Relevance of Aromatic Residues in Transmembrane Segments V to VII for Binding of Peptide and Nonpeptide Antagonists to the Human Tachykinin NK2 Receptor

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Vol. 290, Issue 2, 487-495, August 1999

Relevance of Aromatic Residues in Transmembrane Segments V to VII for Binding of Peptide and Nonpeptide Antagonists to the Human Tachykinin NK₂ Receptor

A. R. Renzetti, R.-M. Catalioto, M. Criscuoli, P. Cucchi, C. Ferrer, A. Giolitti, M. Guelfi, L. Rotondaro, F. J. Warner and C. A. Maggi

Departments of Pharmacology (A.R.R., R-M.C., M.C., P.C., M.G., C.A.M.), Drug Design (A.G.), and Biotechnology (C.F., L.R.), Menarini Ricerche S.p.A., Firenze, Italy; and School of Physiology and Pharmacology (F.J.W.), University of New South Wales, Sydney, Australia

	Abstract

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We used membranes from Chinese hamster ovary cells stably transfected with the human tachykinin NK₂ receptor, either wild-typeor mutated, at four aromatic residues (His¹⁹⁸, Tyr²⁶⁶, Phe²⁷⁰, Tyr²⁸⁹) located in transmembrane segments V to VII, to assess the roleof these residues in the binding of natural tachykinins and peptideand nonpeptide antagonists. Three radioligands, the agonist [¹²⁵I]neurokinin A (NKA), the peptide antagonist [³H]MEN 11420, and the nonpeptide antagonist [³H]SR 48968 bound to the wild-type receptor with high affinity(K_d = 2.4 nM, 0.3 nM, and 4.0 nM, respectively). Four of the sixmutant receptors tested retained high affinity for at least oneof the radioligands. H¹⁹⁸A mutation abrogated the binding of NKA but not that of MEN 11420or SR 48968 (K_d = 4.8 and 11.5 nM, respectively); Y²⁶⁶F mutation abrogated the binding of MEN 11420 but not that ofNKA or SR 48968 (K_d = 2.8 nM and 1.2 nM, respectively); F²⁷⁰A mutation abrogated the binding of both NKA and MEN 11420 butnot that of SR 48968 (K_d = 1.6 nM); Y²⁸⁹F mutation abrogated the binding of SR 48968 but not that of NKAand MEN 11420 (K_d = 2.0 and 2.9 nM, respectively). Y²⁶⁶A and Y²⁸⁹A mutations abrogated the binding of all radioligands. Among theunlabeled antagonists, the affinity of the nonpeptide GR 159897,at variance with SR 48968, resulted heavily compromised by H¹⁹⁸A and Y²⁶⁶F mutations; the peptide antagonists R396 and MEN 10376 essentiallyfollowed the binding profile of NKA, but R396 showed markedlyincreased affinity for the Y²⁸⁹F mutant receptor. Taken together, these results indicate thatdifferent, partially overlapping sets of sites may be involvedin the binding of agonists and diverse antagonists to the humantachykinin NK₂receptor.

	Introduction

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The mammalian tachykinins substance P (SP), neurokinin A (NKA), and neurokinin B (NKB) form a family of peptides that sharethe common C-terminal sequence Phe-X-Gly-Leu-MetNH₂. Tachykininsare found in many regions of the central and peripheral nervoussystem (Maggio, 1988; Maggi et al., 1993; Otsuka and Yoshioka,1993) and produce their biological effects by stimulating threedistinct G protein-coupled receptors termed tachykinin NK₁, NK₂,and NK₃ receptors (Maggi, 1995, forreview).

The tachykinin NK₁ receptor has been the object of intense investigations to assess the structural determinants of its interactionwith ligands of both peptide and nonpeptide nature, agonists andantagonists, respectively (Schwartz et al., 1995, for review).The site-directed mutagenesis approach has been extensively usedto identify residues putatively involved in the binding of agonistsand antagonists to the tachykinin NK₁ receptor. From these studies,it has been proposed that residues forming the binding site ofnatural agonists on the tachykinin NK₁ receptor are quite distinctfrom those that form the binding site of antagonists, especiallythose of antagonists of nonpeptide nature (Fong et al., 1992;Gether et al., 1993a; Huang et al., 1994).

