The Biologically Crucial C Terminus of Cholecystokinin and the Non-peptide Agonist SR-146,131 Share a Common Binding Site in the Human CCK1 Receptor. EVIDENCE FOR A CRUCIAL ROLE OF MET-121 IN THE ACTIVATION PROCESS

doi:10.1074/jbc.M108563200

The Biologically Crucial C Terminus of Cholecystokinin and the Non-peptide Agonist SR-146,131 Share a Common Binding Site in the Human CCK1 Receptor

EVIDENCE FOR A CRUCIAL ROLE OF MET-121 IN THE ACTIVATION PROCESS^*

Chantal Escrieut, Véronique Gigoux, Elodie Archer, Sophie Verrier, Bernard Maigret^§, Raymond Behrendt^¶, Luis Moroder^¶, Eric Bignon, Sandrine Silvente-Poirot, Lucien Pradayrol, and Daniel Fourmy^**

From INSERM Unite 531, Institut Louis Bugnard, Centre Hospitalier Universitaire Rangueil, Bat. L3, 31403 Toulouse Cedex 4, France, the ^§ Laboratoire de Chimie Théorique, Université de Nancy, 54506 Vandoeuvre les Nancy, France, the ^¶ Max-Planck-Institut für Biochemie, 82143 Martinsried, Germany, and Sanofi-Synthelabo, 195 route d'Espagne, 31036 Toulouse Cedex, France

Received for publication, September 6, 2001, and in revised form, November 21, 2001

ABSTRACT

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

The cholecystokinin (CCK) receptor-1 (CCK1R) is a G protein-coupled receptor, which mediates important central and peripheralcholecystokinin actions. Our aim was to progress in mapping ofthe CCK1R binding site by identifying residues that interact withthe methionine and phenylalanine residues of the C-terminal moietyof CCK because these are crucial for its binding and biologicalactivity, and to determine whether CCK and the selective non-peptideagonist, SR-146,131, share a common binding site. Identificationof putative amino acids of the CCK1R binding site was achievedby dynamics-based docking of the ligand CCK in a refined three-dimensionalmodel of the CCK1R using, as constraints, previous results thatidentified contact points between residues of CCK and CCK1R (Kennedy,K., Gigoux, V., Escrieut, C., Maigret, B., Martinez, J., Moroder,L., Frehel, D., Gully, D., Vaysse, N., and Fourmy, D. (1997) J.Biol. Chem. 272, 2920-2926 and Gigoux, V., Escrieut, C., Fehrentz,J. A., Poirot, S., Maigret, B., Moroder, L., Gully, D., Martinez,J., Vaysse, N., and Fourmy, D. (1999) J. Biol. Chem. 274, 20457-20464).By this approach, a series of residues forming connected hydrophobicclusters were identified. Pharmacological and functional analysisof mutated receptors indicated that a network of hydrophobic residuesincluding Cys-94, Met-121, Val-125, Phe-218, Ile-329, Phe-330,Trp-326, Ile-352, Leu-356, and Tyr-360, is involved in the bindingsite for CCK and in the activation process of the CCK1R. Withinthis hydrophobic network, the physico-chemical nature of residue121 seems to be essential for CCK1R functioning. Finally, thebiological properties of mutants together with dynamic dockingof SR-146,131 in the CCK1R binding site demonstrated that SR-146,131occupies a region of CCK1R binding site which interacts with theC-terminal amidated tripeptide of CCK, i.e. Met-Asp-Phe-NH₂. Thesenew and important insights will serve to better understand theactivation process of CCK1R and to design or optimizeligands.

