Abstract
Transmembrane domains (TMDs) I, II, and VII of the β2-adrenergic receptor (β2AR) were replaced, individually or in combination, with the corresponding regions of the β1AR, and vice versa. The β2-selective binding of salmeterol was not affected by the exchange of TMD I between the β1- and β2ARs. The affinity of salmeterol was slightly decreased (32-fold) by replacement of TMD II of the β2AR with the homologous region of the β1AR; the affinity was strongly decreased (1870-fold) for the β2AR with TMD VII of the β1AR. The affinity of salmeterol was partially restored by the introduction of TMD VII, but not TMD II, of the β2AR into the β1AR. By analyzing alanine-substituted mutants, we found that Tyr308 in TMD VII was mainly responsible for the high affinity binding of salmeterol. Two salmeterol derivatives with the ether oxygen at different positions in the side chain showed 33- and 64-fold decreased affinities for the wild-type β2AR, and a derivative with no ether oxygen showed 147-fold decreased affinity for the wild-type β2AR. These results indicate that Tyr308 in TMD VII is the major amino acid conferring the β2-selective binding of salmeterol to the β2AR and that the position of the ether oxygen in the side chain is also important for β2-selective binding. A three-dimensional model of the salmeterol-β2AR complex shows that the phenyl group of Tyr308 interacts with methylene groups near the protonated amine of salmeterol and the ether oxygen interacts with Tyr316.
The βARs belong to a family of G protein-coupled receptors and have been analyzed as prototypes of these receptors. The binding of agonists induces conformational changes, leading to functional coupling with G proteins. The ligand binding site of the βARs has been extensively characterized by a variety of techniques (Savarese and Fraser, 1992;Strader et al., 1994). Deletion mutagenesis experiments have shown that the hydrophilic intracellular and extracellular loops connecting the seven hydrophobic domains of the β2AR are not required for ligand binding (Dixonet al., 1987). The findings indicated that the ligand binding domain of the β2AR is located within the hydrophobic TMD of the β2AR. Site-directed mutagenesis experiments have revealed the amino acids and regions of the β2AR that are important for ligand binding and G protein coupling (Dohlman et al., 1988; Wong et al., 1988; Hockerman et al., 1996). Several key residues were identified by analyzing point-mutated β2ARs; Asp113 in TMD III interacts with the protonated amine of the agonists, and two serine residues in TMD V (Ser204 and Ser207) form hydrogen bonds with the meta- andpara-hydroxyl groups of the catechol ring (Strader et al., 1988, 1989).
Binding domains of subtype-selective ligands [i.e., β1- and β2-selective antagonists and a slightly selective agonist (norepinephrine)] have been analyzed by several groups. Frielle et al. (1988)reported that TMDs VI and VII of the βAR seem to be important for the high affinity binding of the β1-selective antagonist betaxolol and the β2-selective antagonist ICI118551. Those authors also showed that the β1-selectivity of norepinephrine is largely determined by TMD IV of the β1AR. Dixonet al. (1989) reported that TMD IV of the β1AR is responsible for the β1-selective binding of norepinephrine. Marulloet al. (1990) reported that single TMDs cannot be responsible for the high affinity binding of β1- and β2-selective antagonists, based on examination of β1- and β2AR CHs. However, those authors did not examine the binding domains of β1- and β2-selective agonists. Therefore, domains responsible for the high affinity binding of subtype-selective agonists have not been examined.
Salmeterol is a derivative of salbutamol with an aralkyloxyalkyl substitution at the amine group; it has a long duration of action and high selectivity for the β2AR (Johnson, 1995).Green et al. (1996) recently revealed that the anchoring region of salmeterol, referred to as the “exosite,” is located in the inner part of TMD IV and accounts for the long duration of action. However, it has not been determined which region of the β2AR is involved in the subtype-selective binding of salmeterol.
In this study, we examined the TMDs and the key amino acids that are responsible for the β2AR selectivity of salmeterol and we investigated the role of the ether oxygen in the side chain of salmeterol. We found that Tyr308 in TMD VII was the major amino acid determining the high affinity binding of salmeterol and that the position of the ether oxygen in the side chain was also important for β2-selective binding. We built a three-dimensional model of the salmeterol-β2AR complex to account for this structural information.
Experimental Procedures
Materials.
