Departments of Pharmacology (S.M.W., K-L.L., D.J.M., R.R.N.) and
Internal Medicine/Hypertension (R.R.N.), The University of
Michigan, Ann Arbor, Michigan
Constitutive activation of G protein-coupled receptors (GPCRs) is now
well recognized and many classical GPCR antagonists have been found to
be inverse agonists. For the 
2A-adrenergic receptor (AR)
we determine the relative inverse efficacies of a series of antagonists
and utilize the extended ternary complex model to estimate the fraction
of constitutively active mutant (CAM) receptors in the active state.
Stable Chinese hamster ovary cell lines expressing the porcine
2A-AR in its wild-type (WT) and constitutively activated
(CAM-T373K) form were isolated. Activation of both Gi and
Gs was enhanced for CAM receptors. cAMP production was
suppressed in cells with the CAM 2A-AR and this
suppression was reversed by 2-adrenergic antagonists
with an order of inverse efficacy of rauwolscine > yohimbine > RX821002 > MK912, whereas phentolamine and idazoxan were
essentially neutral antagonists. This striking difference in inverse
efficacy between idazoxan and RX821002 may account for in vivo
pharmacological differences between these two
2-adrenergic antagonists. Agonist binding affinity to
the non-G protein-coupled CAM receptor was 3- to 9-fold higher than to
WT, whereas binding of the most efficacious inverse agonists, yohimbine
and rauwolscine, was 1.7- and 2.1-fold weaker. Analysis of this
difference by the extended ternary complex model indicates that
approximately 50% of the CAM 2A-AR is in the active
(R*) state although there is no detectable constitutive
activity of the WT receptor in the absence of agonist.
 |
Introduction |
Receptors
coupled to G proteins (GPCRs) play a major role in signal transduction
and are the targets of a large number of therapeutic drugs. An
important development in the understanding of GPCRs was the recognition
that they could couple to (Wreggett and De Lean, 1984
; Neubig et al.,
1988) and functionally activate (Costa and Herz, 1989) G proteins in
the absence of an agonist. These initial observations were buttressed
by the identification of mutant receptors that had substantial
constitutive activity (Kjelsberg et al., 1992; Parma et al., 1993;
Shenker et al., 1993). This led to the "Extended Ternary Complex
(ETC) model" (Samama et al., 1993) and the cubic ternary complex
model (Weiss et al., 1996). In these models, the receptor exists in an
equilibrium between an inactive state R and an active state
R* in the absence of drug. This equilibrium, differing for
each receptor, determines basal activity. For wild-type receptors,
R predominates and there is minimal receptor activity in the
absence of agonist. Binding of agonist stabilizes R* causing
G protein coupling and activation of cellular responses. High levels of
receptor expression or constitutively active mutant receptors increase
the concentration of R* inducing a response in the absence
of agonist. In some disease states such as familial male precocious
puberty (luteinizing hormone receptor) (Shenker et al., 1993),
hyperfunctioning thyroid adenoma (thyrotropin receptor) (Parma et al.,
1993), and retinitis pigmentosa (rhodopsin) (Rao et al., 1994),
naturally occurring point mutations that lead to constitutive
activation of GPCRs have been implicated.
Constitutively active GPCRs suggested the concept of inverse agonists
(Barker et al., 1994; Chidiac et al., 1994; Bond et al., 1995)
drugs
that preferentially bind to R and inhibit basal receptor
activity. In contrast, neutral antagonists bind equally well to
R and R*, have no effect on basal receptor
activity, but block the effects of both agonists and inverse agonists.
Indeed, many drugs classically thought of as antagonists were
subsequently found to have inverse agonist activity (Chidiac et al.,
1994). Inverse agonists are expected to have therapeutic utility in the setting of CAM receptors such as in familial male precocious puberty or
thyroid adenomas but more recently, they have been found to have unique
physiological or biochemical effects (Nagaraja et al., 1999) even in
the setting of relatively low levels of expression of wild-type
receptors (Berg et al., 1999). Thus the differentiation of inverse
agonist and neutral antagonist activity is important to our
understanding of drug mechanisms.
Although the general features of the ETC model are accepted,
there have not been clear quantitative tests of that model. For example, it isn't clear what fraction of receptors are in the R* state for WT and CAM receptors. Also, inverse agonists
should have a lower affinity for the R* state of GPCRs but
the data demonstrating this is not clear. Most studies have shown
limited (
2-fold) effects on inverse agonist affinity for CAM mutant
receptors. Here we examine quantitative questions about the ETC model
in the context of the 2A-adrenergic receptor.
2-Adrenergic receptors (AR) play important
physiological roles in the central control of blood pressure, pain, and
neuronal excitability and the 2A-AR subtype is
the major contributor to these responses (MacMillan et al., 1996; Hein
et al., 1999). Furthermore, 2-AR agonists like
clonidine are effective antihypertensive therapies although there
remains some controversy over the relative role of the
2A-AR and the putative
I1 imidazoline receptor in these actions. Like
opioid receptors, 2-ARs are well known to
exhibit a pronounced excitatory withdrawal syndrome upon rapid
cessation of chronic agonist therapy (Neusy and Lowenstein, 1989). The
classical antagonist of the 2-AR, yohimbine,
causes central excitation but it is not clear whether the central
excitatory effects of yohimbine are: 1) manifestations of pure
antagonist activity at the 2-AR, 2) due to the
reported inverse efficacy of yohimbine (Tian et al., 1994), or 3) due
to effects on other receptors such as 5HT receptors (Convents et al.,
1989). Currently, there is insufficient pharmacological
characterization of these 2A antagonists to
define such mechanisms. The identification of
2A adrenergic inverse agonists and neutral
antagonists that are more selective than yohimbine would be desirable.