INTRODUCTION

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Cholecystokinin (CCK)¹ is a neuropeptide that has a wide spectrum of biological actions. CCK is composed of several molecularvariants, the octapeptide (CCK-8: Asp-Tyr(SO₃H)-Met-Gly-Trp-Met-Asp-Phe-NH₂)being the major fully active one (1, 2). Two CCK receptorshave been characterized pharmacologically, biologically and subsequentlycloned, the CCK1 receptor (abbreviated CCK1R, previously namedCCKA receptor) and the CCK2 receptor (abbreviated CCK2R, previouslynamed CCK-B/gastrin receptor), which both belong to the superfamilyof G protein-coupled receptors (3, 4). The CCK1R and CCK2Rcan exist in several conformational states, which bind CCK withhigh, low, and very low affinities, respectively, and share thefunctional coupling to phospholipase C, via binding to heterotrimericGTP-binding protein(s) (5-7). CCK1R-mediated effects includecontrol of gallbladder contraction, pancreatic exocrine secretion,gastric emptying and gut motility, and satiety (8, 9). Thewide spectrum of biological functions regulated by the CCK1R makesit a candidate target for a therapeutic approach in a number ofdiseases related to nutrient assimilation. This led a number ofacademic and pharmaceutical research groups to design specificand highly potent agonists and antagonists for this receptor (8,9).

Pharmacological studies have shown that chemically distinct molecules such as peptides, peptoids, and non-peptides can bindto the CCK1R with very close affinities (8, 9). On the otherhand, within each chemical family of CCK1R ligands, compoundshaving close structures are agonists, partial agonists, or antagonists,indicating that appropriate modifications within the pharmacophoreswitches an agonist to an antagonist and vice versa. This canbe illustrated with both peptide and non-peptide ligands of CCK1R.For instance, JMV 179, a CCK heptapeptide analogue in which theC-terminal amidated phenylalanine and the L-tryptophan have beenreplaced by a phenylethyl ester moiety and a D-tryptophan, respectively,is a full CCK1R antagonist (10). This antagonist has been convertedto JMV 180, a peptide exhibiting dual agonistic/antagonistic activity,by exchanging the D-tryptophan for an L-tryptophan (7, 11).Another interesting example came from the discovery of the non-peptideCCK1R agonist, SR-146,131, by chemical modification of the CCK1Rantagonist, SR-27,897 (12, 13) (Fig. 1). These examples, whichcould probably be extended to multiple G protein-coupled receptors,raise the important questions of whether closely related ligandshaving opposite biological activities share the same binding siteand of which intrinsic mechanism(s) at the binding site levelgovern(s) G protein-coupled receptorfunctioning.

One of our recent objectives has been to define the agonist binding site on the CCK1R and to identify interactions betweencritical residues of that binding site and chemical functionsof the pharmacophoric domain of CCK (Figs. 1 and 3). Amino acidswithin three regions of the CCK1R were identified as belongingto the binding site for CCK. Trp-39 and Gln-40, located at thetop of transmembrane helix I, were shown to interact directlywith the N-terminal portion of CCK (14). Met-195 and Arg-197,located in the second extracellular loop, were then shown to interactwith the sulfated tyrosine (15, 16). More recently, Arg-336and Asn-333, at the top of helix VI, were demonstrated to pairwith the Asp carboxylate and the C-terminal amide of CCK, respectively(17). The first two identified amino acids of the CCK1R (Trp-39and Gln-40) contribute weakly to CCK1R affinity for and responseto CCK, whereas all others play a more critical role because oftheir interaction with residues of CCK, which are essential forboth binding and biological activity of CCK. However, contactpoints within the CCK1R binding site for other key residues ofCCK such as the Trp, Met, and Phe residues have not yet beenidentified.

To progress in the mapping of the CCK1R binding site(s), the three-dimensional model of the CCK1R·CCK complex was optimized,leading to the identification of putative amino acids involvedin the interaction with the Met and Phe residues of the ligandCCK. Mutation of candidate residues and extensive characterizationof the resulting mutants allowed us to position the C-terminalbiological part of CCK in hydrophobic pockets formed by aromaticand nonaromatic amino acids located in the upper half of transmembranehelices III, V, VI, and VII. Our data, therefore, refute the modelof the CCK1R·CCK complex proposed by other investigators in whichthe C terminus of CCK interacts with an amino acid residue (Trp-39)of helix I (18). Furthermore, binding site for the non-peptideagonist SR-146,131 was identified and experimentally validatedas overlapping with that of the C-terminal tripeptide of CCK.Finally, the role of Met-121 located on helix III in the activationof the CCK1R by agonists wasdemonstrated.