Less information is available on the structural determinants of agonist and antagonist binding at the tachykinin NK₂ receptor.Studies using chimeric tachykinin NK₁/NK₂ receptors have shownthat the binding site of the nonpeptide tachykinin NK₂ receptorantagonist SR 48968 is not fully coincident with that of NKA,the natural tachykinin with preferential binding affinity fortachykinin NK₂ receptors (Gether et al., 1993b). A few site-directedmutagenesis studies have also been performed on the human tachykininNK₂ receptor (hNK₂R; Bhogal et al., 1994; Huang et al., 1995).The results of these studies have identified some aromatic residuesin transmembrane segments (TM) V to VII of the hNK₂R as beinginvolved in the binding of NKA and other natural tachykinins,as well as in the binding of the nonpeptide tachykinin NK₂ receptorantagonists SR 48968 (Emonds-Alt et al., 1992) and GR 159897 (Beresfordet al., 1995; Fig. 1). In particular, Tyr²⁸⁹ (TM VII), along with Tyr²⁶⁶ and Phe²⁷⁰ (TM VI), were proposed to form part of the SR 48968 binding pocket(Huang et al., 1995). Discrepant results were reported with regardto the role played by His¹⁹⁸ (TM V) in determining the binding affinity of SR 48968. Bhogalet al. (1994) and Huang et al. (1995) reported a dramatic fallin the binding affinity of NKA at the H¹⁹⁸A mutant tachykinin NK₂ receptor. However, although Bhogal etal. (1994) reported that this residue is crucial for preservingthe binding affinity of SR 48968, Huang et al. (1995) failed todetect any significant change of the affinity with the H¹⁹⁸A mutation, although they reported reduced binding affinity foranother nonpeptide antagonist, GR 159897. The reasons for thisdiscrepancy have not been found.

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Fig. 1. Chemical structures of the tachykinin NK₂ receptor antagonists MEN 11420, SR 48968, and GR 159897.

In this study, we used Chinese hamster ovary (CHO) cell lines stably transfected with the wild-type and mutant tachykininNK₂ receptors to more precisely assess the role played by aromaticresidues in TM V (His¹⁹⁸), TM VI (Tyr²⁶⁶ and Phe²⁷⁰), and TM VII (Tyr²⁸⁹; Fig. 2) in the binding of natural agonists and peptide (includingboth linear and cyclic structures) and nonpeptide antagonists.We performed saturation and competition binding experiments withCHO cell membranes by using [¹²⁵I]NKA, [³H]SR 48968, and [³H]MEN 11420, a new tachykinin NK₂ receptor-selective ligand (Cataliotoet al., 1998, Renzetti et al., 1998; Fig. 1) as radioligands.In particular, we aimed at verifying the hypothesis of the highlyvariable, flexible mode of interaction of the receptor with thedifferent classes of ligands that could be inferred from the previouswork of Bhogal et al. (1994) and Huang et al. (1995).

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Fig. 2. Schematic of the tachykinin NK₂ receptor showing the putative localization of the residues subjected to mutation.

	Materials and Methods

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Chemicals

Penicillin, streptomycin, and trypsin were purchased from GIBCO (Grand Island, NY). Dialyzed fetal calf serum (FCS) was obtainedfrom BioWhittaker (Walkersville, MD). Minimum essential Eagle'smedium $alpha$ -modification ( $alpha$ -MEM) and GTP were purchased from SigmaChemical Co. (St. Louis, MO). Flasks and Petri dishes were purchasedfrom Falcon (Becton Dickinson, Milan, Italy). Protein bindingdye was from Bio-Rad (Richmond, CA). NKA, NKB, and SP were obtainedfrom Neosystem Laboratoire (Strasbourg, France). SR 48968 [(S)-N-methyl-N[4-(4-acetyl-amino-4-phenylpiperidino)-2-(3,4-dichlorophenyl)butyl]benzamide]was kindly provided by Drs. X. Emonds-Alt and G. Le Fur (SanofiRecherche, Montpellier, France). MEN 11420 (c{[( $beta$ -D-GlcNAc)Asn-Asp-Trp-Phe-Dpr-Leu]c(2 $beta$ -5 $beta$ )}),MEN 10376 ([Tyr⁵,D-Trp^6,8,9,Arg¹⁰]NKA (4-10), and GR 159897 [(R)-1-[2-(5-fluoro-1H-indol-3-yl)ethyl]-4-methoxy-4[(phenylsulfinyl)-methyl]piperidine]were synthesized at the Chemistry Department of Menarini Ricerche(Firenze, Italy). R396 (Ac-Leu-Asp-Gln-Trp-Phe-Gly-NH₂) was agift from Prof. D.Regoli.

