Mutation of Asn111 in the Third Transmembrane Domain of the AT1A Angiotensin II Receptor Induces Its Constitutive Activation*

(Received for publication, August 14, 1996, and in revised form, October 21, 1996)

Thierry Groblewski Dagger §, Bernard Maigret , Renée Larguier Dagger , Colette Lombard Dagger , Jean-Claude Bonnafous Dagger par and Jacky Marie Dagger

From Dagger  INSERM U.401, CCIPE, 141 rue de la Cardonille, 34094 Montpellier Cedex 05, France and the  Laboratoire de Chimie Théorique, Université de Nancy I, BP 239, 54506 Vandoeuvre-les-Nancy Cedex, France

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION AND CONCLUSION
FOOTNOTES
REFERENCES


ABSTRACT

A preliminary model of the rat AT1A angiotensin II (AII) receptor (Joseph, M. P., Maigret, B., Bonnafous J.-C., Marie, J., and Scheraga, H. A. (1995) J. Protein Chem. 14, 381-398) has predicted an interaction between Asn111 located in transmembrane domain (TM) III and Tyr292 (TM VII) in the nonactivated receptor; a disruption of this interaction upon AII activation would allow Tyr292 to interact with the conserved Asp74 (TM II). The previous verification that Tyr292 is essential for receptor coupling to phospholipase C (Marie, J., Maigret, B., Joseph, M. P., Larguier, R., Nouet, S., Lombard, C., and Bonnafous, J.-C. (1994) J. Biol. Chem. 269, 20815-20818) prompted us to check the possible alterations in receptor properties upon Asn111 right-arrow Ala mutation. The mutated receptor (N111A) displayed: (i) strong constitutive activity, with amplification of the maximal phospholipase C response to AII; (ii) agonist behavior of the AT2-specific ligand CGP 42112A, [Sar1,Ile8]AII, and [Sar1,Ala8]AII, antagonists of the wild-type receptor; (iii) inverse agonism behavior of the non-peptide ligands DuP 753, LF 7-0156, and LF 8-0129. The results are discussed in the light of the allosteric ternary complex models and other described examples of constitutive activation of G protein-coupled receptors.


INTRODUCTION

Constitutive activation of G protein-coupled receptors, initially reported by Cotecchia et al. (1) for the alpha 1-adrenergic receptor, is now well documented and has been extended to many other members of this large family (2-21). Moreover, mutations inducing receptor constitutive activation have been found to be associated with human diseases (13-16). Data on the beta 2-adrenergic receptors have prompted their authors to propose an extended version of the ternary complex model, based on the existence of active and inactive receptor states (4, 22). The same mechanistic model, either in its initial form (22) or in a refined version (23), have provided interpretations for the "negative antagonism" or "inverse agonism" phenomenon, evidenced for ligands of beta 2-adrenergic (24, 25), B2 bradykinin (26), m5 muscarinic (21), and thyrotropin-releasing hormone (18) receptors. As emphasized by the recent work of Cotecchia's group on the alpha 1B-adrenergic receptor (8), a correlation between mechanistic considerations and molecular events associated to receptor conformational changes is obviously required. The work reported in the present paper is based on a previous molecular modeling study (27) which aimed at predicting modifications of specific amino acid side chain interactions during the process of the angiotensin II type 1 (AT1)1 receptor activation. This preliminary model (27) postulated that an interaction between Asn111 (TM III) and Tyr292 (TM VII) might exist in the non-activated receptor and that activation by AII would induce its disruption to allow Tyr292 to interact with the conserved Asp74 (TM II). Previous experimental work from this laboratory is consistent with an essential role of a Tyr292-Asp74 interaction in the transduction mechanism (28). The model prompted us to check whether the absence of Asn111 would favor this interaction, leading to constitutive receptor activity. In this paper we demonstrate that the N111A mutant receptor displays a strong constitutive activity as well as striking pharmacological changes. The results are discussed in the light of above-mentioned current models (22, 23).


MATERIALS AND METHODS

Reagents

AII, [Sar1]AII, [Sar1,Ile8]AII, and [Sar1,Ala8]AII were purchased from Bachem (Budendorf, Switzerland). CGP 42112A was provided by Drs. M. De Gasparo and S. Bottari (Ciba Geigy, Basel, Switzerland). Non-peptide antagonists LF 7-0156, LF 8-0129, and DUP 753 were synthesized by Fournier Laboratories (Daix, France). AII, [Sar1]AII, and CGP 42112A were radioiodinated as described previously in Refs. 29 and 30, respectively. myo-[2-3H]Inositol was from DuPont NEN. COS-7 cells were from the European Cell Type Collection.