EXPERIMENTAL PROCEDURES

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Materials-- The C-terminal nonapeptide analogue (Nle)-CCK-9 (Fig. 1) was synthesized as described previously (19). The other analoguesof Fig. 1 were synthesized on an ACT 396 synthesizer by applyingthe Fmoc (N-(9-fluorenyl)methoxycarbonyl)/ter-butyl chemistryand chlorotrityl resin (PepChem). Upon deprotection and resincleavage with trifluoroacetic acid/H₂O/triethylsilane (9:0.5:0.5)at 0 °C, the crude products were precipitated by methyl tert-butylether/hexane (2:1) and purified by preparative RP-HPLC (250/20Nucleosil 300/5 C18; Machery & Nagel) and characterized by analyticalRP-HPLC (linear gradient acetonitrile/2% H₃PO₄ from 5 to 90% in15 min; 125/4 Nucleosil 100/5 C18; Machery & Nagel) and ESI-MS(API 165; PerkinElmer Life Sciences); (Ala-7)-CCK: homogeneouson analytical RP-HPLC (t_R = 6,7 min); ESI-MS: m/z: 1209.4 [M +H⁺]; M_r = 1209.5 calculated for C₅₂H₆₉N₁₄O₁₈S₁; (Ala-9)-CCK: homogeneouson analytical RP-HPLC (t_R = 6,5 min); ESI-MS: m/z: 1176.2 [M +H⁺]; M_r = 1175.5 calculated for C₄₉H₇₁N₁₄O₁₈S₁; (Gln-7)-CCK: homogeneouson analytical RP-HPLC (t_R = 7,6 min); ESI-MS: m/z: 1266.8 [M +H⁺]; M_r = 1266.5 calculated for C₅₄H₇₂N₁₅O₁₉S₁. The non-peptideantagonist of the CCK1R, 1-[2-(4-(2-chlorophenyl)thiazol-2-yl)aminocarbonyl-indoyl]aceticacid (SR-27,897), and its tritiated derivative, [³H]SR-27,897 (31 Ci/mmol), as well as the non-peptide agonist ofthe CCK1R, 2-[4-(4-chloro-2-,5-dimethoxyphenyl)-5-(2-cyclohexylethyl)thiazol-2-ylcarbamoyl]-5,7-dimethyl-indol-1-yl-1-aceticacid (SR-146,131), were donated by Sanofi-Synthelabo (Toulouse,France) (12, 13). ¹²⁵INa and myo-[³H]inositol (5 µCi/ml) were from Amersham Biosciences, Inc., LesUlis, France. (Thr,Nle)-CCK-9 was conjugated with Bolton-Hunterreagent, purified, and radioiodinated as described previously(20). The specific activity of the radioiodinated peptide was1600-2000 Ci/mmol. All other chemicals were obtained from commercialsources.

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Fig. 1. Ligands used to map the CCK1R binding site.

Computer Modeling of the CCK1R and CCK1R·CCK Complex-- The model of empty CCK1R was built using the transmembrane (TM) helical arrangement found in the bacteriorhodopsin crystalstructure as starting point (21). It was then modified accordingto the rhodopsin crystal structure (22, 23) and to the mutantdata base "input/output" information scheme defined in the Viseurprogram (24). Extracellular and intracellular loops connectingthe transmembrane helices were then added to the preliminary seven-helixbundle, and the structural model was optimized by the use of simulatedannealing procedures. The entire system was finally relaxed andsubmitted to a 1-ns molecular dynamics with possible translationaland rotational movements of individual TM helices taken into account.The final model respects most transmembrane arrangements foundin the recent x-ray structure of rhodopsin (23). For dockingof CCK ligand into the CCK1R binding site, experimental data thatidentified contact points between residues Trp-39 and Gln-40 andthe N-terminal moiety of CCK served as a first constraint to placeCCK within the CCK1R grove (14). In a first step, manual dockingwas achieved by taking into account molecular electrostatic potentialsat the top of the receptor grove. The resulting complex was submittedto annealing molecular dynamics calculations. The resulting theoreticalpositioning of CCK into the CCK1R binding site was experimentallyvalidated by two-dimensional site-directed mutagenesis. By doingso, Met-195-Arg-197, Arg-336, and Asn-333 were shown to belongthe CCK1R binding site and to interact with the sulfated tyrosineof CCK, the Asp-8 carboxylate, and the C-terminal amide, respectively(15-17). The program package (Insight II, Discover, Homology, Biopolymer)from Molecular Simulations Inc. (San Diego, CA) was used for allthecalculations.