[³H]MEN 11420 (specific activity, 62 Ci/mmol) was synthesized by SibTech Inc. (Elmsford, NY). [¹²⁵I]NKA (specific activity, 2000 Ci/mmol) was purchased from AmershamInternational (Buckinghamshire, UK). [³H]SR 48968 (specific activity, 25.7 Ci/mmol) was purchased fromDupont-NEN Life Sciences (Boston, MA). All other reagents, availablefrom commercial sources, were of analyticalgrade.

Site-Directed Mutagenesis of hNK₂R cDNA. Plasmid pBS/hNK₂R (kindly provided by Dr. J. E. Krause, Washington University, St. Louis, MO) contained a 1.2-kb cDNA forthe ileum hNK₂R cloned in the SmaI site of the pBlueScript IISK( $-$ ) phagemid. Site-directed mutagenesis of the tachykinin NK₂receptor cDNA was performed according to the phosphorothioatetechnique of Eckstein (Taylor et al., 1985; Nakamaye and Eckstein,1986) using single-stranded DNA of the tachykinin NK₂ receptorcDNA in pBlueScript II SK( $-$ ) and an in vitro mutagenesis kit (Sculptor;Amersham International) according to the manufacturer's instructions.Wild-type cDNA was isolated from HindIII/XbaI-digested pBS/hNK₂Rand cloned in pmCMV $beta$ SV1dhfr, partially digested with HindIII,between the HindIII and XbaI sites of the polylinker region, underthe transcriptional control of the murine cytomegalovirus majorimmediate-early promoter. The resulting vector was designatedas pmCMV $beta$ SV1dhfr-hNK₂R. Expression vectors carrying the mutatedcDNAs (H¹⁹⁸A, Y²⁶⁶A, Y²⁶⁶F, F²⁷⁰A, Y²⁸⁹A, Y²⁸⁹F) were constructed by exchanging the 1.2-kb EcoRV/Xbal wild-tachykininNK₂ receptor cDNA in pmCMV $beta$ SV1dhfr-hNK₂R with the EcoRV/Xbal mutatedcDNAs excised from pBS/hNK₂R. pmCMV $beta$ SV1 was constructed by removingG-CSF cDNA sequences from XbaI-digested pmCMV $beta$ G-CSFSV1dhfr (Rotondaroet al., 1997). The structure of all constructs was confirmed byrestriction analysis. The complete coding sequence of wild-typeand mutated tachykinin NK₂ receptor cDNAs cloned into the pmCMV $beta$ SV1dhfrexpression vector was confirmed by DNAsequencing.

Receptor Expression in CHO Cells. Large-scale preparation of vector DNA for transfection experiments was carried out using a Qiagen maxipreparation column (Qiagen,Hilden, Germany). Wild-type and (H¹⁹⁸A, Y²⁶⁶A, Y²⁶⁶F, F²⁷⁰A, Y²⁸⁹A, or Y²⁸⁹F) mutated tachykinin NK₂ receptor cDNAs in pmCMV $beta$ SV1dhfr wereintroduced by lipofection as described previously (Rotondaro etal., 1997) into dihydrofolate reductase (DHFR)-deficient CHO DUKX-B11cells (Urlaub and Chasin, 1980; referred to as CHOdhfr $-$ ). StableDHFR+ transformants were selected in nucleoside-free $alpha$ -MEM containing5% dialyzed FCS; 12 to 14 days after transfection, more than 100individual DHFR+ clones were pooled, grown to mass culture, andused for ligand-binding studies. CHOdhfr $-$ cells and stable CHOtransfectants were grown in $alpha$ -MEM containing ribonucleosides anddeoxyribonucleosides and supplemented with 5% FCS, in a humidifiedatmosphere of 5% CO₂/95% air at 37°C until slightlyconfluent.