Furthermore, recent literature is contradictory as to whether the
classical 2-AR antagonists are inverse
agonists or neutral antagonists (Tian et al., 1994; Wurch et al.,
1999).
Lefkowitz and colleagues (Ren et al., 1993) showed that mutation of
Thr-373 in the 2A-AR results in CAM activity
leading to basal inhibition of adenylyl cyclase and increased receptor affinity for agonist. We use this CAM 2A-AR to
evaluate 2-antagonists for inverse agonist
activity. We wished to determine inverse efficacy of
2-AR antagonists and to examine quantitative
predictions of the ETC model. We found inverse agonist activity among
both alkaloid and imidazoline 2-antagonists
and identified a unique difference between idazoxan and RX821002, which
may have important pharmacological implications. Also, we obtain
estimates of the fraction of the 2A-T373K
mutant receptor in the R* state and set an upper bound for
that fraction for the WT 2A-AR.
| |
Materials and Methods |
Radiochemicals.
[2-3H]Adenine
(21-25 Ci/mmol) was from Amersham Life Science (Arlington Heights,
IL). [3H]Yohimbine (74.5-78 Ci/mmol) was from
DuPont-New England Nuclear (Wilmington, DE).
Chemicals.
Opti-MEM, LipofectAMINE, and Geneticin (G-418)
were obtained from Life Technologies (Gaithersburg, MD).
Fluorescein-labeled anti-[HA]-antibody was from Boehringer Mannheim
(Indianapolis, IN). Pertussis toxin (PTX) and cholera toxin were from
List Biological Laboratories (Campbell, CA). Forskolin was from
Calbiochem (La Jolla, CA). UK-14,304 and prazosin were from Pfizer
(Sandwich, England). Clonidine was from Boehringer Ingelheim
(Ingelheim, Germany), idazoxan from Reckitt & Colman (Hull, England),
MK912 a gift of Dr. Staffan Uhlén, Uppsala University,
phenoxybenzamine from Smith Kline & French Labs (Philadelphia, PA),
phentolamine from Ciba-Geigy (Summit, NJ), propranolol from Ayerst
Laboratories (New York, NY), rauwolscine from Roth (Germany), and
RX821002 from Research Biochemicals, Inc. (Natick, MA).
Isobutyl-1-methyl-xanthine (IBMX), adenosine 5'-triphosphate (ATP),
adenosine 3':5'-cyclic monophosphate (cAMP), 5'-guanylyimidodiphophate
(GppNHp), epinephrine and yohimbine were from Sigma (St. Louis, MO).
Construction of Mutant 2A-Adrenergic Receptor
Plasmids.
The p2Tag H/N construct was
described previously (Wade et al., 1999). It includes an
HA-epitope-tagged porcine 2A-adrenergic receptor with unique silent HindIII and NheI
restriction sites at Ala-359 and Lys-376. Mutagenic cassette ligation
was used to introduce annealed 52-mer oligonucleotides containing the
Thr-373 to lysine constitutively activating mutation into the
HindIII/NheI digested
p2Tag H/N vector. The mutation of the modified
region in the product was confirmed by restriction enzyme digestion
utilizing a silent diagnostic NruI restriction site and
confirmed by DNA sequencing.
Cell Culture and Transfection.
CHO-K1 cells were maintained
in Ham's F-12 medium with 10% fetal bovine serum, 100 units/ml
penicillin and 100 µg/ml streptomycin at 37°C in 5%
CO2. Stable selection for mutants was maintained by the addition of 0.4 mg/ml active G-418.
CHO-K1 cells were cotransfected with the cDNA for HA-epitope-tagged WT
or CAM (T373K) 2A-adrenergic receptor in pCMV4
along with the pSV2neo plasmid containing the neomycin resistance gene (kindly provided by Dr. Jun Sadoshima, University of Michigan). The
ratio of receptor to pSV2neo DNA was 5 to 1. The DNA was added in
Opti-MEM with 6 µl of LipofectAMINE reagent per µg of DNA for 24 h. Cells were returned to complete growth medium and 72 h
after the start of transfection, G-418 was added. After 2 to 3 weeks in
selection medium, G-418 resistant cells were labeled with a fluorescein-conjugated 12CA5 anti-HA monoclonal antibody and single receptor-positive cells sorted into 96-well plates on a Coulter Elite
ESP cell sorter. Using this method, 100% of CAM clones (13/13) expressed high levels of receptor (5 to 80 pmol/mg of protein). One CAM
(C16) and 3 WT (L1, L9, and Tag19) clones were selected for further study.
CHO-K1 Membranes.
Membranes were prepared as previously
described (Wade et al., 1999). The final membrane pellets were
resuspended in TME buffer (50 mM Tris, 10 mM
MgCl2, 1 mM EGTA, pH 7.6), snap frozen, and stored at 
80°C. Protein was determined by Bradford protein assay (Bradford, 1976).
Radioligand Binding Assays.
[3H]Yohimbine binding assays were performed in
96-well plates with 2 to 5 µg of protein per well in a final volume
of 100 µl as previously described (Neubig et al., 1985). For
competition binding measurements, membranes were incubated with the
indicated drugs in TME buffer in the presence of 10 nM
[3H]yohimbine at room temperature for 30 min
and filtered using a Brandel cell harvester. Nonspecific binding was
defined by 10 µM yohimbine.
Whole Cell cAMP Accumulation.