Salmeterol and salmeterol derivatives were kindly synthesized and provided by the Lead Optimization Research Laboratory, Tanabe Seiyaku (Saitama, Japan). Thermus aquaticus andPyrococcus furiosus DNA polymerases were obtained from Takara (Shiga, Japan) and Stratagene (La Jolla, CA), respectively.125I-CYP was obtained from Amersham Pharmacia Biotech (Arlington Heights, IL). (±)-Propranolol and DEAE-dextran were obtained from Sigma Chemical (St. Louis, MO). The plasmids encoding the human β1- and β2ARs were kindly provided by Dr. R. J. Lefkowitz (Duke University, Durham, NC). The mammalian expression vector pEF-BOS was a gift from Dr. S. Nagata (Osaka University, Osaka, Japan).
Construction of chimeric β1/β2ARs and alanine-substituted β2AR mutants.
Chimeric β1/β2ARs were constructed by polymerase chain reaction, as described (Kikkawaet al., 1998). TMDs I, II, and VII of the β2- or β1AR were exchanged with homologous regions of the β1- or β2AR, respectively. The structures of these CHs are shown in Fig. 1. The positions and amino acids of the junctions for individual chimeric β1- and β2ARs are as follows: CH-1, β1Met1–Ala84/β2 Lys60–Leu413; CH-2, β2 Met1–Phe71/β1Ile97–Cys131/β2 Glu107–Leu413; CH-3, β2 Met1–Val295/β1Lys347–Pro381/β2 Asp331–Leu413; CH-4, β2 Met1–Phe71/β1Ile97–Cys131/β2Glu107–Val295/β1Lys347–Pro381/β2 Asp331–Leu413; CH-5, β2 Met1–Ala59/β1Lys85–Val477; CH-6, β1Met1–Phe96/β2Ile72–Cys106/β1 Glu132–Val477; CH-7, β1 Met1–Val346/β2His296–Pro330/β1 Asp382–Val477; CH-8, β1 Met1–Phe96/β2Ile72–Cys106/β1Glu132–Val346/β2His296–Pro330/β1 Asp382–Val477. Alanine-substituted mutants of the β2AR were constructed by polymerase chain reaction using the QuickChange site-directed mutagenesis kit (Stratagene). Briefly, 35–40-base primers encompassing the positions of mutation were used for mutagenesis. The plasmid containing theBglII-EcoRV fragment of the β2AR in pSL1190 (Amersham Pharmacia Biotech) was used as a template. The sequences of the amplified regions were confirmed by the dideoxy chain termination method (Sanger et al., 1977). The fragments containing appropriate mutations were then ligated to construct a full-length β2AR and were finally inserted into XbaI or EcoRI andBamHI sites of mammalian expression vectors pEF-BOS (Mizushima and Nagata, 1990) or pCMV5, respectively. These constructs were transfected into COS-7 cells by the DEAE-dextran method (Cullen, 1987).
Membrane preparations and radioligand binding assays.
The cells were rinsed twice with ice-cold phosphate-buffered saline and mechanically detached in ice-cold buffer containing 10 mmTris·HCl, pH 7.4, 5 mm EDTA, 10 μg/ml benzamidine, 10 μg/ml soybean trypsin inhibitor (type II-S), and 5 μg/ml leupeptin (lysis buffer). The lysate was centrifuged at 45,000 ×g for 10 min at 4°. The pellet was rehomogenized in lysis buffer, with a Potter-type homogenizer, and stored at −80° until use. The competition binding assays were performed in buffer containing 75 mm Tris·HCl, pH 7.4, 12.5 mmMgCl2, and 2 mm EDTA, using 1–5 μg of membrane protein, 50 pm125I-CYP, and 0–100 μm unlabeled ligand in the presence of 100 μm GTP, for 60 min at 37°. The binding reaction was terminated by dilution and rapid filtration through Whatman GF/C filters; the filters were washed three times with solution containing 25 mm Tris·HCl, pH 7.4, and 1 mmMgCl2. Nonspecific binding was determined in the presence of 5 μm (±)-propranolol. The radioactivity on the filters was counted with a γ-counter. The protein concentration was determined by the method of Lowry et al. (1951). Because the expression levels of endogenous βARs in COS-7 cells are <30 fmol/mg of protein (data not shown), the binding activities measured in this study are largely attributable to those of the exogenously expressed chimeric and mutated βARs.
Data analysis.
All data are shown as mean ± standard error of the specified number of determinations. Equilibrium dissociation constants were determined from saturation isotherms. The competition curves were analyzed by nonlinear regression analysis, to determine EC50 andKi values, using PRISM software (GraphPAD Software Inc., San Diego, CA). Statistical significance was assessed by one-way analysis of variance for multiple comparisons. Analysis of variance post hoc comparisons were evaluated with the Dunnett test.
Molecular modeling of the salmeterol-β2AR complex.
