Howard Hughes Medical Institute (R.S., K.W.-S., U.G., B.K.K.),
Division of Cardiovascular Medicine (B.K.K.), Stanford University
Medical School, Stanford, California
The interaction of an agonist-bound G-protein-coupled receptor (GPCR)
with its cognate G-protein initiates a sequence of experimentally quantifiable changes in both the GPCR and G-protein. These include the
release of GDP from G
, the formation of a ternary
complex between the nucleotide-free G-protein and the GPCR, which has a
high affinity for agonist, followed by the binding of GTP to G, the dissociation of the GPCR/G-protein complex, and
the hydrolysis of GTP. The efficacy of an agonist is a measure of its
ability to activate this cascade. It has been proposed that efficacy
reflects the ability of the agonist to stabilize the active state of
the GPCR. We examined a series of 
2-adrenoceptor (2AR) agonists (weak partial agonists to full agonists)
for their efficacy at promoting two different steps of the G-protein
activation/deactivation cycle: stabilizing the ternary complex
(high-affinity, GTP-sensitive agonist binding), and steady-state GTPase
activity. We obtained results for the wild-type 2AR and
a constitutively active mutant of the 2AR
(2ARCAM) using fusion proteins between the
GPCRs and Gs to facilitate GPCR/G-protein interactions.
There was no correlation between efficacy of ligands in activating
GTPase and their ability to stabilize the ternary complex at
2ARCAM. Our results suggest that the GPCR
state that optimally promotes the GDP release and GTP binding is
different from the GPCR state that stabilizes the ternary complex. By
strongly stabilizing the ternary complex, certain partial agonists may
reduce the rate of G-protein turnover relative to a full agonist.
 |
Introduction |
Many
hormones and neurotransmitters exert their effects through GPCRs that
activate heterotrimeric G-proteins and, thereby, change the activity of
effector systems (Gilman, 1987
; Kobilka, 1992). Binding of an agonist
to a GPCR induces distinct conformational changes in the receptor
protein that enable GPCR to promote GDP release from
G (Wess, 1997; Gether and Kobilka, 1998). The agonist-occupied GPCR forms a high-affinity ternary complex with guanine nucleotide-free G (Kent et al., 1980;
Kobilka, 1992; Seifert et al., 1998a,b). Upon binding of GTP or the
hydrolysis-resistant GTP analog GTP
S to G,
the high-affinity ternary complex is disrupted, and both
G and
G
can regulate the
activity of effector systems (Kent et al., 1980; Gilman, 1987; Kobilka,
1992; Seifert et al., 1998b). G-protein deactivation is accomplished by
the GTPase activity of G (Gilman, 1987).
Several models have been developed to conceptualize the as yet
incompletely understood mechanisms of GPCR activation (for a historical
perspective, see Kenakin, 1996a; Colquhoun, 1998). The ternary complex
model of GPCR activation states that there is a correlation between the
efficacy of agonists at stabilizing the ternary complex and at
promoting multiple G-protein activation/deactivation cycles (Kent et
al., 1980). The ternary complex model has been elaborated into the
extended ternary complex model to explain the finding that GPCRs can
activate G-proteins even in the absence of agonist and that certain
receptor ligands, namely, inverse agonists, suppress G-protein
activation by agonist-free GPCRs (Costa and Herz, 1989; Lefkowitz et
al., 1993; Gether and Kobilka, 1998). The agonist-independent GPCR
activity is referred to as "constitutive activity". The extended
ternary complex model assumes that agonists stabilize GPCR in the
active (R*) state, while inverse agonists stabilize the inactive (R)
state. It has been proposed that for constitutively active mutant (CAM)
GPCRs, the equilibrium between R and R* is shifted toward R* as a
result of diminished structural constraints that control spontaneous R
to R* transition. Experimentally, this results in increased agonist
affinity and potency and increased efficacy of partial agonists at
CAM-GPCRs compared with wild-type GPCRs (Samama et al., 1993). In
addition, the relative inhibitory effects of inverse agonists at
CAM-GPCRs are larger than at wild-type GPCRs (Samama et al., 1994;
Gether and Kobilka, 1998).
Of interest, an increasing number of experimental results cannot
readily be explained by the extended ternary complex model. As an
example, certain 2AR ligands behave like
"protean drugs", i.e., they act as agonist in one setting, but as
inverse agonist in another (Chidiac et al., 1994). Additionally, the
efficacy and potency of 2AR agonists is
strongly dependent on the specific purine nucleotide present for
G-protein activation and the specific G-protein to which the
2AR couples (Seifert et al., 1999a;
Wenzel-Seifert and Seifert, 2000). Moreover, the agonist-free and
agonist-occupied 2AR differ from each other
with respect to their ability to activate different cellular effectors
(Zhou et al., 1999). These and other experimental findings (Keith et
al., 1996; Blake et al., 1997; Krumins and Barber, 1997; Zuscik et al.,
1998; Thomas et al., 2000) could be reconciled by a multistate model of
GPCR activation in which ligands stabilize unique and ligand-specific
GPCR conformations, which enable GPCR to modulate its cognate
G-protein(s) in a ligand-specific manner (Kenakin, 1996a,b; Tucek,
1997; Gether and Kobilka, 1998).
