of NOS subunit interactions could, therefore, provide a mechanism for modulation of enzyme activity in vivo. The cofactors, prosthetic groups, domains, and amino acid residues of iNOS important for subunit interactions have been studied in detail (4, 9, 12, 13, 14, 15, 16, 17). Certain features of eNOS and nNOS oligomerization have also been investigated (10, 18, 19, 20). Studies of eNOS suggest that this isoform may be different from the other NOS isoforms in terms of its requirements for dimer formation. For example, whereas all of the determinants for iNOS dimerization are thought to be contained in the oxygenase domain of the enzyme (4, 16, 17), eNOS dimer formation has been reported to involve both oxygenase and reductase domains (18). Moreover, while it is now well established that binding of BH4 plays a critical role in formation of the iNOS dimer (8, 9, 12, 13, 14), recent evidence suggests that BH4 may not be required for eNOS dimer formation (20).
To date, a comprehensive investigation of the cofactors, prosthetic groups, domains, and amino acid residues of eNOS involved in oligomerization has not been carried out. Furthermore, conclusions about the differences and similarities in dimerization requirements of NOS isoforms can currently be made based only on individual studies of a single isoform. Comparative analysis of all three isoforms in the same experimental model system has not been performed. In this study, therefore, we have investigated eNOS dimerization requirements by expression and purification of wild-type and mutant forms of the bovine enzyme in a baculovirus/Sf9 insect cell system. In addition, we have investigated interactions of eNOS oxygenase and reductase domains in a yeast two-hybrid system. Human nNOS and murine iNOS have been expressed in the same two systems allowing direct comparisons to be made of all three NOS isoforms.
Sf9 insect cells, baculovirus transfer vector
pVL1393, and BaculogoldTM viral DNA were obtained from
Pharmingen (San Diego, CA). Bovine aortic endothelial cells (BAEC) were
purchased from Cell Systems Inc. (Kirkland, WA). Monoclonal antibodies
to eNOS and iNOS were purchased from Transduction Laboratories
(Lexington, KY). AG 50W-X8 cation exchange resin was obtained from
Bio-Rad, and L-[14C]arginine and ECL reagents
were purchased from Amersham Corp. 2,5
-ADP-Sepharose was from
Pharmacia Biotech Inc. pGBT9 (DNA binding domain hybrid cloning
vector), pGAD424 (activation domain hybrid cloning vector), and
Saccharomyces cerevisiae SFY526 were purchased from Clontech
(Palo Alto, CA). Chlorophenol red-
-D-galactopyranoside came from Boehringer Mannheim and
(6R)-5,6,7,8,-tetrahydro-L-biopterin came from Research
Biochemicals International. Oligonucleotide primers for PCR, Protein A
and G agarose and immunoprecipitin were purchased from Life
Technologies, Inc.
Baculovirus pVL1393 plasmid transfer
vectors encoding wild-type bovine eNOS, wild-type murine iNOS,
wild-type human nNOS, (myr) eNOS, and
CaM eNOS have been described
previously (21, 22). The (
heme) eNOS mutant in pVL1393 was created by
mutating the cysteine 186 codon (TGC) in the wild-type bovine eNOS
cDNA to an alanine codon (GCC) using the PCR-based splicing by
overlap extension technique (23). cDNA constructs encoding hybrids
of the NOS oxygenase and reductase domains and the GAL4 DNA binding and
activation domains were created by subcloning into the
shuttle/expression vectors, pGBT9 and pGAD424 (Clontech). DNA sequences
encoding bovine eNOS residues 1-505 and 506-1205, murine iNOS residues 1-498 and 499-1144, and human nNOS residues 1-744, 239-744, and 745-1433 were generated by PCR amplification of (
myr) eNOS, wild-type iNOS, and wild-type nNOS full-length cDNAs, respectively. PCR primers were designed to incorporate 5
EcoRI and
SalI restriction sites into amplified products for
subcloning. G442A and A445I point mutations in eNOS fusion constructs
were created using the overlap extension technique to replace the
glycine 442 (GGC) codon and the alanine 445 (GCC) codon with alanine
(GCC) and isoleucine (ATC) codons, respectively. G450A and A453I
mutants of iNOS fusion constructs replaced glycine 450 (GGC) with
alanine (GCC) and alanine 453 (GCA) with isoleucine (ATA). All DNA
constructs were sequenced in the Molecular Biology Core Facility of the
Institute for Molecular Medicine and Genetics, Medical College of
Georgia, using a Perkin-Elmer ABI 377 automated DNA sequencer. Sequence
analysis confirmed that only the desired mutations were incorporated
into the various constructs and that in-frame fusions were created of
sequences encoding the hybrid proteins.