The positions of the α-carbon of the β2AR were determined by overlaying the amino acids in the TMDs of the β2AR with those of bacteriorhodopsin, using Insight II molecular modeling software (MSI, San Diego, CA). The salmeterol-β2AR complex was then manually obtained by specifying the following interactions between residues of the β2AR and specific groups of salmeterol: Asp113 in TMD III with the amine group, two serines in TMD V with the saligenin moiety, and the inner half of TMD IV with the phenyl group of the side chain. Then constrains were released, and the reasonable model of the salmeterol-β2AR complex was obtained by Monte Carlo simulation.
Results
Affinities of salmeterol for β1/β2AR CHs.
Salmeterol showed very high selectivity for the WT β2AR (β1Ki /β2Ki ratio of approximately 1500) (Table 1). To determine the domain(s) responsible for β2-selectivity, we constructed several β1/β2AR CHs. Structures of various CHs are shown in Fig. 1. Although the affinity of salmeterol was slightly decreased by replacement of TMD I or II of the β2AR (CH-1 or CH-2) with that of the β1AR, the affinity of salmeterol was not affected by the introduction of TMD I or II of the β2AR into the β1AR (CH-5 or CH-6) (Table 1). This finding suggested that TMDs I and II of the β2AR are not primarily involved in the β2-selective binding of salmeterol. On the other hand, the CH (CH-3) that contained TMD VII of the β1AR demonstrated greatly decreased affinity for salmeterol. The contribution of TMD VII of the β2AR to the high affinity binding of salmeterol was confirmed by the finding that the affinity of salmeterol for the β1AR was increased by introduction of TMD VII of the β2AR into the β1AR. The replacement of TMD VII plus TMD II further increased the affinity of salmeterol, suggesting that TMD II indirectly contributes to the β2-selective binding of salmeterol by supporting a role of TMD VII. These results suggest that TMD VII of the β2AR is a major region for the subtype-selective binding of salmeterol.
Analysis of alanine-substituted mutants.
To identify the amino acid that is responsible for the high affinity binding of salmeterol, 10 amino acids in TMD VII of the β2AR that are different from those of the β1AR were individually changed to alanine. The positions of the mutated amino acids are indicated in Fig. 2. TheKd values of125I-CYP for the alanine-substituted β2ARs were not significantly different from that for the WT β2AR (Table2). Eight mutants showed no significant differences in binding affinities for salmeterol. The affinities for salmeterol were decreased in two mutants. The mutation of Tyr308 to alanine (Y308A-β2AR) significantly decreased the affinity for salmeterol (120-fold decrease). The change of Ile309 to alanine (I309A-β2AR) resulted in a receptor that showed 16-fold decreased affinity for salmeterol, although the decrease in the affinity for salmeterol was not significant. The decreases in affinities for Y308A- and I309A-β2ARs were smaller than that for the chimeric receptor (CH-3). The affinity for salmeterol was decreased further, but not additively, in the double mutant (Y308A/I309A-β2AR) (Table3). This finding indicates that two amino acids cooperatively contribute to the high affinity binding of salmeterol.
Effects of the position of the ether oxygen on β2-selectivity.
To examine the importance of the ether oxygen in the side chain of salmeterol for β2-selectivity, we synthesized three salmeterol derivatives; two derivatives had ether oxygens in different positions and one derivative did not have an ether oxygen. Fig.3 shows the structures of the three derivatives of salmeterol. It was reported that the duration of action of salmeterol is altered when the position of the ether oxygen is changed. Derivative 1 (in which the ether oxygen is positioned four carbons from the protonated amine) and derivative 2 (in which it is positioned eight carbons from the protonated amine) showed 33- and 64-fold decreased affinities for the WT β2AR, respectively (Table 3). The affinity of derivative 3 (in which the ether oxygen was removed from the side chain) for the WT β2AR was decreased 147-fold. The affinities of derivatives 1 and 3 for the WT β1AR were essentially the same as that of salmeterol. The affinities of derivative 3 for the Y308A-, I309A-, and Y308A/I309A-β2ARs were close to that for the WT β1AR. The rank order of potency for the WT β2AR was salmeterol > derivative 1 > derivative 2 > derivative 3; those for Y308A-, I309A-, and Y308A/I309A-β2ARs were the same as that for the WT β2AR. This indicates that the ether oxygen does not directly interact with Tyr308 and Ile309.
Molecular model of the salmeterol-β2AR complex.