The aim of this study was to examine the hypothesis that the functional
properties of partial agonists are due to their ability to stabilize
distinct conformational states in GPCRs. Therefore, we characterized
functional differences between full agonists and partial agonists using
fusion proteins between the wild-type 2AR and
Gs
(2ARGs) and
2ARCAM (Samama et al.,
1993; Gether et al., 1997) and Gs
(2ARCAMGs)
expressed in Sf9 insect cells. We and others have shown that fusion
proteins are a very sensitive experimental system for studying
receptor/G-protein interactions (Seifert et al., 1999b; Milligan,
2000). Because of the defined 1:1 stoichiometry of GPCR to
G, fusion proteins eliminate bias in the
analysis of ligand potencies and efficacies caused by varying ratios of
receptor to G-protein (Hoyer and Boddeke, 1993; Kenakin, 1997). In
addition, fusion proteins allow precise determination of agonist and
inverse agonist efficacy in an expression level-independent manner by
measurement of steady-state GTP hydrolysis and ternary complex
formation (Seifert et al., 1999b; Milligan, 2000). The results of our
present study suggest that agonists have different efficacies with
respect to their ability to promote different steps of the G-protein
activation/deactivation cycle and provide evidence for the existence of
multiple ligand-specific conformational GPCR states. Finally, our
results suggest that one possible mechanism for partial agonism is
strong stabilization of the ternary complex, thereby reducing G-protein turnover.
| |
Experimental Procedures |
Materials.
The DNA encoding
2ARCAM was kindly
donated by Dr. R. J. Lefkowitz (Duke University, Durham, NC)
(Samama et al., 1993). Sources of other materials have been described
elsewhere (Seifert et al., 1998a,b).
Construction of
2ARCAMGs Fusion Protein
DNAs.
The fusion proteins used in our present study contained the
long splice variant of Gs. The construction of
2ARGs DNA was
described recently (Seifert et al., 1998a,b). For construction of
2ARCAMGs
DNA, the KpnI/EcoRV-fragment of the
2AR was excised from
pGEM-3Z-2ARGs and
replaced by the corresponding KpnI/EcoRV-fragment
of 2ARCAM DNA. The
KpnI/EcoRV fragment of 2ARCAM DNA differs from
the corresponding 2AR DNA fragment by mutations that encode for four discrete amino acid substitutions in the
third intracellular loop of the receptor (Samama et al., 1993). The
2ARCAMGs
DNA was cloned into the baculovirus expression vector pVL 1392.
Cell Culture and Membrane Preparation.
Recombinant
baculoviruses were generated in Sf9 cells using the BaculoGOLD
transfection kit (Pharmingen, San Diego, CA). After initial
transfection, recombinant baculoviruses were isolated by plaque
purification. High-titer virus stocks were generated by three
sequential amplifications of plaque-purified virus colonies. Culture of
Sf9 cells and membrane preparation were performed as described recently
(Seifert et al., 1998a,b).
[3H]DHA Binding.
Membranes were thawed and
sedimented by a 15-min centrifugation at 4°C and 15,000g
to remove residual endogenous guanine nucleotides as far as possible
and resuspended in binding buffer (12.5 mM MgCl2,
1 mM EDTA, and 75 mM Tris/HCl, pH 7.4). Expression levels of fusion
proteins were determined by incubating Sf9 membranes (15-25 µg of
protein per tube) in the presence of [3H]DHA at
a concentration of 10 nM. Nonspecific binding was determined in the
presence of [3H]DHA (10 nM) plus 10 µM
(±)-alprenolol. The total volume of the binding reaction was 500 µl.
Incubations were performed for 90 min at 25°C and shaking at 250 rpm.
Competition binding experiments were carried out with Sf9 membranes
expressing 2ARGs or 2ARCAMGs
(15-40 µg of protein per tube), 1 nM [3H]DHA
and agonists at various concentrations with or without GTPS (10 µM). Ligand-competition studies were performed in triplicates. Bound
[3H]DHA was separated from free
[3H]DHA by filtration through GF/C filters
using a 48-well harvester (model M-48R; Brandel, Gaithersburg, MD),
followed by three washes with 2 ml of binding buffer (4°C).
Filter-bound radioactivity was determined by liquid scintillation
counting using Cytoscint cocktail from ICN (Irvine, CA). The
experimental conditions chosen ensured that not more than 10% of the
total amount of [3H]DHA added to binding tubes
was bound to filters.
Steady-State GTPase Activity.