Whole cell cAMP accumulation
was determined in 24-well plates as previously described (Wade et al.,
1999). Briefly, cells were plated with 1 µCi/well
[3H]adenine for 18 to 20 h before assay
and where indicated, 100 ng/ml pertussis toxin or 5 µg/ml cholera
toxin was included in this preincubation. Cells were washed once with
DMEM, then the assay was initiated by adding DMEM containing 1 mM IBMX,
30 µM forskolin, and the indicated drugs. Cells were incubated 30 min at 37°C, and the reaction was terminated by aspirating the incubation medium and quenching with 1 ml 5% TCA containing 1 mM ATP and 1 mM
cAMP. Acid soluble nucleotides were separated on Dowex and alumina
columns as described by Salomon et al. (1974). cAMP accumulation was
normalized by dividing the [3H]cAMP counts by
the total [3H]nucleotide counts (sum of ATP and
ADP counts from the Dowex columns and cAMP counts from the alumina columns).
Data Analysis.
All data are reported as mean ± S.E.M.
Fitted curves were determined using an unweighted nonlinear
least-squares method in GraphPad Prism version 3.00 for Windows
(GraphPad Software, San Diego, CA, www.graphpad.com). Statistical
analysis of Kd ratios for WT and CAM
receptors used the two-tailed, one sample t test in GraphPad
Prism to compare the experimental ratio with a theoretical value of
1.0.
| |
Results |
Radioligand Binding and Receptor Conformation.
It is well
recognized that receptor conformation states can be monitored by
radioligand binding. Thus we examined quantitatively both agonist and
antagonist affinities for the WT and CAM
2A-AR. Saturation binding experiments with the
radiolabeled 2-antagonist [3H]yohimbine in membranes from the WT-Tag19
and CAM-C16 cell lines revealed similar levels of receptor expression
with Bmax values of 25 and 19 pmol/mg of
protein, respectively (Table 1 and Fig. 1). Mock-transfected (Neo) cells
displayed negligible specific binding (data not shown). To assess the
conformational equilibria of the receptor independent of G protein
coupling, we measured UK-14,304 competition for
[3H]yohimbine binding in the presence of
GppNHp. As expected, the CAM receptor membranes had a much higher
affinity for the 2-AR agonist UK-14,304 than
did the WT receptor-containing membranes (Table 1). Three pieces of
evidence indicate that this enhanced affinity (13 nM versus 92 nM)
reflects receptor conformations and not G protein coupling. First, the
binding was conducted in the presence of GppNHp, which should uncouple
RG complex. Second, two-site fits (not shown) of the competition
studies even in the absence of GppNHp revealed only a small percentage
of the receptors (<20%) in the high-affinity agonist binding
component and F-tests did not show a statistical improvement by
two-site fits over one-site fits (p > 0.5). Third,
direct [3H]UK-14,304 binding studies showed
only 2 to 3 pmol/mg of binding sites versus ~20 pmol/mg of
[3H]yohimbine binding sites (not shown). Thus,
due to the high receptor expression levels in these stable cell lines
(i.e., greater than the amount of G protein), most of the receptor is
uncoupled from G protein and the increased affinity of the CAM receptor
for UK-14,304 is due to the intrinsic conformational properties of the
receptor rather than to altered G protein coupling.
View this table:
[in this window]
[in a new window]
|
TABLE 1
Binding parameters of WT and CAM stable lines
[3H]Yohimbine binding to WT-Tag19 membranes was performed in
96-well plates for 30 min at room temperature. Data represent the
mean ± S.E.M. of three (yohimbine saturation binding) or four
(UK-14,304 competition binding) separate experiments performed in
duplicate or triplicate. The Kd ratio differs from
1.0 with a p < 0.01 (*) or p < 0.002 (**).
|
|
View larger version (23K):
[in this window]
[in a new window]
|
Fig. 1.
Yohimbine saturation binding of WT and CAM porcine
2A-AR. Saturation binding to WT-Tag19 ( )
or CAM ( ) membranes was performed in 96-well plates using 1 to 40 nM
[3H]yohimbine for 30 min at room temperature.
Nonspecific binding, defined in the presence of 10 µM yohimbine,
represented less than 10% of the total binding and was subtracted.
Data represent the mean ± S.E.M. of three separate experiments
performed in duplicate. The Scatchard plot of the saturation binding
data is shown in the bottom panel.
|
|
To understand conformational changes in the CAM receptor and their
relation to mechanisms of inverse agonism, we wanted to determine
whether antagonist affinities were also altered for the CAM receptor.
Earlier studies had reported little or no difference in antagonist
binding for the CAM versus WT receptor (Ren et al., 1993; Wurch et al.,
1999). Since yohimbine had previously been shown to be an inverse
agonist for Gi activation (Tian et al., 1994), we
carefully determined its Kd value for WT
and CAM receptor-expressing membranes to see if the change in receptor
conformation expected with the activating mutation would alter the
[3H]yohimbine binding. In a total of
nine1 saturation experiments, we
found that in every case the Kd for CAM
membranes was higher than that in WT. Although there was some variation
in the absolute Kd values from experiment
to experiment, the Kd ratio was very
consistent at 1.67 ± 0.17 (n = 9) and was significantly different from 1.0 (p < 0.01, two-tailed
one-sample t test).