Site-directed Mutagenesis and Transfection of COS-7 Cells-- Mutant receptor cDNAs were constructed by oligonucleotide-directed mutagenesis (QuikChange^TM site-directed mutagenesis kit,Stratagene, France) using the human CCK1R cDNAs cloned into pRFENeovector as template (25). Oligonucleotides were designed to includea silent restriction site to facilitate analysis of mutant constructsby restriction endonuclease digestion. The presence of the desiredand the absence of undesired mutations were confirmed by automatedsequencing of both cDNA strands (AppliedBiosystems).

COS-7 cells (1.5 × 10⁶) were plated onto 10-cm culture dishes and grown in Dulbecco's modified Eagle's medium containing 5%fetal calf serum (complete medium) in a 5% CO₂ atmosphere at 37°C. After overnight incubation, cells were transfected with 2.5µg/plate of pRFENeo vectors containing the cDNA for the wild-typeor mutated CCK1 receptors, using a modified DEAE-dextran method.Cells were transferred to 24-well plates at a density of 80,000-150,000cells/well 24 h aftertransfection.

Receptor Binding Assay-- Approximately 24 h after the transfer of transfected cells to 24-well plates, the cells were washed with phosphate-bufferedsaline, pH 6.95, 0.1% BSA and then incubated for 60 min at 37°C in 0.5 ml of Dulbecco's modified Eagle's medium, 0.1% BSA witheither 71 pM ¹²⁵I-BH-(Thr,Nle)-CCK-9 or 1.83 nM [³H]SR-27,897 in the presence or the absence of competing agonistsor antagonists. The cells were washed twice with cold phosphate-bufferedsaline, pH 6.95, containing 2% BSA, and cell-associated radioligandwas collected with 0.1 N NaOH added to each well. The radioactivitywas directly counted in a $gamma$ counter (Auto-Gamma, Packard, DownersGrove, IL) or added to scintillant and counted for the tritiatedradioligand.

Inositol Phosphate Assay-- Approximately 24 h after the transfer to 24-well plates and following overnight incubation in complete medium containing 2µCi/ml myo-2-[³H]inositol, the transfected cells were washed with Dulbecco'smodified Eagle's medium and then incubated for 30 min in 1 ml/wellDulbecco's modified Eagle's medium containing 20 mM LiCl at 37°C. The cells were washed with PI buffer at pH 7.45: phosphate-bufferedsaline containing 135 mM NaCl, 20 mM HEPES, 2 mM CaCl₂, 1.2 mMMgSO₄, 1 mM EGTA, 10 mM LiCl, 11.1 mM glucose, and 0.5% BSA. Thecells were then incubated for 60 min at 37 °C in 0.3 ml of PIbuffer with or without ligands at various concentrations. Thereaction was stopped by adding 1 ml of methanol/chlorhydric acidto each well, and the content was transferred to a column (DowexAG 1-X8, formate form, Bio-Rad) for the determination of inositolphosphates. The columns were washed twice with 3 ml of distilledwater and twice more with 2 ml of 5 mM sodium tetraborate, 60mM sodium formate. The content of each column was eluted by additionof 2.5 ml of 1 M ammonium formate, 100 mM formic acid. 0.5 mlof the eluted fraction was added to scintillant, and $beta$ radioactivitywascounted.