Binding Assays. Confluent cells were harvested in PBS, pelleted by centrifugation at 200g (4°C), and homogenized using a Polytron PT3000 (Kinematica,Lucerne, CH) at 13,000 rpm for 15 s in 20 ml of 50 mM Tris, pH7.4, containing bacitracin (100 µg/ml), chymostatin (10 µg/ml),leupeptin (5 µg/ml), and 10 µM thiorphan (buffer A). The homogenatewas centrifuged for 1 h at 25,000g (4°C), and the pellet was resuspendedin the binding buffer (pH 7.4) composed of buffer A supplementedwith 150 mM NaCl, 5 mM MnCl₂, and 0.1% BSA at a protein concentrationof about 0.6 mg/ml. The membranes (50-90 µg protein/assay) wereincubated for 30 min ([¹²⁵I]NKA and [³H]SR 48968) or 60 min ([³H]MEN 11420) at 20°C. In saturation experiments, either increasingconcentrations (0.09-15.0 nM) of [³H]SR 48968 or [³H]MEN 11420 (hot experiments) or a fixed concentration (150 pM)of [¹²⁵I]NKA with various concentrations of unlabeled NKA (0.01 nM to1 µM; cold experiment) was used. For competition experiments,0.4 to 1.0 nM [³H]MEN 11420, 0.6 nM [³H]SR 48968, or 150 pM [¹²⁵I]NKA was used, with or without varying concentrations (0.001nM to 10 µM) of the competing compounds in a final volume of 0.5ml. Then, 1 µM unlabeled MEN 11420, SR 48968, or NKA was usedto define nonspecific binding, depending on the radioligand. Thereaction was terminated by the addition of 4 ml of ice-cold Tris(50 mM, pH 7.4) followed by rapid filtration through Whatman GF/Bfilter sheets (presoaked in 0.3% polyethylenimine for [³H]MEN 11420 or 0.5% BSA for [³H]SR 48968 and [¹²⁵I]NKA, for at least 3 h using a Brandel (Montreal, Quebec, Canada)cell harvester. Filters were washed three times with 4 ml of ice-cold50 mM Tris buffer, pH 7.4. The trapped radioactivity was determinedby liquid scintillation using a $beta$ -scintillation counter (2200CA; Packard, Milan, Italy) or using a gamma counter (Cobra,Packard).

Analysis of Binding Data

Saturation and competition data were processed according to Munson and Rodbard (1980) by the step-wise application of EBDAand LIGAND programs in the KELL software for Macintosh (Biosoft,Cambridge, UK). The maximal binding (B_max), equilibrium dissociationconstant (K_d), and equilibrium inhibition constant (K_i) valueswere calculated. They are reported as mean values with approximateS.E.s as estimated by LIGAND. The goodness of fit, according tothe single- or multiple-site binding models, was evaluated bythe Fratio.

Statistical comparisons were made by using one-way ANOVA followed by Tukey's test whereappropriate.

	Results

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Saturation Experiments

The specific binding of [¹²⁵I]NKA, [³H]SR 48968, and [³H]MEN 11420 was directly proportional to the membrane concentration (datanot shown). At protein concentrations between 50 and 90 µg/assay,as used in competition experiments, the specific binding representedapproximately 80 to 90% of the total binding for each radioligand,respectively. Scatchard transformation of the saturation experimentsdata showed a monophasic interaction with the wild-type NK₂ receptorwith K_d values of 2.4 ± 0.43, 0.3 ± 0.08, and 4.0 ± 0.44 nM andB_max values of 206 ± 28, 3274 ± 1489, and 1664 ± 416 fmol/mg proteinfor [¹²⁵I]NKA, [³H]SR 48968, and [³H]MEN 11420, respectively (n = 5-6; Table 1).

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TABLE 1
Saturation analysis-derived binding constants of the three diverse radioligands for wild-type and mutant human tachykinin NK₂ receptors expressed in CHO cells
K_d (nM) and B_max (fmol/mg protein) values are expressed as mean ± S.E.M. of the number of independent determinations indicated in parentheses.

Y²⁶⁶A and Y²⁸⁹A mutant receptors did not bind any of the radioligands (Table 1). For the other mutant receptors, the specific bindingof [¹²⁵I]NKA, [³H]SR 48968, and [³H]MEN 11420 was directly proportional to the membrane concentration(data not shown). Saturation experiments always produced datacongruent with monophasic ligand-receptor interaction. NeitherK_d nor B_max values for [¹²⁵I]NKA changed with the mutant receptors, which maintained theability to interact with the agonist ligand (Table 1). The B_maxvalues for [³H]SR 48968 and [³H]MEN 11420, considerably higher than that measured for [¹²⁵I]NKA, were not statistically different from each other. They,too, despite an apparent variability, did not change in a significantmanner throughout the responsive receptors; the only exceptionwas the H¹⁹⁸A mutant, which showed both lower expression and reduced affinityfor the antagonist ligands (Table 1).