The binding of a series of other agonists and antagonists was examined
by [3H]yohimbine competition studies in the
presence of GppNHp to assess the intrinsic binding properties of the WT
and CAM receptor (i.e., independent of G protein coupling). Figure
2 shows the results for two agonists and
two antagonists, and a summary for all ligands is presented in Table
2. Epinephrine shows the largest effect of the CAM phenotype with a 9-fold increase in affinity. In contrast, the partial agonist clonidine exhibited only a 3.3-fold increase, whereas UK-14,304, discussed above, was more like epinephrine. Thus, as
previously reported (Wurch et al., 1999), the degree of affinity
enhancement by the CAM mutation correlates with the efficacy of the
agonists for activating Gi. The effects of the CAM mutation on antagonist binding are more subtle but are clearly present. As noted above, [3H]yohimbine binding
affinity was decreased 1.67-fold in a series of nine experiments. In
the competition binding data the Ki
difference for yohimbine was similar but slightly smaller, 1.5-fold.
Competition studies showed a range of effects on antagonist binding
from no change with idazoxan (Fig. 2D) to a 2.1-fold decrease in
affinity for rauwolscine (Fig. 2C). IC50 values
from the competition studies were converted to
Ki values (Table 2) by the Cheng-Prusoff
method (1973) using the directly measured
[3H]yohimbine binding affinities. Discussion of
the functional data in Table 2 follows the presentation of the inverse
efficacy results.
View larger version (34K):
[in this window]
[in a new window]
|
Fig. 2.
Binding of selected agonists and antagonists at the
WT and CAM 2A-AR. Competition binding for 10 nM [3H]yohimbine in the presence of 10 µM
GppNHp was performed for 30 min at room temperature with WT-L1 or WT-L9
( ) and CAM () membranes. The agonists epinephrine and clonidine
are shown in panels A and B, respectively, whereas panels C and D
depict the antagonists rauwolscine and idazoxan. Data represent the
mean ± S.E.M. of two (rauwolscine), three (epinephrine and
clonidine), or four to five (idazoxan) separate experiments performed
in duplicate. The rauwolscine data represents two experiments using the
WT-L1 membranes; five additional experiments using the WT-L9 membranes
gave similar results.
|
|
View this table:
[in this window]
[in a new window]
|
TABLE 2
Table of binding affinities and relative inverse agonist efficacies of
drugs
Ki values were calculated from IC50 values
determined by competition binding for 10 nM [3H]yohimbine in
the presence of 10 µM GppNHp (Fig. 2). Membranes were incubated for
30 min at room temperature in the presence of increasing concentrations
of the indicated drugs. Relative affinities are the CAM
Ki divided by the WT Ki for each
drug. Data are from two to seven separate experiments performed in
duplicate. EC50 values and maximum [3H]cAMP produced
were determined from dose-response curves for the indicated drugs using
whole cell adenylyl cyclase assays (Fig. 6). CAM cells were incubated
for 30 min at 37°C in the presence of 1 mM IBMX, 30 µM forskolin,
and increasing concentrations of the indicated drugs. Data are from
three to seven separate experiments performed in duplicate except for
phenoxybenzamine and prazosin, which are single experiments.
|
|
CAM Receptor Constitutively Inhibits cAMP Accumulation.
To
evaluate the functional activity of the CAM receptor and the effects of
potential inverse agonists, whole cell cAMP measurements were done.
Forskolin-stimulated [3H]cAMP production in CAM
cells was about 20 to 25% of that seen in either mock-transfected
(Neo) cells or in cells expressing the WT receptor, p < 0.01 for CAM versus Neo (Fig. 3, top).
The cAMP level in cells with the CAM receptor was similar to that observed with the WT receptor in the presence of the full agonist UK-14,304. Pretreatment with pertussis toxin decreased the cAMP production in our Neo cells by about 60%, and a similar effect was
seen with WT receptor expressing cells. In contrast, cAMP actually
increased 3-fold in the CAM cells upon PTX treatment, abolishing the
differences among the three cell types (Fig. 3, bottom, open bars).
This indicates that the low cAMP production from the constitutive
activity of the mutant was mediated via agonist-independent activation
of Gi and that WT receptor has minimal
constitutive activity on its own, despite the high-expression level (25 pmol/mg of protein). When the agonist UK-14,304 was added to WT
receptor-containing cells in the absence of PTX, cAMP production was
inhibited, however cAMP was stimulated by UK-14,304 in
pertussis-treated WT cells. This is consistent with previous reports of
dual coupling of 2A-AR to both
Gi and Gs (Eason et al.,
1992; Wade et al., 1999). In CAM cells, however, UK-14,304 stimulated
cAMP production both with and without pertussis pretreatment (Fig. 3).
This suggests that the Gi response is already
fully saturated in CAM cells before the agonist is added so only a
Gs response is observed. UK-14,304 had no effect
on adenylyl cyclase activity in mock-transfected (Neo) cells (Brink et
al., 2000).
View larger version (25K):
[in this window]
[in a new window]
|
Fig. 3.
Pertussis-sensitivity of transfected cell lines in
the presence or absence of agonist. Whole cell adenylyl cyclase assays
were performed on mock-transfected (Neo), WT, and CAM cells with
(bottom panel) or without (top panel) PTX pretreatment. Cells were
incubated with (filled bars) or without (open bars) 10 nM UK-14,304 for
30 min at 37°C in the presence of 1 mM IBMX and 30 µM forskolin.
Results are the mean ± S.E.M. of three separate experiments
performed in duplicate. Forskolin-stimulated [3H]cAMP
production in CAM cells was about 20 to 25% of that seen in Neo cells.