Membranes were thawed and
sedimented by a 15-min centrifugation at 4°C and 15,000g
to remove residual endogenous guanine nucleotides as far as possible
and resuspended in 10 mM Tris/HCl, pH 7.4. Assay tubes contained Sf9
membranes expressing
2ARGs or 2ARCAMGs
(10 µg of protein per tube), 1.0 mM MgCl2, 0.1 mM EDTA, 0.1 mM ATP, 1 mM adenylyl imidodiphosphate, 100 nM GTP, 5 mM
creatine phosphate, 40 µg of creatine kinase, 0.2% (w/v) bovine
serum albumin in 50 mM Tris/HCl, pH 7.4, and
2AR ligands at various concentrations.
Reaction mixtures (80 µl) were incubated for 3 min at 25°C before
the addition of 20 µl of [-32P]GTP
(0.2-0.5 µCi/tube). Reactions were conducted for 20 min at 25°C.
Reactions were terminated by the addition of 900 µl of a slurry
consisting of 5% (w/v) activated charcoal and 50 mM
NaH2PO4, pH 2.0. Charcoal
absorbs nucleotides but not Pi. Charcoal-quenched reaction mixtures were centrifuged for 15 min at room temperature at
15,000g. Seven hundred microliters of the supernatant fluid of reaction mixtures was carefully removed to avoid any aspiration of
charcoal, and 32Pi was
determined by liquid scintillation counting. Enzyme activities were
corrected for spontaneous degradation of
[-32P]GTP. Spontaneous
[-32P]GTP degradation was determined in
tubes containing all of the above-described components plus a very high
concentration of unlabeled GTP (1 mM) that, by competition with
[-32P]GTP, prevents
[-32P]GTP hydrolysis by enzymatic activities
present in Sf9 membranes. Spontaneous
[-32P]GTP degradation was <1% of the total
amount of radioactivity added. The experimental conditions chosen
ensured that not more than 10% of the total amount of
[-32P]GTP added was converted to
32Pi.
Miscellaneous.
Protein was determined using the Bio-Rad DC
protein assay kit (Bio-Rad, Hercules, CA). Immunoblotting studies were
performed as described (Seifert et al., 1998a,b). Ligand competition
curves and concentration-response curves were analyzed by nonlinear
regression, using the Prism program (GraphPad, San Diego, CA).
| |
Results |
Expression of 2ARGs and
2ARCAMGs in Sf9
Membranes.
Similar to nonfused 2AR and
2ARCAM (Gether et al.,
1997), the maximum expression level of
2ARCAMGs
in Sf9 cells was ~2.5-fold lower than the expression level of
2ARGs
(2ARGs, 7.2 ± 2.1 pmol/mg;
2ARCAMGs,
3.2 ± 1.2 pmol/mg). However, the different expression levels of
the fusion proteins were not of relevance for our studies since the
efficacies of ligands at stabilizing the ternary complex and at
promoting GTP hydrolysis are expression level-independent (Seifert et
al., 1999; Milligan, 2000). Immunoblotting studies with the M1 antibody
recognizing the N-terminal FLAG epitope of 2AR
and 2ARCAM (Gether et
al., 1995, 1997) and anti-Gs Ig confirmed that
2ARGs and 2ARCAMGs
expressed in Sf9 membranes were structurally intact (data not shown).
Agonist and Inverse Agonist Regulation of Steady-State GTPase
Activity in Sf9 Membranes Expressing
2ARGs and
2ARCAMGs.
An important
hallmark of constitutive GPCR activation is the increased relative
inhibitory effect of inverse agonist at CAM-GPCR compared with
wild-type GPCR (Lefkowitz et al., 1993; Gether and Kobilka, 1998). In
addition, the agonist-affinity of CAM-GPCRs is increased relative to
wild type-GPCRs, while the inverse agonist-affinity is decreased. The
full agonist (
)-ISO was more potent at activating GTP hydrolysis at
2ARCAMGs
(EC50 = 2.4 ± 1.1 nM) than at 2ARGs,
(EC50 = 13 ± 3 nM), while the inverse
agonist ICI was less potent at
2ARCAMGs
(IC50 = 8.5 ± 2.5 nM) than at 2ARGs
(IC50 = 2.8 ± 1.0 nM) (Fig.
1). For
2ARGs, 17% of the
ligand-regulated GTPase activity (the difference between maximum
()-ISO-stimulated and minimum ICI-inhibited GTP hydrolysis) was
attributable to the inverse agonist, while for
2ARCAMGs, 48% of the ligand-regulated GTPase activity was attributable to ICI.
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Fig. 1.
Effects of ()-ISO and ICI on GTPase activity in Sf9
membranes expressing 2ARGs and
2ARCAMGs. GTPase activity in
membranes expressing 2ARGs (6.5 pmol/mg)
(A) or 2ARCAMGs (2.5 pmol/mg)
(B) was determined as described under Experimental
Procedures. Reaction mixtures contained ()-ISO or ICI at the
concentrations indicated on the abscissa. The dashed lines are
extrapolations of basal GTPase activities to illustrate the relative
contributions of ()-ISO and ICI at the ligand-regulated enzyme
activity. To reliably quantitate the inhibitory effect of ICI on GTPase
in membranes expressing 2ARGs, this
construct was expressed at a higher level than
2ARCAMGs. Therefore, the
absolute GTPase activities in A are higher than in B. To facilitate
comparison of the two constructs, the scales of the ordinates in A and
B are different. Data shown are the means ± S.D. of three
independent experiments performed in duplicate.