Membrane Preparation-- Approximately 65 h after transfection, the cells were washed three times with phosphate-buffered saline, pH 6.95, scrapedfrom the plate in 10 mM Hepes buffer, pH 7.0, containing 0.01%soybean trypsin inhibitor, 0.1% bacitracin, 0.1 mM phenylmethylsulfonylfluoride and frozen in liquid N₂. After thawing at 37 °C, thecells were subjected to another cycle of freeze/thawing and thencentrifuged at 25,000 × g for 20 min. The membrane pellet wasresuspended in 50 mM Hepes buffer, pH 7.0, containing 115 mM NaCl,5 mM MgCl₂, 0.01% soybean trypsin inhibitor, 0.1% bacitracin,1 mM EGTA, 0.1 mM phenylmethylsulfonyl fluoride (binding buffer);aliquoted; and stored at $-$ 80 °C until use. Membrane protein concentrationswere determined using the Bio-Rad protein assay kit. To assessthe effect of GTP $gamma$ S on CCK binding, membranes from transfectedCOS-7 cells (0.4-4 µg of proteins) were incubated with 71 pM ¹²⁵I-BH-(Thr,Nle)-CCK-9 in the absence or in the presence of increasingconcentrations GTP $gamma$ S in binding buffer for 120 min at 25 °C. Nonspecificbinding was measured in the presence of 1 µM CCK.

RESULTS

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Importance of Methionine 7 and Phenylalanine 9 of CCK for Binding and Activation of the CCK1R-- Previous structure-activity studies using synthetic replicates of CCK and pancreatic acini from rodents, a biological modelnaturally expressing CCK1R, have clearly shown the importanceof both Met and Phe residues for binding and activity of CCK;however, no such study has been reported for human CCK1R in anyexpression system (26). Therefore, we first determined to whatextent the Met and Phe side chains contribute to the affinityof CCK for human CCK1R expressed in COS-7 cells and to its capacityto induce production of total inositol phosphates. As shown inFig. 2, replacement of Met-7 in CCK by an Ala residue caused 4000-and 390-fold decrease in affinity and potency, respectively. Incontrast, substitution of Met-7 by Nle did not affect affinityand potency of CCK. Furthermore, exchange of Phe for Ala was foundto induce a 4900- and 2700-fold decrease in affinity and potencyof the analogues, respectively. The efficacies of (Nle-7)-CCK,(Met-7)-CCK, and (Ala-7)-CCK were comparable, whereas that of(Ala-9)-CCK reached only 40% referred to the parent analogue (Nle-7)-CCK.Hence, both Met-7 and Phe-9 side chains contribute significantlyto receptor binding and activation potency of CCK, confirmingdata obtained previously on receptors from rodents and guineapig (27, 28). These results also confirm that replacementof Met-7 with Nle does not affect affinity and activity of CCK.

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Fig. 2. Importance of Met-7 and Phe-9 of CCK for binding (a) and production of inositol phosphates (b). a, COS-7 cells expressing the human wild-type CCK1R were incubated with ¹²⁵ I-BH-(Thr,Nle)-CCK-9 alone or in the presence of increasing concentrations of competition peptide as described under "Experimental Procedures." Specific binding in each assay is expressed as percentage of specific binding in absence of competitor. Affinity calculated from three individual determinations was (IC₅₀, concentration of competitor inhibiting 50% of specific binding): (Nle-7)-CCK: 1.2 ± 0.1 nM; (Met-7)-CCK: 1.3 ± 0.2 nM; (Ala-7)-CCK: 4,200 ± 90 nM; (Ala-9)-CCK: 5990 ± 580 nM. b, production of inositol phosphates by COS-7 expressing the wild-type human CCK1R receptor upon stimulation by CCK analogues was assayed as described under "Experimental Procedures." Results are expressed as percentage of maximal inositol phosphate production obtained after stimulation by each peptide. Efficacies (maximum production of inositol phosphates) of (Nle-7)-CCK, (Met-7)-CCK, and (Ala-7)-CCK were similar, whereas that of (Ala-9)-CCK reached only 40% relative to (Nle-7)-CCK. Potency of each agonist (D₅₀: concentration of agonist producing 50% of maximal response) was calculated from three individual experiments using the GraphPad Prism program (Software). D₅₀ values were: (Nle-7)-CCK: 1.3 ± 0.1 nM; (Met-7)-CCK: 1.0 ± 0.1 nM; (Ala-7)-CCK: 507 ± 29 nM; (Ala-9)-CCK: 3,500 ± 1,000 nM.