Values differing significantly from control (Neo without UK-14,304) are
marked, p < 0.05 (*), p < 0.01 (**).
|
|
To further define the mechanisms of the complex effects of agonists on
cAMP in the CAM and WT cells, epinephrine dose-response curves and
effects of pertussis and cholera toxins were examined. Epinephrine
showed a biphasic effect on cAMP production in CHO cells expressing the
WT 2A-AR; inhibition at 1 to 10 nM and a superimposed increase from 100 to 1000 nM (Fig.
4, top). The inhibition of adenylyl
cyclase activity was abolished by pretreatment of cells with pertussis
toxin revealing a pure stimulation (Fig. 4, top panel). This was very
similar to results previously reported with UK-14,304 in CHO cells
(Eason et al., 1992; Wade et al., 1999). The effects are mediated by
the 2A-AR and not an endogenous 
-AR as
there was minimal effect on cAMP production in Neo cells, and the
effects were blocked by yohimbine but not propranolol (Brink et al.,
2000). Similar results were found in the same cell line with UK-14,304
(Wade et al., 1999).
View larger version (28K):
[in this window]
[in a new window]
|
Fig. 4.
Agonist-mediated cyclase activity in WT and CAM
cells. Whole cell adenylyl cyclase assays were performed on WT (top
panel) or CAM (bottom panel) cells that had been pretreated with ()
or without ( ) PTX or with cholera toxin (). Cells were incubated
with increasing concentrations of epinephrine for 30 min at 37°C in
the presence of 1 mM IBMX and 30 µM forskolin. Data are the mean ± S.E.M. of two, three (WT + PTX), or four (CAM control) separate
experiments performed in duplicate or triplicate.
|
|
Epinephrine dose-response curves in cells expressing the CAM receptor
also indicate enhanced Gs activation by the CAM
2A-AR. Epinephrine caused an increase in
forskolin-stimulated cAMP accumulation both with and without pertussis
treatment (Fig. 4, bottom) apparently increasing adenylyl cyclase
activity via Gs. This was confirmed by cholera
toxin pretreatment after which there was no receptor-stimulated change
in cAMP accumulation with epinephrine. The potency for Gs activation in CAM cells was significantly
greater than in WT cells with EC50 values of 3.8 and 210 nM, respectively, in the presence of pertussis pretreatment.
The 50-fold increase in potency is greater than the observed difference
in epinephrine binding affinity for CAM and WT receptors (9-fold)
suggesting that the CAM receptor is more efficiently activating
Gs as well as Gi (see also
evidence for constitutive activation of Gs
described below).
Inverse Efficacies of 2-Adrenergic Antagonists.
We next looked at the effects of antagonists on forskolin-stimulated
cAMP accumulation in CAM cells to determine whether inverse agonist
activity would be observed. Rauwolscine was reported by Tian et al.
(1994) to have the greatest inverse agonist activity at
[35S]GTP
S binding in PC12 cells. Consistent
with that, we saw a striking reversal of the CAM receptor-suppressed
cAMP production by that drug. Cholera toxin pretreatment of CAM cells
did not affect the rauwolscine-mediated increase in cAMP accumulation (data not shown), but the increase was completely abolished by PTX
pretreatment (Fig. 5), evidence of the
Gi dependence of this response. Indeed there is a
small decrease in cAMP with rauwolscine in PTX-treated CAM cells
suggesting a small degree of constitutive activation of
Gs. The WT receptor showed strikingly different results. In contrast to the constitutive activity reported for the WT
rodent 2A-AR in PC12 cells (Tian et al.,
1994), we saw no increase in cAMP with rauwolscine with the WT porcine
2A-AR in our CHO cells (Fig. 5, open squares).
Thus despite very high levels of receptor expression (25 pmol/mg of
protein) there was no evidence with either rauwolscine (Fig. 5) or PTX
(Fig. 3) for constitutive activity of the WT receptor. Four of the five
competitive antagonists tested showed inverse agonist activity in which
the CAM receptor-suppressed cAMP production was significantly increased (Fig. 5, bottom). The sole neutral antagonist was idazoxan. That these
were inverse agonist effects and not agonist effects is evident since
the increase in cAMP was mediated by a PTX-sensitive Gi-dependent mechanism like that of rauwolscine
rather than a Gs-dependent mechanism like
epinephrine or UK-14,304 (Fig. 5, bottom).
View larger version (30K):
[in this window]
[in a new window]
|
Fig. 5.
Pertussis-sensitivity of inverse agonists in CAM
cells. Whole cell adenylyl cyclase assays were performed on cells for
30 min at 37°C in the presence of 1 mM IBMX and 30 µM forskolin.
Top panel, CAM cells pretreated with () or without () PTX and
untreated WT cells () were incubated with increasing concentrations
of rauwolscine. CAM data are the mean ± S.E.M. of two (PTX
treated) or seven (control) separate experiments; WT data are from
three separate experiments. Bottom panel, CAM cells that had been
pretreated with (filled bars) or without (open bars) PTX were incubated
with 10 µM of the indicated drugs. Data are the mean ± S.E.M.
of three to six separate experiments for untreated cells and one or two
separate experiments for PTX-treated cells. All experiments were
performed in duplicate.
|
|
Finally, we wanted to further characterize the inverse efficacy of a
series of 2-antagonists. Drugs were assayed
for their ability to stimulate cAMP production in forskolin-stimulated
CAM cells over a range of concentrations (Fig.
6 and Table 2). Antagonists examined for
their inverse agonist activity in whole cell adenylyl cyclase assays
displayed a rank order of efficacy of rauwolscine > yohimbine > RX821002 > MK912, whereas phentolamine and
idazoxan had little or no effect on cAMP production. Phenoxybenzamine, an irreversible -AR blocking agent, the
1-antagonist prazosin and propranolol, a
-AR antagonist, also had no effect on cAMP accumulation (Table 2).