Site-directed Mutagenesis and Expression

The amino acid mutation Asn111 right-arrow Ala was carried out as described previously (28). The cDNA sequences of the wild type and N111A mutant rat AT1A receptors were subcloned in the XbaI site of the polylinker of the eukaryotic expression vector pCMV (31). Receptors were transiently expressed in COS-7 cells by using the electroporation transfection method: 107 cells were resuspended in 300 µl of electroporation buffer (50 mM K2HPO4, 20 mM CH3COOK, 20 mM KOH, pH 7.40) and incubated for 10 min at room temperature in an electroporation cuvette (0.4-cm electrode gap, Bio-Rad) with 20 µg of pCMV carrier and different amounts of pCMV containing cDNA receptors sequences (30-300 ng range). They were submitted to an electric discharge (950 microfarads, 280 V, 50 ms), then cultured for 2 days at 37 °C in Dulbecco's modified Eagle's medium, 4.5 g/liter glucose, 10% fetal calf serum, 100 units/ml penicillin, 100 µg/ml streptomycin before binding or IP accumulation experiments.

Binding Assays

Plasma Membrane

Crude membranes from COS-7 cells transiently expressing the wild type or mutant AT1A receptors were prepared according to Ref. 28. Protein concentrations were measured as described in Ref. 32. 125I-AII or 125I-CGP 42112A binding assays were performed as described previously (33). In some experiments involving GTPgamma S treatment, the membranes were washed three times with binding buffer (50 mM Na2HPO4, 5 mM MgCl2, 1 mg/ml bovine serum albumin, 1 mg/ml bacitracin, pH 7.40) supplemented with 200 mM NaCl, incubated for 10 min at 30 °C in the presence or absence of 100 µM GTPgamma S before binding experiments carried out in the same medium.

Intact Cells

125I-[Sar1]AII binding to transfected COS-7 cells grown in 6-well tissue culture clusters (5 × 105 cells/well) was effected as in Ref. 28.

Inositol Phosphate Assays

COS-7 cells expressing the wild type or N111A mutant receptors were grown in 6-well tissue culture clusters and labeled for 24 h with [2-3H]inositol (1.5 ml/well, 1 µCi/ml) in minimum essential medium deprived of serum and unlabeled inositol. Before stimulation, cells were incubated at 37 °C for 1 h in Dulbecco's phosphate-buffered saline (pH 7.40). After a 15-min LiCl treatment, cells were incubated in the presence or absence of peptide ligands for 15 min at 37 °C in Dulbecco's PBS supplemented with 10 mM LiCl, 1 mg/ml bovine serum albumin, and 1 mg/ml bacitracin. LiCl was omitted in short-time [Sar1]AII stimulation experiments (15 and 30 s). For experiments involving non-peptide ligands, cells were incubated, after the 1-h PBS incubation, in the presence or absence of non-peptide compounds for 30 min at 37 °C in Dulbecco's PBS supplemented with 10 mM LiCl and 0.1 mg/ml bacitracin without LiCl pretreatment. Pooled inositol phosphates (IPs) were extracted and measured as described previously (28, 34).