Competition Experiments

Wild-Type. Among the tachykinins, only NKA competed with high affinity for the binding of the three radioligands to the wild-type hNK₂R.When using either [³H]SR 48968 or [³H]MEN 11420 as tracers, the competition of unlabeled NKA was biphasic,probably reflecting its binding to the high-affinity (i.e., Gprotein-coupled) and low-affinity (i.e., G protein-uncoupled)states of the tachykinin NK₂ receptor (Fig. 3). The rank orderof affinity of the receptor antagonists, which was independentfrom the radioligand used to label tachykinin NK₂ receptors, wasas follows: SR 48968 > GR 159897 > MEN 11420 > MEN 10376 $>>$ R396(Table 2). The curves describing the displacement of [³H]SR 48968 and [³H]MEN 11420 by the prototype antagonists SR 48968, GR 159897,and MEN 11420 are shown in Figs. 4A and 5A.

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Fig. 3. Homologous and heterologous displacements of [¹²⁵I]NKA ( $black-triangle$ ), [³H]SR 48968 ( $black-square$ ), and [³H]MEN 11420 (

) by unlabeled NKA in membrane preparations of CHO cells transfected with wild-type nNK₂R. Data shown represent the mean of at least three separate determinations in duplicate. Curves were fitted by the simultaneous analysis of all data sets to a one-site (for [¹²⁵I]NKA) or two-site (for [³H]SR 48968 and [³H]MEN 11420) binding model by GraphPAD Prism.

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TABLE 2
Binding affinity of tachykinins and selective antagonists for wild-type and mutant human tachykinin NK₂ receptors expressed in CHO cells
K_i values (from heterologous competition studies) or K_d values (from saturation studies) obtained with all the radioligands recognized by each receptor are reported. Data are expressed as mean ± approximate S.E.M. as calculated by simultaneous analysis of four to ten independent experiments by using LIGAND software.

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Fig. 4. Displacement curves of [³H]SR 48968 binding to CHO cell membranes transfected with wild-type (A), H¹⁹⁸A (B), Y²⁶⁶F (C), and F²⁷⁰A (D) hNK₂R by GR 159897 ( $black-square$ ), MEN 11420 ( $black-triangle$ ), and SR 48968 (

). Data shown represent the mean of at least three separate determinations in duplicate. Curves were fitted by the simultaneous analysis of all data sets to a one-site binding model by GraphPAD Prism.

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Fig. 5. Displacement curves of [³H]MEN 11420 binding to CHO cell membranes transfected with wild-type (A) and Y²⁸⁹F (B) hNK₂R by GR 159897 ( $black-square$ ), MEN 11420 ( $black-triangle$ ), and SR 48968 (

H¹⁹⁸A. This mutation completely abrogated the binding of [¹²⁵I]NKA to the hNK₂R and reduced by about 16-fold the binding affinity of[³H]SR 48968, whereas binding affinity of [³H]MEN 11420 was reduced by about 3-fold (Table 1). Because asizable binding affinity was measured with [³H]SR 48968 and [³H]MEN 11420, these tracers were used in competition experimentswith natural tachykinins and antagonists of both peptide and nonpeptidenature (Table 2, Fig. 4B).

The affinity of NKA for the H¹⁹⁸A tachykinin NK₂ receptor was then estimated to be decreased by about 143- and 159-fold using[³H]SR 48968 and [³H]MEN 11420 as tracers, respectively (Table 2), whereas no bindingaffinity could be estimated for NKB or SP (Table 2). Confirmingthe results of Huang et al. (1995)

, the binding affinity of GR159897was also markedly decreased as measured by displacing either [³H]SR 48968 or [³H]MEN 11420 (66- and 25-fold, respectively; Table 2). No sizablebinding affinity was measured for the two linear peptide antagonists,MEN 10376 and R396, with either tracer (Table 2).