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Ligand Binding Properties of 2ARGs
and 2ARCAMGs.
Sf9
membranes expressing
2ARGs and
2ARCAMGs
bound the 2AR antagonist
[3H]DHA in a monophasic and saturable
manner and with similar Kd values
(2ARGs, 0.36 ± 0.03 nM;
2ARCAMGs,
0.24 ± 0.05 nM). We also studied the agonist and inverse agonist
binding properties of
2ARGs and
2ARCAMGs.
The ligand competition curves are shown in Figs.
2-4,
and Table 1 summarizes the nonlinear regression analysis
of the binding data. In membranes expressing
2ARGs, strong
agonists [()-ISO, (+)-ISO, SAL, and DOB] efficiently stabilized the
ternary complex as is shown by the GTPS-sensitive high-affinity agonist binding. With these ligands, ~40% of the
2ARs displayed high agonist affinity. For the
partial agonist EPH, distinct high-affinity binding sites at
2ARGs could not be
discriminated, but GTPS could still shift the EPH competition curve
~5-fold to the right. The binding of another partial agonist, DCI, to
2ARGs, was virtually
GTPS insensitive. GTPS did not shift the ICI-competition curve in
membranes expressing
2ARGs.
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Fig. 2.
Competition by ()-ISO, SAL, and DOB of
[3H]DHA binding in Sf9 membranes expressing
2ARGs or
2ARCAMGs: effect of GTPS.
[3H]DHA binding in Sf9 membranes was performed as
described under Experimental Procedures. Reaction
mixtures contained Sf9 membranes (15-40 µg of protein per tube)
expressing 2ARGs (3.3-7.5 pmol/mg)
(A-C) or 2ARCAMGs (2.5-4.9
pmol/mg) (D-F), 1 nM [3H]DHA, and ligands at the
concentrations indicated on the abscissa. Reaction mixtures
additionally contained distilled water (control) or GTPS (10 µM).
Data shown are the means ± S.D. of four to seven independent
experiments performed in triplicate.
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Fig. 3.
Competition by EPH, DCI, and ICI of
[3H]DHA binding in Sf9 membranes expressing
2ARGs or
2ARCAMGs: effect of GTPS.
[3H]DHA binding in Sf9 membranes was performed as
described under Experimental Procedures. Reaction
mixtures contained Sf9 membranes (15-40 µg of protein per tube)
expressing 2ARGs (3.3-7.5 pmol/mg)
(A-C) or 2ARCAMGs (2.5-4.9
pmol/mg) (D-F), 1 nM [3H]DHA, and ligands at the
concentrations indicated on the abscissa. Reaction mixtures
additionally contained distilled water (control) or GTPS (10 µM).
Data shown are the means ± S.D. of four to seven independent
experiments performed in triplicate.
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Fig. 4.
Competition by ()-ISO and (+)-ISO of
[3H]DHA binding in Sf9 membranes expressing
2ARGs or
2ARCAMGs: effect of GTPS.
[3H]DHA binding in Sf9 membranes was performed under
Experimental Procedures. Reaction mixtures contained Sf9
membranes (15-40 µg of protein per tube) expressing
2ARGs (3.3-7.5 pmol/mg) (A and B) or
2ARCAMGs (2.5-4.9 pmol/mg)
(C and D), 1 nM [3H]DHA, and ligands at the
concentrations indicated on the abscissa. Reaction mixtures
additionally contained distilled water (control) or GTPS (10 µM).
Data shown are the means ± S.D. of four to seven independent
experiments performed in triplicate.
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TABLE 1
Ligand binding properties of 2ARGs and
2ARCAMGs expressed in Sf9 membranes:
effect of GTPS
[3H]DHA binding was determined as described under
Experimental Procedures in Sf9 membranes expressing
2ARGs (3.3-7.5 pmol/mg) or
2ARCAMGs (2.5-4.9 pmol/mg). The ligand
competition binding curves shown in Figs. 2, 5, and 7 were analyzed by
nonlinear regression for best fit to single-site or two-site binding.
Kh and Kl designate the
dissociation constants for high- and low-affinity agonist binding,
respectively. %Rh indicates the percentage of
receptors displaying high agonist affinity. The corresponding values
obtained in the presence of GTPS (10 µM) are designated
KhGTPS, KlGTPS, and
%RhGTPS, respectively. Dissociation constants
for ICI are listed below Kl and
KlGTPS, respectively. Data shown represent the
means ± S.D. of four to seven independent experiments performed
in triplicate.