RESULTS

Constitutive Activation of the N111A Mutant AT1A Receptor

The detailed analysis of basal inositol phosphate production, in the presence of Li+ ions, by the WT or N111A receptors transiently expressed in COS-7 cells revealed strong constitutive activation of the N111A mutant AT1A receptor (Fig. 1A). A significant difference between basal IP production by the WT and the N111A mutant receptors was detected for expression levels of about 105 sites/cell. This constitutive activation might be overlooked in the cases of lower expression levels. In this respect, the electroporation technique is well adapted to the provision of homogeneous cell transfection over a wide range of expression levels. The maximal extent of [Sar1]AII stimulation of IP production was greatly potentiated in the N111A mutant receptor (Fig. 1B). This potentiation was evident at stimulation times as short as 15 s (Fig. 1C), which indicates that it resulted from an intrinsic activation property of the receptor rather than desensitization or sequestration phenomena. In addition, these short-time experiments carried out in the absence of Li+ ions showed that the steady-state levels of IPs are similar in the WT and mutant receptor (Fig. 1C, t = 0), the constitutive activation requiring the addition of IP1 phosphatase inhibitors. The Kact value for the N111A mutant receptor was not significantly altered: 2.88 ± 1.03 nM versus 1.03 ± 0.40 nM for the WT receptor (Fig. 2) which is consistent with Kd values for [125I-Sar1]AII binding (1.1 ± 0.2 nM and 0.76 ± 0.10 nM for N111A and WT receptors, respectively) (35). In order to dissect the changes in receptor coupling properties upon Asn111 right-arrow Ala replacement, we checked the effect of GTPgamma S, a non-hydrolyzable analog of GTP, on the affinities of the WT and mutant receptor for 125I-AII. The expected decreased in WT receptor affinity (increase in Kd value from 1.34 ± 0.23 nM to 4.31 ± 0.65 nM) was no longer observed for the constitutively active mutant receptor (Kd values: 2.12 ± 0.36 nM and 1.84 ± 0.11 nM in the absence and presence of GTPgamma S, respectively) (Fig. 3). These data concerning the comparison of binding affinities and Kact values for the WT and N111A receptors (which contrast with other examples of constitutive activation of G protein-coupled receptors (1, 3-5, 7, 18, 21)) and the effects of GTPgamma S treatment on agonist binding will be discussed later in the light of published mechanistic models (22, 23).


Fig. 1. Constitutive activation of the N111A mutant AT1A receptor. Amplification of the [Sar1]AII response. The WT and N111A mutant receptors were transiently expressed, at variable levels, in COS-7 cells, and the basal or [Sar1]AII-stimulated levels were determined, as described under "Materials and Methods." The levels of receptor expression in B and C were 4.4 × 105 and 5.3 × 105 sites/cell for WT and N111A receptors, respectively. Each experimental measurement was performed in triplicate. The data are representative of four separate experiments. A, basal activities as a function of receptor expression level. B, extent of IP production stimulation by saturating doses of [Sar1]AII (1 µM). C, time course of [Sar1]AII amplification of IP production. After a 1-h equilibration period in PBS buffer, cells were stimulated by 1 µM [Sar1]AII for 15 or 30 s without any LiCl added. The steady-state IP levels (t = 0) are obtained by direct IP extraction as described under "Materials and Methods."
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Fig. 2. Dose-dependent [Sar1]AII stimulation of IP production for WT and N111A mutant AT1A receptors. The stimulation of IP production by various concentrations of [Sar1]AII was analyzed in COS-7 cells expressing the WT or N111A mutant receptors (expression levels: 1.2 × 105 and 1.5 × 105 sites/cell, respectively) as described under "Materials and Methods." The calculated Kact values were 1.03 ± 0.40 nM and 2.88 ± 1.03 nM for WT and N111A receptors, respectively (mean of three independent experiments).
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Fig. 3. Effect of GTPgamma S treatment on the affinities of 125I-AII for the WT and N111A mutant receptors. Membranes from COS-7 cells expressing the WT and N111A mutant receptors were pretreated and incubated for 10 min at 30 °C in the presence of 100 µM GTPgamma S before determination of their 125I-AII binding parameters by Scatchard analysis. The measured Kd values are indicated in the figure. The presented typical experiment is representative of three separate experiments. Each assay was performed in triplicate.
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Changes in Pharmacological Properties of the AT1A Receptor upon Asn111 right-arrow Ala Mutation

We noted earlier (35) that the N111A mutant receptor displayed an increased affinity for the AT2-specific ligand CGP 42112A. Direct binding of 125I-CGP 42112A to membranes from COS-7 cells expressing the N111A mutant receptor led to a Kd value of 96 nM, in agreement with a previously determined Ki value (35). Moreover, CGP 42112A displayed a marked partial agonist activity for the N111A mutant receptor (maximal response: 27% of the response to [Sar1]AII) (Fig. 4A) with a Kact value of 42 nM (Fig. 4C). The other peptidic compounds [Sar1,Ile8]AII and [Sar1,Ala8]AII, which possess unchanged affinities for the mutant receptor (35) and are devoid of agonist activity for the recombinant WT receptor, also behaved as partial agonists for the N111A mutant (Fig. 4A) (maximal activities: 52% and 27%, respectively, of the response induced by [Sar1]AII). We previously demonstrated that Asn111 right-arrow Ala replacement induced a strong decrease in receptor affinity for all tested non-peptide ligands: DUP 753, LF 7-0156, LF 8-0129 (35). In spite of these reduced affinities, we could check the ability of these ligands to modulate the IP responses of the WT and N111A mutant receptors. While the activity of the WT receptor was not significantly affected, a marked decrease in IP production was observed upon treatment with the three non-peptide ligands (Fig. 4B). These inverse agonism properties were characterized by Kact values of 2.4 µM, 0.40 µM, and 0.38 µM for DUP 753, LF 7-0156, and LF 8-0129, respectively (Fig. 4C).