Expression of NOS proteins in the baculovirus/Sf9 insect
cell system and purification of the proteins by 2,5
-ADP-Sepharose was
carried out as described previously (21, 22). Enzyme activity was
determined by monitoring the rate of formation of
L-[14C]citrulline from
L-[14C]arginine under the conditions
described previously (21).
Purified enzymes (1-5 µg) were incubated for 10 min at 37 °C in the presence or absence of various cofactors. 2 × SDS sample buffer (0.5 M Tris-HCl, pH 6.8, 6% SDS, 30% glycerol, 14% (v/v) 2-mercaptoethanol, and 0.0025% bromphenol blue) was added, and samples were incubated for a further 30 min at 0, 20, 30, 40, 50, and 60 °C. Samples were loaded on 6.0 or 7.5% polyacrylamide gels and subjected to electrophoresis at a constant current of 30 mA. Gels and buffers were cooled to 4 °C prior to electrophoresis. Gels were also run in a refrigerated cold box in order to maintain the temperature of the gel below 15 °C. Migration of proteins on gels was visualized by Coomassie staining or by immunoblotting with anti-NOS antibodies.
Immunoprecipitation and ImmunoblottingSf9 cells were coinfected with baculovirus constructs encoding eNOS and iNOS. After three days of infection, cells were lysed in ice-cold RIPA buffer (2 ml) containing 20 mM Tris-HCl, pH 7.4, 2.5 mM EDTA, 1% Triton X-100, 1% sodium deoxycholate, 0.1% SDS, 1% phenylmethylsulfonyl flouride, 10 µg/ml leupeptin, 10 µg/ml pepstatin A, and 5 µg/ml aprotinin. Lysates were centrifuged at 10,000 × g for 20 min to remove insoluble material. 1 ml of lysate was precleared with 10 µl of 50% immunoprecipitin for 1 h at 4 °C. Samples of lysate from the eNOS/iNOS coinfection were subjected to immunoprecipitation with either anti-eNOS or anti-iNOS antibodies. Proteins precipitated by anti-eNOS were separated by gel electrophoresis, transferred to nitrocellulose membranes by electroblotting, and immunoblotted with anti-iNOS. Proteins precipitated by anti-iNOS were immunoblotted with anti-eNOS. Bound antibody was visualized by the ECL chemiluminescent detection system and autoradiography.
Transformation of Yeast andS. cerevisiae strain SFY526 was cotransformed
by the lithium acetate method (24) with various pairwise combinations
of pGBT9 and pGAD424 fusion plasmids. Transformants were grown on
plates lacking tryptophan and leucine to select for the presence of the pGBT9 and pGAD424 derivatives, respectively. 3-4 days after
transformation, cells were assayed for -galactosidase activity by
the colony lift filter assay method (24). Reporter gene expression was also determined by liquid culture assay using chlorophenol
red-
-D-galactopyranoside as substrate (24). Assays were
performed in triplicate, and the specific
-galactosidase activity
was calculated by the method of Miller (25). All DNA-binding domain and
activation domain fusion constructs were confirmed not to activate
reporter gene transcription by themselves, and all activation domain
fusion constructs were confirmed not to activate transcription when
combined with the unrelated pLAM 5
(human lamin C-(66-230) in
pGBT9).