View larger version (29K):
[in this window]
[in a new window]
|
Fig. 6.
Range of inverse efficacy of 2
antagonists. Whole cell adenylyl cyclase assays on CAM cells were
carried out for 30 min at 37°C in the presence of 1 mM IBMX, 30 µM
forskolin, and increasing concentrations of the indicated drugs. Data
are the mean ± S.E.M. of three to seven separate experiments
performed in duplicate.
|
|
A comparison of the binding affinities of the antagonists with their
inverse efficacy is revealing (Table 2). The
Ki values in this table are derived from
NLLSQ fits of averaged curves from the indicated number of competition
experiments. Rauwolscine showed the largest affinity difference and had
the greatest inverse efficacy, whereas idazoxan showed no difference in
affinity between CAM and WT receptors and was a neutral antagonist. The
other four inverse agonists, yohimbine, RX821002, MK912, and
phentolamine, had intermediate affinity differences. Because of the
small magnitude of the changes in binding affinity, extra replicates of
the rauwolscine and idazoxan experiments were done with more closely
spaced concentrations (three per decade) and the curves (seven for
rauwolscine and five for idazoxan) were analyzed individually for
statistical treatment. As with the fits of the pooled data, rauwolscine
showed a significant increase in Ki in each
individual experiment. The mean ratio of Ki
for CAM/WT was 2.24 ± 0.28, which was significantly different from 1.0 (p < 0.005, two-tailed one-sample
t test) whereas idazoxan had a ratio of 0.99 ± 0.15, which was not significantly different from 1.0 (p > 0.95). A theoretical analysis of the expected affinity differences due
to conformational changes in the extended ternary complex model is
presented in the Appendix. The magnitude of the Ki ratio and the degree of cAMP increase
indicates that approximately 50% of the CAM receptor is in the
R* state before agonist binding (see full analysis and
assumptions under Appendix).
A final point about the inverse agonists to note in Table 2 is the
difference between the Ki values for
binding competition and the EC50 values for the
increase in cAMP. In each case, the EC50 is
greater than the Ki (5- to 50-fold). This
is a somewhat unusual pharmacological behavior in that spare receptors
will lead to a "left-shift" of the dose-response curve compared
with the binding but in this case we have a "right-shift". Some of the difference may be due to different conditions of the two
assaysTris buffer with no sodium versus DMEM, which has sodium
chloridebut this seems unlikely as sodium chloride tends to increase
the affinity of antagonists at the 2A-AR
(Limbird et al., 1982). Thus the results seem more consistent with a
"threshold" behavior in which no response is seen until a
significant portion of the receptors is occupied. This could occur if
there were sufficient receptors activated by the CAM mutation to
produce a "spare receptor" phenomenon for adenylyl cyclase
inhibition. In this case, occupancy of 50% of the receptors by inverse
agonist would not be sufficient to reverse the spontaneous inhibition
by 50%. An even greater degree of receptor occupancy (say 80-90%)
might be required. In this case, the EC50 would
be significantly greater than the measured Kd. This type of mechanism would not be
surprising in the context of high-receptor expression, and a large
number of spare receptors previously demonstrated for the
2a-AR agonist response at the WT receptor
(Brink et al., 2000).
| |
Discussion |
We have used a constitutively active mutant of the
2A-AR stably expressed in CHO-K1 cells to
examine mechanisms of 2A-AR signaling. From
these studies, at least three new conclusions can be drawn. First, the
2A-AR T373K has enhanced signaling to both
Gi and Gs. Second, the
inverse efficacy of a series of 2-AR antagonists is examined, and a novel difference between idazoxan and
methyl-idazoxan (RX821002) has been found. This point is important for
interpreting physiological studies that use these two compounds. Finally, the fraction of active 2A-AR for the
T373K CAM mutant is approximately 50% for our whole cell cAMP
accumulation assay, whereas the WT receptor appears to have a very low
percentage of receptor active in the absence of agonist.
The effects of constitutively active receptor mutants on different G
proteins are not always concordant as reported for the 1-AR by Perez et al. (1996). Ren et al. (1993)
previously showed for the 2A-AR that the T373K
mutation adjacent to TM6 causes dramatically enhanced basal activation
of Gi, a result that we confirm here. We also
demonstrate enhanced activation of Gs by the
T373K mutant. This appeared as a modest degree of basal
Gs response with the T373K mutant (Fig. 5, filled
circles), but a more pronounced effect was seen on the
EC50 for epinephrine-induced Gs activation. The EC50 was
reduced >50-fold for the mutant versus WT whereas the
Kd was reduced less than 10-fold, indicating
enhanced Gs coupling. This does not appear to be
just a shift in activity for Gi versus
Gs since Gi effects were
eliminated in this experiment by PTX treatment. However, this is
difficult to evaluate quantitatively in part due to the fact that the
2A-AR has a much reduced ability to activate
Gs compared with Gi (Eason
et al., 1992; Brink et al., 2000). Wurch et al. (1999) found increased
Gz coupling by the T373K mutant in a transient
cotransfection system with mouse G15 in COS-7
cells using inositol phosphate production as their readout. Thus, the
T373K mutant of the 2A-AR appears to have a
generalized ability to activate both Gi and
Gs although quantitatively a comparison of the
degree of activation is not possible.