To obtain structural information regarding the salmeterol-β2AR complex, we built a molecular model using Insight II software (Fig. 4). It showed that the phenyl group of Tyr308, which is important for the β2-selective, high affinity binding of salmeterol, seemed to interact with methylene groups in the side chain near the protonated amine of salmeterol, via hydrophobic interactions. Another feature of the model is a possible interaction of the ether oxygen with Tyr316 in TMD VII. The ether oxygen in the side chain could not directly interact with Tyr308 because of constraints on the structures of salmeterol and the β2AR. The model can explain the decrease in the affinities of the β2AR for salmeterol derivatives. Changes in the position of the ether oxygen would result in disruption of the interactions with Tyr316. This molecular model also suggested that Asp113 in TMD III, which interacts with the protonated amine of agonists, would become close to the ether oxygen and would compensate for the lost interaction of the ether oxygen with Tyr316.
Discussion
We constructed a series of β1/β2 chimeric receptors and alanine-substituted β2ARs, to examine the binding domain for the β2-selective agonist salmeterol. We previously reported that the binding domains of the chimeric receptors for the agonist isoproterenol were largely preserved after TMDs of the β1AR were exchanged with those of the β2AR, or vice versa (Kikkawaet al., 1998). The exchange of TMD I between the β2AR and the β1AR (CH-1 and CH-5) did not affect the binding characteristics of salmeterol. This suggests a small contribution of TMD I to the β2-selective binding of salmeterol.
The affinity of salmeterol was slightly decreased in CH-2. This finding suggests that TMD II contributes to the high affinity binding of salmeterol, compared with the contribution of TMD I. However, the introduction of TMD II of the β2AR did not increase the affinity for salmeterol, suggesting that TMD II does not contain the sites of direct contact with salmeterol. The affinity of salmeterol for the CH (CH-3) containing TMD VII of the β1AR was essentially the same as that for the β1AR. The introduction of TMD VII of the β2AR into the β1AR partially restored the high affinity binding of salmeterol, and the replacement of both TMD II and TMD VII of the β1AR with the corresponding regions of the β2AR further increased the affinity for salmeterol. It is important to produce not only loss-of-function mutants but also gain-of-function mutants, because the loss of binding activity may be the result of a nonspecific alteration of binding sites (Strader et al., 1995). These data suggest that TMD VII plays a major role in the high affinity binding of salmeterol and TMD II plays a supportive role in the β2-selective binding of salmeterol.
There have been several reports that specific amino acids in TMDs II and VII are close in space and have functional interactions [i.e., the interactions of Asn87 in TMD II of the gonadotropin-releasing hormone receptor with Asp318 in TMD VII (Zhou et al., 1994), Asp120 in TMD II of the 5-hydroxytryptamine type 2A receptor with Asn376 in TMD VII (Sealfon et al., 1995), and Asp71 in TMD II of the thyrotropin-releasing hormone receptor with Asp316 in TMD VII (Perlmanet al., 1997)]. It is possible that similar interactions between TMDs II and VII stabilize the structure of the β2AR and form a binding pocket for salmeterol.
Salmeterol is a β2-selective agonist with very long-lasting physiological actions (Johnson, 1995). The structural feature of salmeterol include a long side chain that has a phenyl group at the end, and the interaction of the phenyl group with the so-called exosite is assumed to govern the kinetics of salmeterol (Colemanet al., 1996). The exosite is an unique site that can participate in the persistent binding of salmeterol to the β2AR. Green et al. (1996) reported recently that the exosite is located within the inner part of TMD IV of the β2AR, because a chimeric β1/β2 receptor containing the inner part of TMD IV of the β1AR lost the long duration of action. Interestingly, the binding characteristics of salmeterol for the CH were same as those for the WT β2AR. Those authors indicated that the exosite in the inner part of TMD IV does not contribute to the subtype-selective binding, supporting our observation that the β2-selective high affinity binding site is mainly located within TMD VII of the β2AR.
The results with the chimeric receptors indicate that at least one of the amino acids in TMD VII is responsible for the high affinity binding of salmeterol. Analysis of the binding characteristics of alanine-substituted mutants revealed that Tyr308 contributes to the β2-selective binding of salmeterol. We recently reported that the β2-selective binding of TA-2005, a β2-selective agonist, was mainly determined by Tyr308 in TMD VII of the β2AR (Kikkawa et al., 1998). Considering the results with TA-2005, we concluded that Tyr308 is a critical amino acid conferring high affinity binding of β2-selective agonists to the β2AR. Because agonist binding domains are assumed to be located within TMDs, and the homologies of TMDs IV and VII (58–63%) between the β1- and β2ARs are lower than those of other TMDs (71–88%), TMD VII seems to be a good target for the design of β2-selective agonists. According to a model proposed by Schwartz and Rosenkilde (1996), consisting of a deep pocket formed by TMDs III, IV, V, and VI and a shallow pocket formed by TMDs II, III, and VII, Ser204 and Ser207 in TMD V, Phe293 in TMD IV, and Asp113 in TMD III seem to face the deep pocket; Tyr308 in TMD VII, which is important for β2-selectivity, faces the shallow pocket.