The eNOS protein has been
shown previously to elute anomalously from gel filtration columns (26),
a property that precludes analysis of eNOS quaternary structure by
conventional means. Like nNOS and iNOS, however, eNOS has the capacity
to oligomerize (18). Moreover, the eNOS oligomer is a dimer rather than
a higher order oligomer as shown recently by Rodríguez-Crespo
et al. (20) using LT-PAGE. In this previous study (20),
bovine eNOS was overexpressed in Escherichia coli where it
was found in a 50:50% monomer-dimer equilibrium. It is not clear,
however, whether such an equilibrium exists when the enzyme is
expressed in a eukaryotic expression system or when naturally expressed
in endothelial cells. To address this question, we have expressed
wild-type bovine eNOS in a eukaryotic baculovirus/Sf9 insect cell
expression system and purified the enzyme to >95% homogeneity by
affinity chromatography on 2,5
-ADP-Sepharose. Purified protein was
suspended in SDS sample buffer (to a final concentration of 3% SDS and
7% 2-mercaptoethanol) and incubated for 30 min at 0, 20, 30, 40, 50, and 60 °C. Dimeric and monomeric forms of the enzyme were then
separated by LT-PAGE and visualized on gels by Coomassie staining. As
shown in Fig. 1A, eNOS migrated on LT-PAGE
almost entirely as a dimer if samples were not heated before running
the gel. The critical temperature for subunit dissociation under these
denaturing conditions was 30-40 °C. In contrast to the prokaryotic
expression system (20), therefore, expression of eNOS in eukaryotic
cells results in close to 100% of the enzyme forming stable,
SDS-resistant homodimers. Furthermore, eNOS is found entirely in
dimeric form, not only when expressed and purified from the baculovirus
system but also when naturally expressed in endothelial cells. BAEC
lysates were also analyzed by LT-PAGE. Monomeric and dimeric eNOS
expressed in BAEC were visualized on LT-PAGE by immunoblotting with
anti-eNOS antibody. As shown in Fig. 1B, eNOS in BAEC exists
under basal conditions exclusively in dimeric form. It is unlikely,
therefore, that cofactor or substrate induction of dimer formation
functions as a regulatory mechanism for increasing eNOS activity in
endothelial cells. In this respect, eNOS differs from iNOS, which is
50-75% monomeric in macrophages (9, 14) and is thus thought to be regulated in part by factors that promote dimer assembly (9).
A previous report by Klatt et al. (10) has shown that
BH4 and L-arginine synergistically convert
purified porcine nNOS from a monomeric to dimeric form. In addition,
cofactor and amino acid substrate binding together increase the
stability of the dimer in a cooperative manner. To determine whether
dimeric eNOS is similarly stabilized by these two effectors, purified
eNOS enzyme was preincubated with either BH4 (0.1 mM) or L-arginine (1 mM) alone or
the combination of the two compounds. Preincubated proteins were then
suspended in SDS sample buffer and incubated for a further 30 min at 0, 20, 30, 40, 50, and 60 °C. As shown in Fig. 2,
preincubation of eNOS with BH4 stabilized the dimer,
increasing the critical temperature for dissociation from 30-40 to
40-50 °C. However, in contrast to what has been reported previously
for porcine nNOS (10), L-arginine alone had no detectable
effect on dimer stability nor did it enhance the effect of
BH4 on stability. Other enzyme cofactors including
Ca2+/CaM (200 units), FAD (4 µM), FMN (4 µM), NADPH (1 mM), and hemin chloride (4 µM) were also tested for effects on dimer stability. None
of these factors had any detectable effect on the critical temperature
for dimer dissociation indicating that BH4 is the only
cofactor that alters the stability of the eNOS oligomer.
The lack of effect of L-arginine on eNOS dimer stability
represents a true structural difference between eNOS and nNOS and is
not an artifact of baculovirus expression, as determined by experiments
with baculovirus-expressed human nNOS. Wild-type human nNOS was
expressed in the baculovirus system under the same conditions used to
express eNOS and was purified to >95% homogeneity by affinity chromatography on 2,5
-ADP-Sepharose. Analysis of nNOS dimer stability
by LT-PAGE showed that, in the absence of preincubation with
BH4 and L-arginine, the purified nNOS enzyme
existed in a 60:40% monomer-dimer equilibrium (Fig.
3A). Preincubation of the enzyme with either
L-arginine (1 mM) or BH4 (0.1 mM) increased both the amount of the nNOS dimer and the
critical temperature for nNOS subunit dissociation (Fig. 3,
B and C). Preincubation with both compounds
together stabilized the dimer to a greater extent than either alone
(Fig. 3D). Human nNOS purified from the baculovirus system,
therefore, is stabilized by both BH4 and
L-arginine in an identical manner to nNOS purified from
porcine brain (10).