Identification of Candidate Amino Acid Residues of the CCK1R for Interaction with Nle/Met-7 and Phe-9 of CCK Using Molecular Modeling-- Considering the major anchoring points of CCK inside the receptor discovered in our previous studies, it appears that theNle/Met-7 residue is located in the vicinity of a hydrophobicpocket constituted by residues Leu-50, Ile-51, Leu-53, Pro-101,Val-125, Met-121, Ileu-352, and Leu-356. In the model of the (WT)-CCK1R,both Nle-7 or Met-7 side chains are positioned in the same way.The Phe-9 aromatic side chain of CCK is also positioned into awell defined cavity delineated by Phe-330 at the bottom, and Pro-177,Val-125, Leu-214, Ile-329 around Phe-330, which itself belongsto a large aromatic cluster constituted by the side chains ofCys-94, Phe-130, Trp-166, Phe-170, Phe-218, Phe-322, Phe-323,Trp-326, and Tyr-360. These two pockets are connected via theVal-125 side chain so that helix movements changing the structureof one of them may have consequences on the other. Examinationof the organization of the two clusters in the three-dimensionalmodel of the CCK1R·CCK complex suggests that not only a single,but several hydrophobic residues are contributing to the bindingenergy between Nle/Met-7 or Phe side chains of CCK and the CCK1R.As a consequence and unlike the charged residues of the bindingpocket that were characterized previously, a mutation of onlyone of these amino acid residues of the CCK1R was not expectedto induce changes in affinity and biological potency of the CCK1Rto an extent comparable with effects caused by replacements ofNle/Met or Phe in CCK.

Effects of CCK1R Mutations on CCK1R Expression and Affinity for the Non-peptide Antagonist SR-27,897-- Among all residues forming hydrophobic clusters around the Nle/Met-7 and Phe-9 side chains, in a first instance those in closestcontact were chosen for mutagenesis experiments (Fig. 3). Thesewere exchanged for amino acids lacking the chemical functionsthought to be responsible for the interactions. In addition, Met-121and Ile-329, which appear to be important for the equilibriumwithin the hydrophobic clusters surrounding Nle/Met-7 and Phe-9of CCK, were each exchanged for more bulky and hydrophobic residues,namely Val and Phe, respectively. In a first series of experiments,COS-7 cells expressing mutated receptors were assayed for bindingof the non-peptide antagonist [³H]SR-27,897. Indeed, binding of this antagonist, unlike that ofan agonist, offers the advantage of allowing detection of CCK1Rindependent of the coupling state to G protein(s), thus yieldingaccurate expression levels of all mutants (15, 17). Ligandbinding data are summarized in Table I. No binding of [³H]SR-27,897 was found with the (I329F)-CCK1R mutant, a resultthat could be interpreted at this stage of the study either byan absence of expression of the mutant or by a direct or indirecteffect of the mutation on receptor affinity for the ligand. Resultswith all other CCK1R mutants confirmed their expression at COS-7cell surface at levels varying from 0.6 to 10.0 pmol/10⁶ cells, which permitted further characterization. In addition,the binding data clearly revealed that all mutants (except (I329F)-CCK1R)bind the non-peptide antagonist with an affinity very close tothat of (WT)-CCK1R. This finding indicates that the mutationsdid not dramatically disturb the conformational state of the CCK1Rand that the mutated residues are not directly involved in thebinding pocket of the antagonist SR-27,897.