Rosenkilde et al. (1994) recently reported that point mutations in TMD II of the neurokinin-1 receptor induce a conformation of the receptor that impairs interconversion from an antagonist-bound form to an agonist-bound form. They showed that binding of agonist to the mutated receptor cannot shift the equilibrium of the receptor conformation toward the agonist-bound form when antagonists are already bound to the receptor. It is possible that mutation of Tyr308 of the β2AR induced and fixed the conformation that showed high affinity for 125I-CYP and low affinity for salmeterol. However, this possibility is unlikely, because the binding of isoproterenol was not affected by the mutation of Tyr308 to alanine (Kikkawa et al., 1998). This indicates that the decrease in the affinity of Y308A-β2AR actually reflects a specific alteration of the binding site that is important for the high affinity binding of salmeterol.
Frielle et al. (1988) reported, using chimeric β1/β2ARs, that the majority of the βAR-selective binding of betaxolol and ICI118551 is determined by TMD IV, although multiple domains seem to be involved in the determination of the βAR-selective binding of these two antagonists. The contribution of TMD IV to subtype-selective antagonist binding was supported by the fact that TMD IV shows the greatest difference in primary amino acid sequences between the β1- and β2ARs (58% identity). It would be interesting to determine whether TMD IV of the β2AR plays a role in the high affinity binding of salmeterol.
The affinities of the two derivatives of salmeterol with the ether oxygen at different positions were decreased 30–60-fold, and the affinity of the derivative of salmeterol with no ether oxygen was decreased approximately 150-fold. However, these derivatives still showed higher affinities for the β2AR than for the β1AR. Therefore, the position of the ether oxygen in the side chain is important for the β2-selective high affinity binding of salmeterol, although it is not the sole determinant for β2-selective binding. Johnson (1995) reported that 1) compounds in which ether oxygens are placed two or eight carbons from the protonated amine show reduced durations of action of <30 min, compared with >12 hr for salmeterol (in which the ether oxygen is located six carbons from the amine), 2) the saligenin head of salmeterol produces high β2-selectivity, and 3) the kinetics at the receptor are governed by the side chain. It is apparent that the side chain containing the ether oxygen of salmeterol adopts a turn to interact with the amino acids in TMDs III, IV, and V. The results with alanine-substituted mutants suggested that candidate amino acids to interact with the ether oxygen were Tyr308 and Ile309 in TMD VII. However, the molecular modeling did not support this idea. Tyr308 could not directly interact with the ether oxygen of salmeterol because of the constraints on the flexible movement of the side chain, considering the well-established interaction sites. The present model predicted that the ether oxygen would interact with Tyr316 in TMD VII, instead of Tyr308. The model also suggested that Asp113 in TMD III interacted with the ether oxygen when more favorable interactions with Tyr316 were disrupted. It is necessary to perform more mutagenesis experiments to establish a model of the salmeterol-β2AR complex, especially focusing on the long-lasting action of salmeterol. In conclusion, we demonstrated that Tyr308 in TMD VII is the key amino acid for the β2-selective binding of salmeterol and that the position of the ether oxygen in the side chain plays an important role in the β2-selectivity of salmeterol.
Acknowledgments
We are grateful to Dr. H. Inoue (Tanabe Seiyaku, Saitama, Japan) for kindly synthesizing salmeterol derivatives for us. We also thank Dr. R. J. Lefkowitz for the pBC-β1 and -β2 plasmids and Dr. S. Nagata for the pEF-BOS plasmid.
Footnotes
-
Send reprint requests to: Dr. Hitoshi Kurose, Laboratory of Pharmacology and Toxicology, Graduate School of Pharmaceutical Sciences, University of Tokyo, 7–3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan. E-mail: kurose{at}mol.f.u-tokyo.ac.jp
-
↵1 Current affiliation: Toray Industries, Inc., Basic Research Laboratories, Kamakura, Kanagawa 248-8555, Japan.
-
This work was supported in part by grants from the Ministry of Education, Science, Sports, and Culture of Japan (T.N.) and the Mochida Memorial Foundation for Medical and Pharmaceutical Research (H.K.).
- Abbreviations:
- βAR
- β-adrenergic receptor
- TMD
- transmembrane domain
- CYP
- cyanopindolol
- CH
- chimera
- WT
- wild-type
- Received April 27, 1998.
- Accepted June 23, 1998.
- The American Society for Pharmacology and Experimental Therapeutics