Wild-type murine iNOS was also expressed in the baculovirus system,
purified to >90% homogeneity by 2,5
-ADP-Sepharose, and analyzed by
LT-PAGE. Under certain denaturing conditions, iNOS has been found to
migrate as a dimer on LT-PAGE (15). Under the conditions used in the
present study, however, purified iNOS migrated on LT-PAGE exclusively
as a monomer. Failure to detect dimeric iNOS on gels was probably due
to both subunit dissociation during purification and to inability of
the purified dimer to remain intact in denaturing sample buffer
containing 3% SDS. That the enzyme was purified in at least partially
dimeric form is indicated by our finding that purified enzyme had
significant catalytic activity (~300 nmol of citrulline
produced/mg/min) prior to suspension in denaturing buffer. Monomeric
iNOS has been shown previously to be completely inactive (8, 9,
12, 13, 14, 15). Dissociation of the iNOS dimer in SDS sample buffer is
suggested further by our failure to detect dimeric iNOS on LT-PAGE even
after preincubation of the purified enzyme with the combination of
L-arginine (1 mM), BH4 (0.1 mM), and hemin chloride (4 µM), conditions
that have been shown previously to induce iNOS dimer formation in
nondenaturing buffers (9).
Expression of iNOS in the same eukaryotic expression system as eNOS and nNOS demonstrates that the iNOS dimer is the least stable of the NOS dimers. This is consistent with previous reports that iNOS loses its heme prosthetic group and dissociates into inactive monomers in the absence of BH4 and L-arginine (8, 9). Under the same conditions, nNOS and eNOS retain their dimeric structure (10, 19, 20). However, because a significant portion of the nNOS oligomer (but not the eNOS oligomer) dissociates either during purification or upon suspension in SDS sample buffer and because the eNOS dimer has a higher critical temperature for dissociation than the nNOS dimer has, we conclude that the order of stability of NOS oligomers is eNOS > nNOS > iNOS.
Quaternary Structure of Mutant Forms of eNOS Expressed and Purified from a Baculovirus SystemOnly BH4 (of all eNOS
cofactors, prosthetic groups, and substrates) stabilizes the eNOS dimer
after it has been formed. Certain ones of these factors, however, may
be necessary for assembly of the dimer from its monomeric subunits
in vivo. To gain further insight into which factors are
involved in dimer assembly, we have expressed several mutant forms of
eNOS in the baculovirus system. Expressed proteins were purified by
2,5
-ADP-Sepharose and analyzed by LT-PAGE. In a recent report,
Hellerman and Solomonson (27) have concluded that binding of
Ca2+/CaM by eNOS is a requirement for enzyme dimerization.
In the present study, however, we have found that eNOS purified from the baculovirus system is 98% dimeric. Because the protein was purified under conditions (2 mM EGTA) that yield an enzyme
that is 100% dependent on exogenous Ca2+/CaM for activity
(21, 22), it is unlikely that the purified dimer contains any bound
CaM. CaM binding, therefore, appears not to be a prerequisite for
dimerization. In order to confirm this conclusion, we have expressed a
CaM mutant of bovine eNOS in the baculovirus system. This protein,
which has been characterized previously (21), lacks a CaM-binding
domain because residues 493-512 have been deleted from the cDNA
coding sequence.
CaM eNOS was purified and analyzed by LT-PAGE. Like
wild-type eNOS,
CaM eNOS migrated on LT-PAGE in 98% dimeric form
(Table I). The critical temperature for dissociation of
the mutant dimer was 30-40 °C.
|
Two additional eNOS mutants were expressed in the baculovirus system
and analyzed by LT-PAGE. A myristoylation-deficient mutant of bovine
eNOS, designated (myr) eNOS, has also been characterized previously
(21). This mutant, in which glycine 2 has been mutated to an alanine,
differs from wild-type eNOS in that it is neither myristoylated nor
palmitoylated and, consequently, is not membrane-associated (21, 28,
29). Like wild-type eNOS, purified (
myr) eNOS migrated on LT-PAGE in
98% dimeric form with a critical temperature for subunit dissociation
of 30-40 °C (Table I). Neither fatty acylation nor membrane
association of eNOS, therefore, appears to be required for dimer
formation. A final mutant form of bovine eNOS to be analyzed was
designated (
heme) eNOS. In this expressed protein, we have changed
the cysteine 186 codon (TGC) to an alanine (GCC). Cysteine 186 of
bovine eNOS is equivalent to the cysteine 184 heme ligand of human
eNOS. Mutation of this residue has been shown to result in loss of
incorporation into eNOS of the heme prosthetic group (30). Klatt
et al. (19) have recently shown that heme-deficient
wild-type nNOS is unable to form dimers. These authors concluded that
incorporation of the heme prosthetic group into nNOS is a requisite for
dimerization. In the present study, (
heme) eNOS expressed and
purified from the baculovirus system was also found to exist
exclusively in monomeric form when analyzed by LT-PAGE (Table I).