Fig. 4. Agonism properties of peptides and inverse agonism properties of non-peptide ligands induced by Asn111 right-arrow Ala replacement in the AT1A receptor. The effects of peptide and non-peptide ligands on IP production were evaluated on the WT and N111A mutant AT1A receptors, transiently expressed in COS-7 cells, as described under "Materials and Methods." The data are representative of three separate experiments performed in triplicate. A, agonist properties of [Sar1,Ile8]AII, [Sar1,Ala8]AII, and CGP 42112A. Maximal doses of the peptides (1 µM) were added after the initial equilibration in Li+-containing medium. B, inverse agonism properties of DUP 753, LF 7-0156, and LF 8-0129. Saturating doses (10 µM) of the non-peptide ligands were added at the beginning of the Li+ equilibration period. Expression levels in A and B were 4.4 × 105 and 5.3 × 105 sites/cell for the WT and N111A receptors, respectively. C, dose-dependent stimulation or inhibition of IP production by peptide and non-peptide ligands in COS-7 cells expressing the N111A receptor. Experiments were carried out as described in A for CGP 42112A and B for non-peptide derivatives, using variable ligand concentration. The expression level of the N111A receptor was 4.9 × 105 sites/cell. The Kact values were 42 nM for CGP 42112A, 2.4 µM for DUP 753, 0.38 µM for LF 7-0156 and 0.4 µM for LF 8-0129.
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DISCUSSION AND CONCLUSION

The data reported in this paper demonstrate striking changes in the properties of the rat AT1A receptor induced by Ala replacement of the Asn111 residue, located in the third transmembrane domain: constitutive activation of basal IP production and amplification of the response to angiotensin II; induction of inverse agonism properties of the non-peptidic ligands DUP 753, LF 7-0156, and LF 8-0129, evidenced in spite of their greatly decreased affinities for the mutated receptor (35); induction of partial agonist properties of the AT2-specific peptide ligand CGP 42112A, associated with an increased affinity, as well as [Sar1,Ile8]AII and [Sar1,Ala8]AII derivatives which are antagonists of the wild-type receptor.

We tried to correlate these observations with mechanistic interpretations of the "allosteric ternary complex" models previously proposed by Lefkowitz's group (22) and discussed and refined by Kenakin (23) (Fig. 5). Classical simulation curves (not shown) (4) easily demonstrated that the various changes associated with Asn111 right-arrow Ala replacement are thermodynamically consistent with multiple combined variations of the parameters describing the equilibria between the involved entities. Appropriate choices of these parameters can explain: the constitutive activation associated with an increase in maximal response to AII, without significant changes in Kd and Kact values; the lack of GTPgamma S effect on the affinity of the mutant receptor for AII which is a function of the Rright-arrowR* isomerization and the affinity of R* for G; the above-mentioned pharmacological changes, the latter providing verification that the parameters alpha  and/or beta  and or gamma  (Fig. 5) have been affected by the mutation.


Fig. 5. Allosteric ternary complex model of ligand interaction with a G protein-coupled receptor. This model proposed by Kenakin (23) is a refinement of the initial model of Lefkowitz et al. (22). Parameter definition has been transposed according to Ref. 22: alpha , beta , and gamma  parameters help to define the agonist, antagonist, or inverse agonist properties of ligands; J characterizes the isomerization equilibrium between inactive and active receptor conformations in the absence of ligand. The ability of the receptor to induce signal transduction is function of R*G for basal activity (with possible constitutive activation) and R*G + LR*G for ligand modulated activity.
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As a consequence of the variations of one or several of these parameters, the Kd values relative to the hormone recognition by mutated receptor may vary in unpredictable directions. Previous interpretations of decreases in Kd values for mutated receptors displaying constitutive activity were based on the assumption that these parameters were unaffected by the mutations (22).

However, the model depicted in Fig. 5 is oversimplified, as earlier discussed (23) and as emphasized by the recent evidence for the existence of multiple activation states of the alpha -1B adrenergic receptor (7). Obviously, more precise interpretations would imply the experimental availability of the subtle conformational changes involved in receptor activation processes.