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The ligand binding properties of
2ARCAMGs
differed considerably from the ligand binding properties of
2ARGs. The high-affinity Ki values of ()-ISO,
(+)-ISO, SAL, and DOB at
2ARCAMGs were about 4 to 10 times lower than at
2ARGs. While there was no large change in the fraction of
2ARCAM displaying high agonist affinity when liganded to ()-ISO and SAL compared with 2ARGs, the fraction
of receptors displaying high agonist-affinity upon binding of DOB and
(+)-ISO in
2ARCAMGs
was substantially higher than in
2ARGs. In contrast to
2ARGs, where distinct
high-affinity binding sites for EPH and DCI could not be distinguished,
highly effective formation of GTPS-sensitive ternary complexes with
EPH and DCI was observed at
2ARCAMGs. In agreement with data obtained for nonfused
2AR and
2ARCAM (Samama et al.,
1994), the affinity of ICI for
2ARCAMGs was about 2-fold lower than for
2ARGs. GTPS
increased the affinity of ICI for
2ARCAMGs
by ~2.5-fold.
Efficacies of Partial Agonists on Steady-State GTPase Activity in
Sf9 Membranes Expressing 2ARGs and
2ARCAMGs.
The precise
determination of partial agonist efficacy constitutes a major problem
since efficacy is influenced by numerous variables such as the
expression level of GPCR and the availability of G-protein and effector
system (Hoyer and Boddeke 1993; Kenakin 1996a, 1997). The fusion
protein approach offers a unique possibility to assess agonist efficacy
in an expression level-independent manner by measuring steady-state
GTPase activity (Seifert et al., 1999; Milligan, 2000). At
2ARGs, ligands
activated GTP hydrolysis in the order of efficacy ()-ISO ~ SAL 
(+)-ISO > DOB > EPH > DCI (Figs. 5 and
6; Table
2). In accordance with data obtained for effector system
activation by nonfused 2AR and
2ARCAM (Samama et al.,
1993), the potencies of agonists for GTPase activation at
2ARCAMGs
were higher than at
2ARGs. There was a small but significant increase in the efficacy of the partial agonists
DOB, EPH, and DCI at activating GTPase in membranes expressing 2ARCAMGs
compared with membranes expressing
2ARGs. For SAL and
(+)-ISO, the increase in efficacy at
2ARCAMGs versus 2ARGs was not
significant.
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Fig. 5.
Concentration-response curves for the stimulatory
effects of ()-ISO, SAL, DOB, EPH, and DCI on steady-state GTPase
activity in membranes expressing 2ARGs
and 2ARCAMGs. GTPase activity
in membranes expressing 2ARGs (3.3-7.5
pmol/mg) (A) or 2ARCAMGs
(2.5-4.9 pmol/mg) (B) was determined as described under
Experimental Procedures. Reaction mixtures contained
ligands at the concentrations indicated on the abscissa. For each
construct, the stimulatory effect of ()-ISO (10 µM) on GTP
hydrolysis was set 100%, and all data points were referred to this
stimulation. Data shown are the means ± S.D. of three to six
independent experiments performed in duplicate.
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Fig. 6.
Concentration-response curves for the stimulatory
effects of ()-ISO and (+)-ISO on steady-state GTPase activity in
membranes expressing 2ARGs and
2ARCAMGs. GTPase activity in
membranes expressing 2ARGs (3.3-7.5
pmol/mg) (A) or 2ARCAMGs
(2.5-4.9 pmol/mg) (B) was determined as described under
Experimental Procedures. Reaction mixtures contained
ligands at the concentrations indicated on the abscissa. For each
construct, the stimulatory effect of ()-ISO (10 µM) on GTP
hydrolysis was set 100%, and all data points were referred to this
stimulation. Data shown are the means ± S.D. of three to six
independent experiments performed in duplicate.
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TABLE 2
Efficacies and potencies of 2AR ligands at the GTPase of
2ARGs and 2ARCAMGs
GTPase activity was measured as described under Experimental
Procedures in Sf9 membranes expressing various
2ARGs and 2ARCAMGs.
Reaction mixtures contained 2AR ligands at 0.1 nM-1mM as
appropriate to obtain saturated concentration-response curves. Ligand
efficacies and potencies (EC50 values) were obtained by
nonlinear regression analysis of the concentration-response curves
shown in Figs. 3 and 4. The efficacy of ()-ISO was set 1.00, and the
effects of other ligands are referred to this effect. Data shown are
the means ± S.D. of three to seven independent experiments
performed in duplicate. The data shown for 2ARGs
were previously reported in Seifert et al. (1999a). Data
for 2ARGs were compared versus
2ARCAMGs using the t test.
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Discussion |
Sf9 Cell Membranes Expressing GPCR-G Fusion Proteins
as Model System for the Analysis of Ligand-Receptor Interactions.
In the present study, we expressed a wild-type GPCR and a CAM-GPCR
fused to G in Sf9 cells to study
ligand-receptor interactions. Compared with conventional coexpression
systems, the fusion protein approach offers several advantages.