Incorporation of the heme prosthetic group, therefore, appears to be a
requirement for dimerization not only of nNOS but also of eNOS.
Bovine eNOS expressed in E. coli lacks the posttranslational modifications of the native enzyme and is BH4-free. This purified enzyme, however, migrates on LT-PAGE in 50% dimeric form (20). It has been concluded that BH4 binding is not required for eNOS dimer formation and that eNOS is thus fundamentally different from both iNOS and nNOS (20). Whether BH4-independent eNOS dimer formation occurs with native eNOS or whether this previous observation is an artifact of prokaryotic expression is not clear. We have, therefore, examined the BH4 dependence of eNOS dimerization in the baculovirus expression system, where eukaryotic posttranslational modifications such as fatty acylation and phosphorylation are known to occur. Because the BH4 binding site of eNOS has not yet been identified, expression of a BH4-free mutant of eNOS in the baculovirus system was not feasible. In order to manipulate the BH4 content of eNOS, we expressed the wild-type protein in the absence or presence of 10 mM 2,4-diamino-6-hydroxypyrimidine (DAHP), an inhibitor of GTP cyclohydrolase I, the rate-limiting enzyme in BH4 biosynthesis (31). It has been shown previously that DAHP treatment of Sf9 cells expressing rat nNOS results in a reduction of the BH4 content of the purified enzyme from 0.47 to 0.07 mol of BH4/mol of subunit. Reduction of BH4 content was correlated with a proportional decrease in the specific activity of the enzyme (32). Other investigators have also reported that activities of purified NOS enzymes are directly proportional to the amount of bound BH4 with full activity requiring 1 mol of BH4/mol of subunit (6, 33). In the present and previous (21) studies, purified eNOS was found to be 45-50% independent of exogenous BH4 for activity. The purified enzyme expressed in the absence of DAHP, therefore, contains 0.45-0.50 mol of bound BH4/mol of subunit. However, when the enzyme was expressed in the presence of DAHP, the purified protein was found to have only 3% of full activity in the absence of exogenously added BH4, indicating that this enzyme preparation was virtually BH4-free. Analysis of the BH4-free enzyme on LT-PAGE showed that it was 98% dimeric (Table I). Thus, BH4 binding is not required for eNOS dimer formation in the baculovirus system. Similar conclusions have been reported by Rodríguez-Crespo et al. (20) following expression of the enzyme in an E. coli expression system. These authors concluded further that eNOS is unique in this respect as compared with both iNOS and nNOS. In order to determine whether the BH4 requirements for nNOS dimer formation are more similar to those of eNOS or to those of iNOS, we have expressed human nNOS in Sf9 cells in the absence and presence of DAHP. Activity of nNOS expressed without the inhibitor was 55% BH4-independent while nNOS expressed in DAHP-treated cells was only 2% independent of BH4 for activity, indicating that this enzyme preparation was virtually BH4-free. Both enzymes, however, migrated on LT-PAGE in an identical 60:40% monomer-dimer equilibrium. Thus, although BH4 promotes nNOS dimerization in vitro (Fig. 3), it is not required for dimer formation in situ. It appears that nNOS (like eNOS), differs significantly from iNOS, which has an absolute dependence on BH4 for oligomerization (8, 9, 12, 13, 14).