Interestingly, the pharmacological behavior of this basal
Gz activation was distinct from our results. For
adenylyl cyclase inhibition, we show a clear order of inverse efficacy
of rauwolscine > yohimbine > RX821002 > MK912 with
RX821002 having substantial inverse efficacy. Phentolamine and idazoxan
were neutral antagonists. In contrast, Wurch et al. (1999) reported
that the basal Gz-mediated PLC activation with
the T373K 2A-AR could not be attenuated by RX821002, MK912 or idazoxan. They did not, however, report results with
the most efficacious inverse agonists, rauwolscine or yohimbine. We
would have expected a significant reduction in activation of Gz by RX821002 if it behaved in a manner similar
to what we observe for Gi. Studying the rat
2D-receptor (which is an ortholog of the human
and porcine 2A-AR), Tian et al. (1994) used
[35S]GTPS binding in PC12 cells to show that
yohimbine, rauwolscine, phentolamine, and idazoxan were all inverse
agonists. They reduced basal GTPS binding by 30 to 40% but that
group did not test RX821002 or MK912. Interestingly, their ability to
detect constitutive signaling (and inverse agonist effects) was
abolished when sodium chloride was included in the assay.
For the endogenous 2C-receptor in HepG2 cells,
Cayla et al. (1999) found that treatment with RX821002 or yohimbine
resulted in a significant increase in receptor number but phentolamine did not. They concluded that RX821002 and yohimbine thus behaved as
inverse agonists, whereas phentolamine behaved as a neutral antagonist
in this system. Although this was a different receptor subtype and a
different experimental readout, their pharmacological profile
completely agrees with ours. Interestingly, we were not able to
demonstrate any significant changes in
2A-receptor number after treatment of either
WT or CAM 2A-AR with UK-14,304 or rauwolscine (data not shown). This difference may be due to the well known resistance of 2A-AR to internalization and the
substantial pool of 2C-AR, which is
intracellular in the absence of agonist (Daunt et al., 1997).
Thus several factors, such as the type of assay, receptor
subtypes, cell type, and local cellular G protein concentrations may
affect constitutive receptor activity and thus will be important for
detection of inverse agonist activity at a receptor subtype (for
review, see Pauwels and Wurch, 1998). Interestingly, the best
concordance of the pharmacological data mentioned above is between our
results with 2A-AR-mediated inhibition of cAMP
accumulation and the receptor up-regulation studies of Cayla et al.
(1999) with 2C-AR. Yohimbine and RX821002 were
inverse agonists in both studies. There is a direct contradiction
between our results and those of Tian et al. (1994) in that
phentolamine and idazoxan are clearly neutral antagonists in our hands.
In particular, idazoxan showed both neutral antagonist behavior in the
functional assay and absolutely no preference for R* in the
binding studies.
One of the other major questions that we address here is the
fraction of receptor that is active in the absence of agonist. Also, we
wanted to understand why CAM mutations have minimal effect on apparent
affinity of even the most efficacious inverse agonists. The two-state
ETC model has been frequently used to explain constitutive activation
and inverse agonists (Samama et al., 1993), and it would predict that
an inverse agonist must have a substantial difference in affinities for
R and R*. Although some recent data indicate that
either an induced fit model or multiple active receptor states may be
required to account for observations such as agonist-directed trafficking of receptor stimulus (Kenakin, 1995) or differential constitutive activation of signaling pathways (Perez et al., 1996), the
ETC model is still a useful starting point for analysis. Although a
lower affinity of inverse agonists for CAM receptors has been observed
(Costa and Herz, 1989; Samama et al., 1994), the effects were very
small (2-fold), and numerous other studies have not reported such an
effect (Kjelsberg et al., 1992; Ren et al., 1993). In our theoretical
examination of this question (see Appendix), we show that
the expected changes in antagonist affinity are indeed modest and
depend on the degree to which the receptor is spontaneously in the
active state (i.e., depends on L, the equilibrium constant governing the R to R* equilibrium). Only if a
very large fraction of the receptor (i.e., >90%) is spontaneously in
the R* state would you expect to see a large
affinity shift of an inverse agonist for a WT versus CAM receptor. The
approximately 2-fold shift that we see for rauwolscine is consistent
with approximately half of the CAM receptor being in the R*
state (see Appendix for details). Furthermore, the lack
of inverse agonist effect with the WT
2A-AR despite very high expression indicates
that a very small percentage of the WT receptor is active in the
absence of agonist. This is in contrast to the
2-AR for which the WT receptor appears to have
approximately 7% of the activity of the CAM mutant (Samama et al.,
1993).
This very low level of constitutive activity of the WT
2A-AR seems in conflict with results of Tian
et al. (1994). They used PC-12 cells stably expressing a cloned rat
2D-AR to look at the effects of rauwolscine on
[35S]GTPS binding to membrane preparations.
The 2D-AR is the rodent ortholog of the human
or porcine 2A-AR. They found that rauwolscine was able to decrease basal [35S]GTPS binding
and that this decrease was dependent on both the level of receptor
expression and upon sodium concentration in their assay (as noted
above). Furthermore, their pharmacological profile of inverse efficacy
was very different from ours. There are many potential explanations for
the differences between our results and theirs: 1) the different
species of origin of the receptor (rat versus pig), 2) different cell
types used (CHO versus PC12), 3) the different readout of the assay
(GTPS binding versus adenylyl cyclase inhibition), and 4) the
presence of sodium in our intact cell cAMP accumulation assays, which
was absent from their nucleotide binding studies. Sodium, which is
present in intact systems, has been shown to suppress basal activity
for opioid receptors (Costa et al., 1990).