Y²⁶⁶F. This mutation did not affect the binding of [¹²⁵I]NKA, slightly affected (4-fold decrease) the binding of [³H]SR 48968, and abrogated the binding of [³H]MEN 11420 to the hNK₂R (Table 1). The binding affinity of unlabeledMEN 11420 at the mutant receptor was decreased by about 12-foldwhen using either [¹²⁵I]NKA or [³H]SR 48968 as tracers (Table 2, Fig. 4C). The binding affinityof NKB, MEN 10376, and R396 was not substantially altered by theY²⁶⁶F mutation (Table 2), whereas the binding affinity of GR 159897was markedly decreased, by about 185- and 149-fold when using[¹²⁵I]NKA or [³H]SR 48968 as tracers, respectively (Table 2, Fig. 4C).

F²⁷⁰A. This mutation completely abrogated the binding of [¹²⁵I]NKA and [³H]MEN 11420 with only a minor effect on the binding of [³H]SR 48968 (Table 1). When using [³H]SR 48968 as a tracer, a 66-fold decrease in the binding affinityof MEN 11420 was estimated (Table 2, Fig. 4D), whereas no competitionwas exerted by NKA up to 10 µM (Table 2). Likewise, no bindingaffinity of NKB and SP could be estimated using [³H]SR 48968 as a tracer. The binding affinity of GR 159897 was,if any, slightly increased (5-fold) by the F²⁷⁰A mutation (Table 2, Fig. 4D), whereas the binding affinity ofthe linear peptide antagonists was decreased (MEN 10376; 17-fold)or abolished (R396; Table 2).

Y²⁸⁹F. This mutation completely abrogated the binding of [³H]SR 48968 without affecting the binding of [¹²⁵I]NKA and [³H]MEN 11420 (Table 1). In competition experiments, a 2741- and3088-fold decrease in binding affinity of SR 48968 was estimatedwhen using [¹²⁵I]NKA and [³H]MEN 11420 as tracers, respectively (Table 2, Fig. 5B). Thebinding affinity of NKB and SP was unaffected by the Y²⁸⁹F mutation (Table 2). The binding affinity of GR 159897 was totallyabrogated (Table 2, Fig. 5B), whereas that of MEN 10376 was unaffectedwhen using either [¹²⁵I]NKA or [³H]MEN 11420 as tracers (Table 2). Interestingly, the bindingaffinity of the linear antagonist R396 was consistently increased,by about 18-fold, by the Y²⁸⁹F mutation, when using either radioligand (Table 2).

	Discussion

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In the attempt to overcome problems that may be related to transient transfection and variable levels of expression of thereceptor, we prepared cell lines stably transfected with wild-typeand mutant hNK₂Rs. This approach enabled us to produce a systematicpharmacological analysis of the mutant receptors by using threedifferent radioligands and a panel of agonists andantagonists.

The even B_max values found with the agonist [¹²⁵I]NKA generally represent only a fraction of the receptor density estimated withthe antagonist radioligands, which are not able to discriminatebetween G protein-coupled and -uncoupled states of the NK₂ receptor.This is likely due to the fact that transfected receptors areexpressed in excess relative to the G protein-coupling capabilityof the CHO. In the case of the H¹⁹⁸A mutant, a significant reduction in the B_max value accompaniedthe decrease in affinity for the recognizedantagonists.

It is interesting to note that three of the four aromatic residues mutated in this study (His¹⁹⁸, Phe²⁷⁰, and Tyr²⁸⁹ in the sequence of the hNK₂R) are fully conserved at equivalentpositions in the sequence of the various mammalian tachykininreceptors cloned so far; the fourth residue (Tyr²⁶⁶ in the sequence of the hNK₂R) is conserved in the mammalian tachykininNK₂ and NK₃ receptors and is replaced by Phe at the equivalentposition of the mammalian tachykinin NK₁ receptor. Due to theirlipophilic nature, these conserved residues are likely to playa structural role in the correct positioning of the TMs. Fromthe present data, we have evidence that each one of the H¹⁹⁸A, Y²⁶⁶F, F²⁷⁰A, and Y²⁸⁹F mutant receptors maintained high-affinity binding for at leastone of the three radioligands used. This can be considered asa kind of positive control (i.e., it allows us to exclude thepossibility that these mutations produced a marked alterationin the gross structure of the receptor or that the mutant receptorprotein was synthesized but not expressed at the cell membranelevel). Therefore, the observed changes in the affinity of a givenligand for each of these mutant receptors can be confidently assumedas indications that the corresponding residues represent a truepoint of drug-receptor interaction or, alternatively, that themutation has modified the geometry of the ligand-binding pocket,thus indirectly influencing the affinity of theligand.