Interactions of eNOS, nNOS, and iNOS Oxygenase and Reductase Domains in a Yeast Two-hybrid SystemPrevious studies have
concluded that all of the determinants for iNOS dimer formation are
contained in the oxygenase domain of the enzyme (4, 16, 17). However,
evidence has been presented for eNOS that suggests that both the
N-terminal oxygenase domain and the C-terminal reductase domain are
involved in dimerization (20). At present, it is not known whether
these divergent results reflect intrinsic differences between iNOS and
eNOS oligomerization or whether they are due to differences in
experimental approach. In order to gain additional insight into which
domains of the NOS isoforms contribute to subunit interactions, we have
utilized the yeast two-hybrid system developed originally by Fields and Song (34). The two-hybrid system takes advantage of the modular nature
of the yeast GAL4 transcriptional activator. The GAL4 protein consists
of a site-specific DNA-binding domain that is distinct from the domain
responsible for transcriptional activation. Various proteins are
expressed in the two-hybrid system as fusions (or hybrids) with either
the GAL4 DNA-binding domain or the GAL4 activation domain. The capacity
of the two fusion proteins to interact is determined by cotranformation
into a strain of S. cerevisiae, which contains an integrated
copy of a lacZ reporter gene. If the two proteins interact,
the two domains of GAL4 are brought into close physical proximity,
resulting in reconstitution of GAL4 activity and -galactosidase
reporter gene transcription.
GAL4 DNA-binding domain and activation domain fusion plasmids were
constructed of the eNOS, iNOS, and nNOS oxygenase and reductase domains
using the shuttle/expression vectors, pGBT9 and pGAD424. Various
pairwise combinations of plasmid constructs were then introduced into
the yeast strain, SFY526. Interactions of fusion proteins in
vivo were first determined by -galactosidase activity assay of
cotransformants by a colony lift filter assay using X-Gal as substrate.
Fusion proteins that interact in this system give a positive (blue)
signal on filters. Fusion proteins that do not interact give a negative
(white) signal. The strength of the two-hybrid interaction was
quantitated further by liquid culture assay using chlorophenol
red-
-D-galactopyranoside as substrate. As shown in Table
II, eNOS oxygenase domain (residues 1-505) fusion
proteins (fused to either the GAL4 DNA-binding domain or the GAL4
activation domain) interacted strongly in the two-hybrid system due to
hemidimer formation. Strong interactions were also detected between
both of two different combinations of eNOS oxygenase domain and the eNOS reductase domain (residues 506-1205) hybrids. Weaker but significant interactions were detected between pairs of eNOS C-terminal reductase domain fusion proteins. However, in marked contrast to the
results with eNOS hybrids, iNOS oxygenase domain (residues 1-498) and
reductase domain (residues 499-1144) fusion proteins interacted in the
two-hybrid system only through head to head interactions of N-terminal
oxygenase domains (Table II). No head to tail or tail to tail
interactions were detected with iNOS hybrids. Differences between eNOS
and iNOS demonstrated in this system were not due to insufficient
concentrations of endogenous BH4 in yeast because identical
results were obtained when cells were grown on plates containing added
BH4 (0.1 mM).
|
When nNOS oxygenase domain (residues 1-744) and reductase domain
(residues 745-1433) fusions were tested in the two-hybrid system,
interactions were very similar to those detected for eNOS. nNOS
oxygenase and reductase domains interacted strongly in both head to
head and head to tail fashion and weakly in a tail to tail manner
(Table II). Interestingly, hybrids of the nNOS oxygenase domain
(residues 239-744), which lacked the nNOS N-terminal extension known
as the PDZ domain, did not interact in the two-hybrid system. The PDZ
domain of nNOS interacts with 1-syntrophin in the dystrophin complex
in skeletal muscle (35) and with the postsynaptic density protein,
PSD-95, in brain (36). The results of the present study suggest that
the PDZ domain may also be involved in nNOS dimer formation.
Alternatively, attachment of the PDZ domain to the nNOS oxygenase
domain may alter the folding or conformation of the oxygenase domain
and thereby affect dimer formation indirectly. Furthermore, our
comparative analysis of NOS oxygenase domain and reductase domain
interactions in the two-hybrid system provides an explanation for
differences in dimer stability of the NOS isoforms. eNOS and nNOS
dimers are very likely more stable than iNOS dimers due to more
extensive subunit interactions of the enzymes involving, not only head
to head interactions of oxygenase domains but also tail to tail
interactions of reductase domains and head to tail interactions between
oxygenase and reductase domains.