In spite of the obvious limitations of models based on the structure of bacteriorhodopsin, the preliminary model of the AT1A receptor activation (27), which prompted us to investigate a possible role of Asn111, constitutes a first step in the prediction of these conformational changes: AII receptor activation would cause a disruption of an Asn111-Tyr292 interaction, allowing Tyr292 to interact with Asp74 (Fig. 6). Recent experiments from our laboratory support a possible role of Tyr292-Asp74 interaction in receptor activation (28). The results are consistent with the existence, in the wild-type receptor, of an intramolecular bond between Asn111 and another residue; the absence of this interaction in the N111A mutant receptor could favor conformational flexibility and constitutive activation (Fig. 6). Although the model (27) suggests that Tyr292 is a likely candidate to interact with Asn111, it is difficult at the present time to exclude the possibility that one (or several) other amino acid(s) might act as (a) relay(s) in the cascade of conformational changes leading to receptor coupling to a specific G protein.


Fig. 6. Molecular modeling of WT and N111A AT1A receptors. The model of N111A mutant receptor has been built by Asn111 right-arrow Ala replacement in the previously described model of WT receptor (27). The model of WT receptor (left panel) predicts a possible hydrogen bond between Asn111 and Tyr292 in the non-activated receptor, the hormone activation resulting in disruption of this interaction to allow Tyr292 to interact with Asp74. Suppression of Asn111 (right panel) would favor this latter interaction in the absence of hormone, thus inducing constitutive activation. A molecular dynamic study has been shown to be consistent with this hypothesis (Silicon Graphics Indigo2 workstation, DISCOVER 95.0 software; non-bonded cut-off distance: 12 Å, dielectric constant epsilon  = 1·r; C-alpha fixed; dynamic run: 80 ps, 310 K).
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Many examples of constitutive activity of G protein-coupled receptors have been reported. It appeared possible to induce constitutive activation of numerous members of this family by mutation of amino acids located at various receptor positions (1-21). The problem of molecular event conservation in activation processes of GPCR is raised. It can be envisaged that some of these events are conserved, while others are specific to some receptors or some subfamilies. A recent work on the alpha -1B receptor has emphasized the role of conserved polar amino acids in receptor activation, the mutation of some of these residues leading to constitutively active receptors. The dissection of conformational changes underlying receptor activation and the prediction of the molecular nature of receptor-activated states have been attempted through the use of molecular dynamics (8). The Asn111 residue of the AT1A receptor, the mutation of which induces constitutive activation, is found at homologous positions in other peptide hormone receptors: AT2 and Xenopus angiotensin receptors, bradykinin, opiod, interleukin 8, and somatostatin receptors for instance. It is noticeable that mutation of Cys128 (7) in the alpha -1B adrenergic receptor, which occupies a position homologous to that of Asn111 in the AT1A receptor, also induces constitutive activation. Tyr292 of the AT1A receptor, which is postulated to interact with Asn111 in the non-activated receptor (27), is not conserved in all GPCR. More direct proof for Asn111-Tyr292 interaction are obviously required, even if the lack of tyrosine conservation is not necessarily inconsistent with the model. Nevertheless, in the absence of high resolution crystallographic data for GPCR, mutagenesis experiments which lead to constitutive activation can support hypotheses about receptor stabilization through interaction between specific residues and their rearrangements upon hormonal activation. Data about rhodopsin (10, 11) suggest that disruption of a critical salt bridge between Lys296 (TM VII) and Glu113 (TM III) induces constitutive activation. They provide insight into structural features inasmuch as they can provide information on the relative spatial positions of the transmembrane alpha  helices and interactions between them.


FOOTNOTES

*   This work was supported in part by INSERM, CNRS, Laboratoires Fournier (Daix, France), and the Ministère de l'Enseignement Supérieur et de la Recherche. The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
§   Supported by fellowships from the Ministère de l'Enseignement Supérieur et de la Recherche and the Association pour la Recherche contre le Cancer (ARC).
par    To whom correspondence should be addressed: INSERM U.401, CCIPE, 141 rue de la Cardonille, 34094 Montpellier Cedex 05, France. Tel.: 33-4-67142919; Fax: 33-4-67542432.
1    The abbreviations used are: AT1 receptor, type 1 angiotensin II receptor; AT2 receptor, type 2 angiotensin II receptor; AII, angiotensin II; Sar, sarcosine; GTPgamma S, guanosine 5'-O-(3-thiotriphosphate); IP, inositol phosphate; PBS, phosphate-buffered saline; WT, wild type; TM, transmembrane domain; GPCR, G protein-coupled receptor.

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