With regard to the binding of natural tachykinins, our data demonstrate that both His¹⁹⁸ and Phe²⁷⁰ are crucial for maintaining the high-affinity binding of NKA(see Huang et al., 1995) and that these residues are also of relevancefor the binding of NKB and SP to the wild-type tachykinin NK₂receptor.

His¹⁹⁸, putatively located on TM V of the hNK₂R, corresponds to His¹⁹⁷ in the sequence of the hNK₁R. In the latter, the Phe $right-arrow$ Ala replacementabolished the binding of several nonpeptide receptor antagonistswithout affecting the binding of SP (Fong et al., 1993). On theother hand, SP displayed a weak but sizable binding to the wild-typetachykinin NK₂ receptor (K_i = 1.8 µM against [¹²⁵I]NKA), which was lost in the H¹⁹⁸A mutant (K_i > 10 µM). This observation, along with the data ofFong et al. (1993), implies that the mode of interaction of SPwith the tachykinin NK₁ and NK₂ receptors are different (i.e.,the same tachykinin interacts with different regions of the tachykininNK₁ and NK₂receptors).

Our data also indicate that the ---OH function of Tyr²⁶⁶ and Tyr²⁸⁹ is not involved in determining the binding affinity of naturaltachykinins to the hNK₂R. On the other hand, the actual role ofthe aromatic function of these two Tyr residues in the bindingof tachykinins could not be definitely assessed; indeed, Ala replacementof Tyr²⁶⁶ and Tyr²⁸⁹ completely abolished the binding affinity for each of the threeradioligands tested. Unfortunately, this also means that no positivecontrol (as defined above) was any more available, which hamperedany speculation on the relevance of thesedata.

Our findings provide a clear demonstration that the binding of peptide antagonists to the hNK₂R is partially overlapping butnot coincident to that of nonpeptide antagonists SR 48968 andGR 159897. Moreover, differences in binding behavior also emergedbetween linear and cyclic peptide antagonists. In general, theobserved changes in the binding affinity of linear peptide antagonistsMEN 10376 (Maggi et al., 1991) and R396 (Dion et al., 1990) forthe mutant tachykinin NK₂ receptors follow quite closely thoseobserved for NKA and agonists. In fact, Ala substitution of His¹⁹⁸ and Phe²⁷⁰ almost completely abrogated the binding of MEN 10376 and R396,whereas the Tyr $right-arrow$ Phe replacement at position 266 was irrelevantfor both antagonists and, for MEN 10376, the Tyr $right-arrow$ Phe replacementat position 289 had no effect on binding affinity. Our data forMEN 11420, a glycosylated bicyclic peptide (Catalioto et al.,1998), indicate that in common with NKA, Phe²⁷⁰ is relevant for determining the high-affinity binding of thisantagonist to the hNK₂R. On the other hand, although His¹⁹⁸ is clearly relevant for the binding of NKA, MEN 10376, and R396,this residue is apparently less important for the binding of MEN11420.

Huang et al. (1995) described some pharmacological properties of Tyr²⁶⁶ mutants of the hNK₂R. They reported that although the Y²⁶⁶F mutant maintains a full binding affinity for both NKA and SR48968, the binding affinity was largely lost when Tyr²⁶⁶ was mutated to Ser or Ala (findings confirmed by the presentresults). Because a functional response (phosphoinositol formation)to NKA was preserved in the Y²⁶⁶S mutant, the derived affinity estimates for NKA and SR 48968could be computed and found to be obviously low (0.3 and 3.4 µM,respectively; Huang et al., 1995). From this, they concluded thatthe aromatic group of Tyr²⁶⁶ is involved, directly or indirectly, in the binding of NKA andSR 48968 to the hNK₂R. In this study, we observed that it is sufficientto remove the ---OH function of Tyr²⁶⁶ to abrogate the high-affinity binding of [³H]MEN 11420 to the hNK₂R. This indicates that the binding siteof MEN 11420 on the hNK₂R is partly different from that of bothNKA and SR 48968. The drop in affinity of MEN 11420, as estimatedfrom competition experiments against [¹²⁵I]NKA or [³H]SR 48968, is relatively small (about 10-fold) but consistentand evidently sufficient to prevent the detection of a specificbinding at the low concentrations of the radioligand used in saturationexperiments. This same mutation did not affect the binding affinityof the linear peptides MEN 10376 and R396, nor that of SR 48968,but decreased the binding affinity of GR 159897. This may suggestthat the ---OH function of Tyr²⁶⁶ directly interacts with some moiety present in both MEN 11420and GR 159897 but not in SR 48968. An hydrogen-bond donor/acceptorinterplay between the ---OH function of Tyr²⁶⁶ and the indole amino group present in both MEN 11420 and GR 159897could be postulated (Fig. 6).