Specifically, the defined 1:1 stoichiometry of GPCR and
G eliminates bias in the analysis of ligand
potencies and efficacies because of varying
GPCR/G ratio (Seifert et al., 199b; Milligan,
2000). In addition, the physical proximity of GPCR and
G ensures efficient interaction of the
proteins. Fusion proteins allow for the sensitive analysis of ligand
potencies and efficacies in an expression level-independent manner
directly at the G-protein level by measuring steady-state GTP
hydrolysis. This is a very important point because nonfused 2ARCAM expresses at
considerably lower levels than 2AR (Samama et
al., 1993; Gether et al., 1997), resulting in different GPCR/G-protein ratios. Finally, for GPCRs mediating adenylyl cyclase activation such
as the 2AR, the number of effector molecules
limits signal output (Alousi et al., 1991), introducing additional bias
into the analysis of ligand potencies and efficacies.
GPCR-G fusion proteins are not naturally
occurring so that caution must be exerted when extrapolating
conclusions obtained with fused proteins to the in vivo situation.
Perhaps most evident, in native membranes there is a large excess of
Gs molecules relative to
2AR molecules (Ransnäs and Insel, 1988).
However, the mere excess of G-protein relative to GPCR does not
automatically imply that one GPCR molecule activates multiple
G molecules. Rather, recent data from various
GPCR/G-protein combinations, including the
2AR/Gs pair indicate
that even in coexpression systems with a high G-protein to GPCR ratio,
GPCRs activate G-proteins only linearly (Seifert et al., 1998a;
Wenzel-Seifert et al., 1999; Wenzel-Seifert and Seifert, 2000). Thus,
GPCR-G fusion proteins may mimic the close
association of GPCRs and G-proteins in vivo (Seifert et al., 1999b).
Another issue that needs to be considered is the GTP concentration in
our experiments. Ternary complex formation in membranes was studied in
washed membranes, i.e., in the virtual absence of GTP. GTPase studies
were conducted with a substrate concentration of 100 nM (under
Experimental Procedures). It could be argued that such
studies are not of relevance for the in vivo situation because the bulk
intracellular GTP concentration is in the high micromolar range (Otero,
1990; Jinnah et al., 1993). In addition, adenylyl cyclase assays in
membranes have been routinely performed with GTP concentrations in the
high micromolar range (Samama et al., 1993; Chidiac et al., 1994;
Gether et al., 1995). However, the concentration of GTP available to
G-proteins in vivo has not been determined. First, the access of GTP to
G-proteins is restricted (Otero, 1990; Wieland and Jakobs, 1992;
Klinker et al., 1996). Second, there is a remarkable discrepancy
between the high intracellular GTP concentration and the low
Km of G-proteins for GTP (~0.1 µM) (Seifert et al., 1998a; Wenzel-Seifert et al., 1999), and in vivo, most
enzymes work at substrate concentrations around the
Km value. These data suggest that even
in vivo G-proteins may operate under nonsaturating GTP concentrations,
allowing for at least some ternary complex formation and efficient
regulation of G-protein turnover by modulating the GTP concentration in
the G-protein vicinity.
Can the extended ternary complex model explain the functional
properties of 2ARGs and
2ARCAMGs?
Several of our
results are in agreement with the extended ternary complex model, which
proposes that GPCRs exist in an equilibrium between an inactive R state
and an active R* state (Lefkowitz et al., 1993; Gether and Kobilka
1998). The model proposes that in CAM-GPCRs, R to R* isomerization
occurs more readily than in wild-type GPCRs, but there is no
fundamental difference in the R and R* states of CAM-GPCRs. Thus, the
model predicts that the relative inhibitory effects of inverse agonists
at CAM-GPCRs are higher than at wild type-GPCRs. The increased relative
inhibitory effect of ICI at
2ARCAMGs compared with
2ARGs is in agreement with this model
(Fig. 1). The extended ternary complex model also predicts that the
inverse agonist affinity and potency at CAM-GPCR is lower than at
wild-type GPCR (Samama et al., 1994). Again, our findings with fusion
proteins are in agreement with the model (Figs. 1 and 3). Another
postulate of the extended ternary complex model is that guanine
nucleotides increase inverse agonist affinity of GPCR, presumably by
uncoupling of GPCR from G-protein and, thereby, stabilizing the R state
(Barker et al., 1994; Leeb-Lundberg et al., 1994). In agreement with
this postulate, we found an increase in inverse agonist-affinity of
2ARCAMGs by GTPS (Fig. 3; Table 1).