A final observation relates to different inverse efficacies of
closely related imidazoline compounds. A role has been postulated for a
novel imidazoline I1 type receptor in mediating
many effects of clonidine and other imidazoline-containing
2 agonists (Ernsberger and Haxhiu, 1997). One
pharmacological distinction between imidazoline receptor effects and
those of 2-AR has been the difference between effects of idazoxan and its methyl-substituted congener RX821002. This
difference has been ascribed to selectivity of RX821002 to bind to the
2-AR but not to the putative
I1 receptor. In contrast, idazoxan binds to both
types of sites (Meana et al., 1997). Interestingly in our study,
RX821002 (2-methoxy idazoxan) is a fairly efficacious inverse agonist
whereas idazoxan is a neutral antagonist. Although different types of
evidence have pointed to the I1 receptor as the
mediator of imidazoline drug-induced physiological effects, differences
between the actions of RX821002 and idazoxan or other compounds must
now take into account the relative inverse efficacy of these drugs at
the 2A-AR.
In conclusion, we describe the relative inverse efficacies of a series
of 2A-AR antagonists and the relation of
inverse efficacies to binding properties. We provide new information
both about 2A-adrenergic receptor
conformational regulation as well as potentially important pharmacological distinctions among different
2A-AR antagonists.
Although it is clear that constitutively activated receptors have
a greater fraction of receptor in the active state in the absence of
agonist than do wild-type receptors, in most cases it has not been
determined what fraction of receptors are active in the CAM receptor.
The extended ternary complex model describes the relation between
ligand affinity for the two states of a receptor and the conformational
changes of the receptor, which occur upon ligand binding. In the
simplest version of this model2 (Fig.
7), there are two receptor states:
inactive, R, and active, R*. Since the affinity
of an inverse agonist is lower for R* than for R,
we may be able to use changes in inverse agonist binding to
estimate the fraction of a CAM receptor in the R* state.
This analysis is based on the assumption that the mechanism of
constitutive activation is a change in the equilibrium between the
R and R* states without a significant change in
the microscopic equilibrium constant for ligand binding to the basal
receptor state R (K). In addition to the changes
in antagonist binding, agonist binding affinities may also
provide information about the fraction of active receptor. However, the
agonist binding analysis may be complicated by the profound effects of
G protein coupling on agonist binding and by the fact that agonist
itself will increase the fraction of R*.
What is the expected binding of an inverse agonist to a CAM
receptor compared with its binding to a WT receptor? There are two
parameters that determine both ligand binding and the amount of active
receptor R* in the presence of ligand (i.e., the initial equilibrium between the active and inactive conformations,
L = R*/R, and the ratio of
affinities of the ligand for the active and inactive state,
K'/K). Two assumptions that we make for this analysis are: 1) that the only mechanism by which the inverse agonist
effects a change in receptor activity is by its differential affinity
(K'/K) for the active (R*) and
inactive (R) states of the receptor, and 2) that the only
difference between the WT and CAM receptor is a different value of
L, the parameter describing the equilibrium between the
active and inactive state in the absence of ligand.
We also must examine the effect of an inverse agonist on
receptor activity. We define the fraction of receptor that is active in the absence of ligands to be
We can also put an upper limit on the fraction of WT receptor in
the active state. We recently showed that the L1 cell line exhibits a
receptor reserve of approximately 103 for
UK-14,304 (Brink et al., 2000). Thus activation of ~0.1% of
receptors can produce a 50% inhibition of cAMP accumulation. Based on
the PTX and rauwolscine results, there appears to be little
(conservatively <20%) inhibition of cAMP accumulation by the WT
receptor in this line. This suggests that the amount of spontaneously
active receptor may be as little as ~ 0.04% [i.e., <(20%/50%) × 0.1%] in the absence of agonist.
Supported by National Institutes of Health HL46417. Production
and flow cytometry screening of the mutant receptors received assistance from UM-MAC, National Institutes of Health P60-AR20557.
GPCR, G protein-coupled receptor;
CAM, constitutively active mutant;
ETC, extended ternary complex;
WT, wild-type;
AR, adrenergic receptor;
5-HT, 5-hydroxytrytamine;
PTX, pertussis toxin;
IBMX, isobutylmethylxanthine;
HA, hemagglutinin;
CHO, Chinese hamster ovary;
DMEM, Dulbecco's modified Eagle's medium;
GppNHp, 5'-guanylyimidodiphosphate;
NLLSQ, non-linear least squares
regression.
![[Feedback]](/icons/banner/feedbackACT.gif){kind=icon}
![[For Subscribers]](/icons/banner/subscriberACT.gif){kind=icon}
![[Archive]](/icons/banner/archiveACT.gif){kind=icon}
![[Search]](/icons/banner/searchACT.gif){kind=icon}
![[Contents]](/icons/banner/tocACT.gif){kind=icon}
2A-Adrenergic
Receptor
Top
Abstract
Introduction
![=[(1+L<SUB><UP>CAM</UP></SUB>)/(K+L<SUB><UP>CAM</UP></SUB> · K′)]/[(1+L<SUB><UP>WT</UP></SUB>)/(K+L<SUB><UP>WT</UP></SUB> · K′)]](/content/vol59/issue3/fulltext/532/img010.gif)
![R*<SUB>A=∞</SUB>/R*<SUB>A=0</SUB>=[L · K′/(K+L · K′)]/[L/(1+L)]](/content/vol59/issue3/fulltext/532/img020.gif)
![=[L · (K′/K)/(1+L · (K′/K))]/[L/(1+L)]](/content/vol59/issue3/fulltext/532/img021.gif)