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Fig. 3. Simplified representation of the CCK1 receptor and of its agonist binding site. Top, side view of the three-dimensional model of the active high affinity CCK1R·CCK complex. The model was built as described under "Experimental Procedures" using the program package from Molecular Simulations Inc. (San Diego, CA). For clarity, the detailed view shows only identified amino acid side chains in interaction with CCK in the phospholipase C-coupled high affinity CCK1R·CCK complex. Bottom, serpentine representation of the human CCK1R with the amino acids involved in binding and activity marked. Amino acids that are the subject of the current study are yellow. Other mentioned amino acids, Trp-39/Gln-40, Met-195/Arg-197, Arg-336, and Asn-333, have been demonstrated previously to interact with the N-terminal moiety, the sulfated tyrosine, the Asp-8 carboxylate, and the amide of CCK, respectively (14-17).

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Table I
Effects of CCK1R mutations on CCK1R expression and affinity for the non-peptide antagonist, SR-27,897 and the peptide agonist, CCK
Binding properties of mutated CCK1R were determined using the non-peptide antagonist radioligand [³H]SR-27,897 (1.83 nM) and the peptide agonist radioligand ¹²⁵I-BH-(Thr,Nle)-CCK-9 (71 pM). Data from three to six individual experiments from different batches of transfected cells were analyzed, and K_d values were determined using kell program (Biosoft) and were expressed as mean ± S.E. The mutation factors (F_mut) were calculated as K_d (mutated receptor)/K_d ((WT)-CCK1R). ND, not detectable.

Effects of Mutations on the CCK1R Affinity for CCK-- To verify if the amino acid residues identified by molecular modeling are effectively involved in the CCK1R binding pocketfor CCK, COS-7 cells expressing the mutated receptors were testedfor binding of the agonist radioligand (¹²⁵I-BH-(Thr,Nle)-CCK-9). Binding parameters calculated from Scatchardanalysis of binding values are summarized in Table I. Accordingto these binding data, the CCK1R mutants can be classified infour categories. A first series of mutants, i.e. (C94L)-, (M121A)-,(M121V)-, (F218A)-, and (F330A)-CCK1R, bind the radioligand CCKto a single class of binding sites with affinities that are 62-,1.8-, 16-, 2.3-, and 10.5-fold lower that that of the high affinitysites of the (WT)-CCK1R, respectively (Table I). Several of themutants such as (L356A)-, (Y360F)-, and (I329A)-CCK1R bind CCKto two affinity classes of binding sites as does the wild-typereceptor; however, the affinity of either the high or low affinitycomponent, or both, was modified. For instance, (L356A)-CCK1Rand (I329A)-CCK1R showed minor changes in their high affinitysites relative to the (WT)-CCK1R, but a 5.5-8.5-fold decreasein affinity of the low affinity sites, respectively. A third categoryof mutants, i.e. (L50A)-, (I51A)-, (L53A)-, (V125A)-, and (W326A)-CCK1R,exhibited binding features that were very similar to those ofthe (WT)-CCK1R because radioligand binding to two affinity classesof binding sites was observed, both with affinities similar tothose of their equivalents in the (WT)-CCK1R. Finally, two mutants,i.e. (I329F)- and (I352A)-CCK1R, did not bind ¹²⁵I-BH-(Thr,Nle)-CCK-9, even when the radioligand concentrationwas increased up to 250 pM.

The maximal number of binding sites for CCK were either similar as in the mutants (C94L)-, (M121V)-, (M121A)-, (F218A)-, (F330A)-CCK1R,or lower (all other mutants) to expression levels calculated frombinding experiments with the non-peptide antagonist [³H]SR-27,897.