An additional prediction of the extended ternary complex model is that
CAM-GPCRs possess a higher agonist affinity and potency than wild-type
GPCRs (Lefkowitz et al., 1993; Samama et al., 1993). Our data with
2ARGs and
2ARCAMGs
show that this property of GPCRs is preserved in fusion proteins
(Tables 1 and 2). Moreover, the extended ternary complex model predicts
that the efficacies of partial agonists are higher at CAM-GPCR than at
wild-type GPCR (Samama et al., 1993). This was also the case for
2ARGs and
2ARCAMGs,
but the differences were small (Table 2). The explanation for these
only small differences in agonist efficacies between the two fusion
proteins presumably is that we studied coupling of the
2AR and
2ARCAM to the long
splice variant of Gs and that this G-protein
confers to the wild-type 2AR properties of
high constitutive activity in terms of partial agonist efficacy
(Seifert et al., 1998b). It is likely that the differences in partial
agonist efficacies between 2AR and
2ARCAM would have been
more evident if coupling of these GPCRs to the short splice variant of
Gs had been analyzed. However, we did not
construct a fusion protein of
2ARCAM and the short
splice variant of Gs because a fusion protein
of the 2AR and this G-protein expresses less
well than a fusion protein of the 2AR and the
long splice variant of Gs (Seifert et al.,
1998a,b). Given the fact that 2ARCAM expresses much
less well than 2AR (see Results;
Gether et al., 1997), we predicted that the expression levels of a
fusion protein of 2ARCAM
and the short splice variant of Gs would be
too low for sensitive quantitative analysis of ternary complex formation and particularly GTPase activation.
Certain effects of agonists on the functional properties of
2ARGs and
2ARCAMGs
are less readily explained by the extended ternary complex model.
Specifically, the extended ternary complex model also predicts that
there is a correlation between the efficacy of agonists at stabilizing
the ternary complex and their efficacy at promoting multiple G-protein
activation/deactivation cycles. This concept is based on the observed
highly significant correlation between the efficacy of agonists at
stabilizing the ternary complex and the efficacy of agonists at
promoting effector system activation (Kent et al., 1980). We studied
the outcome of multiple G-protein activation/deactivation cycles more
directly by assessing steady-state GTPase activity. In agreement with
the results of a previous study (Kent et al., 1980), we observed
significant correlations between the efficacy of agonists at
stabilizing the ternary complex (as determined by the percentage of
high-affinity agonist-binding sites and the ratio
KlGTPS/Kh) and the efficacy of agonists at activating GTPase for
2ARGs (Fig.
7, A and C). However, no such correlation
was observed for 2ARCAMGs
(Fig. 7, B and D). Most strikingly, at
2ARCAMGS, EPH, DCI, and particularly DOB exhibited a higher percentage of high-affinity binding sites than ()-ISO. In contrast, all of these
ligands had lower efficacies than ()-ISO at stimulating GTPase. In
addition, ()-ISO and (+)-ISO, which differ from each other only in
the chirality of the -carbon hydroxyl group of the ethylamine side
chain of the phenyl ring, differed considerably from each other in
their ability to stabilize the ternary complex at
2ARCAMGs
(Fig. 4). However, the efficacies of ()-ISO and (+)-ISO at activating
GTPase in membranes expressing
2ARCAMGs were similar (Fig. 6; Table 2).
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Fig. 7.
Relation between the efficacy of agonists at
stabilizing the ternary complex and the ligand efficacy at activating
GTPase in Sf9 membranes expressing 2ARGs
and 2ARCAMGs. The efficacies
of ligands at stabilizing the ternary complex in membranes
expressing 2ARGs and
2ARCAMGs (Figs. 2-4; Table
1) were plotted against the respective efficacies of these ligands at
activating GTPase (Figs. 5 and 6; Table 2). Data were analyzed by
linear regression analysis. In A and B, ternary complex formation is
expressed as the percentage of receptors displaying high agonist
affinity (Rh, %). A,
r2 = 0.71; p = 0.035. B, r2 = 0.08; p, = 0.586 (slope not significantly different from zero). In C and D,
ternary complex formation is expressed as the ratio
KlGTPS/Kh.
For EPH and DCI, distinct Kh values at
2ARGs could not be determined. Therefore,
we used the values listed under Kl in Table
1 to calculate the ratio. C, r2 = 0.86;
p = 0.007. D, r2 = 0.04; p = 0.716 (slope not significantly different
from zero). The dotted lines indicate the 95% confidence interval of
the regression lines.
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Dissociation in the efficacy of agonists at stabilizing the ternary
complex and promoting multiple cycles of G-protein
activation/deactivation were observed previously. First, when the
2AR couples to either the long or the short
splice variant of Gs, SAL and DOB are similarly efficient at stabilizing the ternary complex. However, with
respect to GTPase activation, the two ligands are more effective at the
2AR coupled to the long splice variant of
Gs compared with the
2AR coupled to the short splice variant of
Gs (Seifert et al., 1998b). Second, at the
2AR and
2ARCAM expressed in
Chinese hamster ovary cells, DOB is more effective than SAL at
stabilizing the ternary complex, but not at activating adenylyl cyclase
(Samama et al., 1993). Third, at certain mutants of the
2AR (Hausdorff et al., 1990), histamine
H2 receptor (Smit et al., 1996), prostaglandin EP3 receptor (Irie et al., 1994),
5-hydroxytryptamine2A receptor (Roth et al.,
1997), and M4 muscarinic acetylcholine receptor (Van Koppen et al., 1994) the ability of agonist to promote multiple G-protein activation/deactivation cycles is severely reduced compared with their wild-type counterparts, but the ability of mutant GPCRs to
form ternary complexes is normal. Nonsignaling ternary complexes were
also reported for the 
1B-adrenergic receptor
(Chen et al., 2000), cannabinoid CB1 receptor
(Bouaboula et al., 1997), and the MOR-1 opioid receptor (Brown and
Pasternak, 1998). Based on these observations encompassing multiple
GPCRs coupled to G-proteins from different families it can be concluded
that the GPCR conformation that optimally promotes multiple G-protein
activation/deactivation cycles is distinct from the GPCR conformation
that promotes high-affinity interactions between GPCR and G-protein.