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Fig. 6. Molecular models of the binding of the tachykinin NK₂ receptor antagonists MEN 11420 (top) and SR 48968 (bottom) to the tachykinin NK₂ receptor. Presented view is from outside the cell membrane, along the $alpha$ -helix axis. TM I and TM II have been omitted for clarity.

With regard to the binding of SR 48968 at the H¹⁹⁸A mutant receptor, we found a sizable but limited decrease in affinity (about16-fold): in this respect, our data differ from those of Huanget al. (1995), who reported that the binding of SR 48968 is unaffectedby the H¹⁹⁸A mutation, and from those of Bhogal et al. (1994), who reportedthat binding of SR 48968 is abrogated by the H¹⁹⁸A mutation. Because both previous studies were performed on transientlytransfected cell lines, it is possible that variable levels ofreceptor expression had influenced the results. With regard tothe other residues, our data confirm the observation (Huang etal., 1995) that the removal of the ---OH function of Tyr²⁸⁹ almost totally eliminated the binding affinity of SR 48968. Onthe other hand, the F²⁷⁰A mutation, which impaired the binding of most other ligands tested(with the exception of GR 159897), also had little effect on thebinding of SR 48968 to the hNK₂R. The equivalent residue (Phe²⁶⁸) in the sequence of the hNK₁R has been recently proposed to bepartially involved, directly or indirectly, in the binding ofboth SP and various nonpeptide antagonists to the tachykinin NK₁receptor, with the exception of SR 140333 (Holst et al., 1998).

On the whole, the two nonpeptide antagonists appear to have quite different sensitivities to residue mutation: the bindingaffinity of GR 159897 was heavily compromised by mutations atsites (His¹⁹⁸ and Tyr²⁶⁶), which have a weaker effect on the binding of SR 48968. Thisstrongly suggests that similar to the tachykinin NK₁ receptor(Holst et al., 1998), nonpeptide ligands of different chemicalclasses possess different modes of interaction with the tachykininNK₂receptor.

An interesting further observation is that relative to the ligand-dependent variation of the affinity of GR 159897 for theH¹⁹⁸A mutant receptor, the affinity of GR 159897 was about 4-foldhigher if measured in competition with [³H]MEN 11420 than with [³H]SR 48968 (K_i = 58 and 214 nM, respectively). A similar (5-fold)difference was observed when SR 48968 was tested in homologous(saturation) or heterologous (competition versus [³H]MEN 11420) binding assays (K_d = 5.2 nM, K_i = 1.0 nM, respectively).These observations suggest that [³H]MEN 11420 and [³H]SR 48968 may label different conformers of the tachykinin NK₂receptor, both unable to signal second messenger activation, andthat the His¹⁹⁸ residue is relatively less important in the binding energy balancefor the ligand-receptor complex formed by [³H]MEN 11420 with the selected receptorconformer.

In conclusion, the present findings provide a detailed pharmacological analysis of the role of some aromatic residues in TMV to VII for binding of different tachykinin receptor agonistsand antagonists to the hNK₂R. With regard to the residues examined,it appears that the binding of linear peptide antagonists is affectedin a similar manner to that of agonists, whereas the chemicalmodification introduced in the cyclic backbone of MEN 11420 partiallychanged the regions of the receptor that provide high-affinitybinding for this ligand. The binding of agonists and antagonists(of both peptide and nonpeptide nature) to the hNK₂R only partlyoverlaps.

	Footnotes

Accepted for publication April 6, 1999.

Received for publication January 29, 1999.

Send reprint requests to: Dr. Anna Rita Renzetti, Pharmacology Department, Menarini Ricerche S.p. A., Via Rismondo 12A, I-50131 Florence, Italy.

	Abbreviations

SP, substance P; CHO, Chinese hamster ovary; NKA, neurokinin A; NKB, neurokinin B; TM, transmembrane segment; $alpha$ -MEM, minimum essential medium $alpha$ -modification; DHFR, dihydrofolate reductase; hNK₂R, human tachykinin NK₂ receptor; FCS, fetal calf serum.

	References

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