Within certain mammalian cell types, including cardiac myocytes (37) and microvascular endothelial cells (38), eNOS and iNOS are coexpressed. It has recently been speculated (18) that heterooligomerization of the two enzymes could provide a novel mechanism for regulation of NO production in vivo. Because eNOS and iNOS are 50-60% identical in primary structure (2) and because certain proteins with this degree of homology (for example, vascular endothelial and placenta growth factors (39)) are known to form functional heterodimers in situ, we have tested whether eNOS and iNOS subunits can form eNOS/iNOS heterodimers in Sf9 cells. eNOS and iNOS were co-expressed in the baculovirus system under conditions of high expression that is expected to favor heterodimer formation. After 3 days of co-infection, Sf9 cell lysates were immunoprecipitated with either anti-eNOS or anti-iNOS antibodies. Proteins precipitated by anti-eNOS were separated by gel electrophoresis, transferred to nitrocellulose, and immunoblotted with anti-iNOS. Anti-iNOS immunoprecipitates were immunoblotted with anti-eNOS. Antibody directed against eNOS did not co-precipitate iNOS in these experiments, and antibody directed against iNOS did not co-precipitate eNOS. Many physiologically important protein-protein interactions, however, are too transient or too weak to be detected in co-immunoprecipitation experiments. Interactions of the known protein partners Ras and Raf, for example, are not detectable by co-precipitation but are detectable in the yeast two-hybrid system (40). Therefore, we have also tested whether eNOS and iNOS oxygenase and reductase domains can form heterodimers in this system. eNOS/iNOS oxygenase domain hetero-hemidimer interactions produced positive (blue) signals in the two-hybrid colony lift filter assay. In liquid culture assays, the strength of the interaction was found to be approximately 50% of that of homo-hemidimer formation. Oxygenase domains of both isoforms are thus similar enough structurally to interact in vivo. However, no interactions were detected between eNOS and iNOS reductase domains and no hetero-hemidimer interactions were detected of the head to tail type that occur between eNOS oxygenase and reductase domains. Interactions of the eNOS polypeptide with itself (homodimer formation) are thus expected to be much stronger than those between eNOS and iNOS. Furthermore, because eNOS exists in intact cells in 100% dimeric form, it is unlikely that eNOS and iNOS form heterooligomers in vivo.
Amino Acid Residues of eNOS and iNOS Oxygenase Domains Involved in Subunit InteractionsMutational analysis by Cho et al.
(12) has shown that conservative amino acid substitutions at either
glycine 450 or alanine 453 of murine iNOS abolishes NO production,
dimer formation, and BH4 binding of the enzyme. These two
residues are conserved in all 10 reported NOS sequences including
mammalian eNOS, nNOS, and iNOS, as well as avian and insect NOS
enzymes. Significant homology of iNOS residues 448-480 to regions
within three different BH4-utilizing aromatic amino acid
hydroxylases has led to the conclusion that residues 450 and 453 of
iNOS are directly involved in binding of BH4. It has been
assumed that loss of dimer formation by mutation of either of these
residues is a direct consequence of loss of BH4 binding.
However, as demonstrated in the present study, eNOS does not require
BH4 for dimer formation. Therefore, we hypothesized that,
whereas mutation of Gly-450 or Ala-453 in iNOS oxygenase domain hybrids
should reduce or abolish interactions in the two-hybrid system,
mutation of equivalent residues in eNOS should be without effect. As
shown in Table III, Gly-450 and Ala-453 of murine iNOS
correspond to Gly-442 and Ala-445 of bovine eNOS. We therefore created
equivalent Gly Ala and Ala
Ile mutations in GAL4 activation
domain/NOS oxygenase domain hybrids of eNOS and iNOS and determined
whether there was an effect of mutation on interactions of the hybrid
proteins with the corresponding wild-type oxygenase domains in the
two-hybrid system. Each of the four mutations was found to
significantly reduce the strength of the oxygenase domain interactions
(Table IV). Because eNOS does not require
BH4 for dimer fomation, these results suggest that
site-specific mutation of these residues may affect dimer formation
directly, rather than indirectly due to loss of BH4 binding. The regions in eNOS and iNOS in which these residues are
located may thus represent an important subunit interface of the
enzymes that is involved in subunit-subunit interactions rather than in
subunit-BH4 interactions.
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