These observations suggest that one possible mechanism of partial
agonism is stabilization of the ternary complex relative to GTP binding
and G-protein dissociation. A highly stable ternary complex would be
less likely to bind GTP, thereby reducing G-protein turnover.
Mechanisms of Action of Full and Partial Agonists.
Of
interest, the ratio of EC50 for GTPase activation
to Kh for agonists at
2ARCAMGs
shows a significant correlation with the efficacy of agonists at
activating GTPase (Fig. 8). The data
obtained for 2ARGs
show a similar trend as for
2ARCAMGs but do not reach significance. It is surprising that the ratio of
EC50 to Kh is
significantly higher for full agonists than partial agonists. This
suggests that occupancy of a GPCR by a full agonist is less likely to
lead to a complete G-protein activation/deactivation cycle than is GPCR
occupancy by a partial agonist. A possible mechanism for this
hypothesis is illustrated in Fig. 9. This
model proposes that the ternary complex for partial agonists is more stable, relative to the other GPCR and G-protein states (PR, G, GGDP, GGTP), than is the
ternary complex for full agonists, relative to the other GPCR and
G-protein states (FR, G, GGDP,
GGTP). Thus, rate constants
k1 and
k2 for full and partial agonists may
be similar. However, if the rate constants
k
1,
k2, and
k3 are all smaller for partial
agonists, compared with these constants for full agonists, the relative
amount of the ternary complex (partial agonists) will be greater and
the number of total G-protein hydrolysis cycles will be smaller,
compared with full agonists. The model shown in Fig. 9 also proposes
that the ternary complex for full agonists is more likely to dissociate
without binding GTP, thus k1 and
k2 are greater for full agonists
than for partial agonists. This could explain the larger EC50 to Kh ratio
for full agonists. A larger receptor occupancy would be required to
compensate for larger k1 and
k2 rates for full agonists as
compared to partial agonists.
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Fig. 8.
Relation between the ratio
EC50/Kh and efficacy of agonists
at activating GTPase in Sf9 membranes expressing
2ARGs and
2ARCAMGs. The ratios of the
EC50 for GTPase activation (Figs. 5 and 6; Table 2) and
Kh values (Figs. 2 and 3; Table 1) for
various agonists at 2ARGs and
2ARCAMGs were plotted against
the respective efficacies of these ligands at activating GTPase (Figs.
5 and 6; Table 2). Data were analyzed by linear regression analysis. A,
r2 = 0.653; p = 0.192. B, r2 = 0.82;
p = 0.014. The dotted lines indicate the 95%
confidence interval of the regression line.
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Fig. 9.
Model of the different effects of full and partial
agonists on the G-protein activation/deactivation cycle. The arrows
symbolize the relative rate constants for interconversion of the
various GPCR and G-protein states. G, guanine nucleotide-free
G-protein; GGDP, GDP-liganded G-protein; GGTP,
GTP-liganded G-protein; F, full agonist; P, partial agonist; R,
G-protein-coupled receptor.
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Conclusions.
Our present data and an increasing body of data
obtained with wild-type GPCRs (Chidiac et al., 1994; Chiu et al., 1996;
Keith et al., 1996; Blake et al., 1997; Bouaboula et al., 1997) and constitutively active GPCR mutants (Zuscik et al., 1998; Thomas et al.,
2000) and theoretical considerations (Kenakin 1996a,b; Tucek 1997)
suggest that ligands stabilize distinct GPCR conformations that differ
from each other in their ability to interact with G-proteins. Thus, the
conformations stabilized by ()-ISO, (+)-ISO, and SAL in both
2AR and
2ARCAM are functionally
distinguishable from those induced by agonists with lower efficacies,
i.e., DOB, EPH, and DCI. Additionally, our results suggest that some
GPCR ligands act as partial agonists because the GPCR conformation that
they stabilize promotes a more stable ternary complex than the
conformation stabilized by full agonists. By stabilizing the guanine
nucleotide-free ternary complex these partial agonists reduce G-protein turnover.
We thank Dr. Terry Kenakin (Glaxo-Wellcome, Research Triangle
Park, NC) for stimulating discussions and Maria Bakk for help with the
cell culture.
R.S. and K.W.-S. were the recipients of a research fellowship
of the Deutsche Forschungsgemeinschaft.
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Abstract
Introduction