Effects of Mutations on CCK1R Functional Coupling to Phospholipase-C-- The biological function of the mutated receptors was evaluated by determining inositol phosphate accumulation in transfectedCOS-7 cells upon (Nle-7)-CCK stimulation. Table II summarizespotency (D₅₀) and efficacy (E_max) of the different mutants inresponse to (Nle-7)-CCK stimulation. The mutants (L50A)-, (I51A)-,(L53A)-, (M121A)-, and (F218A)-CCK1R were found to exhibit biologicalpotencies very similar to that of the (WT)-CCK1R. However, thebiological efficacy of some of these mutants was affected. Indeed,maximal production of inositol phosphates by the mutants (I51A)-,(M121A)-, and (F218A)-CCK1R reached 63, 48, and 35% of that achievedby the (WT)-CCK1R. Conversely, the mutants (C94L)-, (I352A)-,(L356A)-, (V125A)-, (W326A)-, (I329A)-, (I329F)-, (F330A)-, and(Y360F)-CCK1R showed, respectively, a 28-, 213-, 29-, 2.3-, 4.3,38-, 468-, 2.6-, and 32-fold decrease in their potency to stimulateinositol phosphate production if compared with the (WT)-CCK1R.The biological efficacy of (C94L)- and (F330A)-CCK1R was reducedto 45 and 57% of that of the (WT)-CCK1R. It is worthy to notethat (I329F)-CCK1R, which failed to bind both the CCK and SR-27,897radioligands, was capable of inducing production of inositol phosphatesafter (Nle-7)-CCK stimulation, although its potency was 507-folddecreased compared with the (WT)-CCK1R. This result suggests thatthe absence of binding was likely because of a drastically reducedaffinity of the mutant for CCK and SR-27,897. Indeed, this explanationwas indirectly confirmed with experiments, which showed that thepotency of SR-27,897 to inhibit CCK-induced production of inositolphosphates by COS-7 cells expressing (I329F)-CCK1R was 625-folddecreased if compared with the (WT)-CCK1R (1500 nM versus 24 nM,n = 2, not shown). Finally, and very surprisingly, the mutant(M121V)-CCK1R failed to induce production of inositol phosphateupon stimulation with (Nle-7)-CCK, whereas (M121A)-CCK1R retainedthe ability to couple to phospholipase C, even though with a moderateefficacy (48% of that of (WT)-CCK1R; see Table II and Fig. 4).These data suggest that Met-121 plays a crucial role in the couplingof CCK1R to G proteins(s), although this residue is located inthe upper part of helix III. Indeed, the importance of the sidechain of residue 121 in the CCK1R for G protein(s) coupling wasfurther evaluated by experiments, which showed that the nonhydrolyzableanalogue of GTP, GTP $gamma$ S, did not dissociate binding of ¹²⁵I-BH-(Thr,Nle)-CCK-9 to (M121V)-CCK1R, whereas it dissociatedbinding of CCK to (M121A)- and (WT)-CCK1R to extents that agreewith the biological efficacies of these receptors (Fig. 4).

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Table II
Effects of CCK1R mutations on (Nle-7)-CCK-induced production of inositol phosphates
Data from three to six individual experiments from different batches of transfected cells were analyzed. Results are expressed as percentage of maximal inositol phosphate production obtained in COS-7 expressing the wild-type CCK1R after stimulation by (Nle-7)-CCK. Potency (D₅₀) and efficacy (E_max) for the different mutants were calculated using GraphPad Prism program (Software). The mutation factors (F_mut) were calculated as D₅₀ (mutated receptor)/D₅₀ ((WT)-CCK1R). ND, not detectable.

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Fig. 4. Effects of Met-121 $right-arrow$ Ala and Met-121 $right-arrow$ Val mutations in CCK1R on functional coupling to GTP binding protein(s) and phospholipase C. a, functional coupling to GTP-binding protein(s) was evaluated by determining the effect of the nonhydrolyzable analogue of GTP, GTP $gamma$ S, at 100 µM on ¹²⁵I-BH-(Thr,Nle)-CCK-9 binding to membranes prepared from COS-7 cells expressing (WT)-CCK1R, (M121A)-CCK1R, or (M121V)-CCK1R. Residual specific binding in presence of GTP $gamma$ S is expressed as the percentage of specific binding obtained in absence of GTP $gamma$ S. Results are from three individual determinations. b, effects of Met-121 mutations on efficacy of CCK1R to couple to phospholipase C, as determined by inositol phosphate production by transfected COS-7 cells. The figure represents inositol phosphate production upon stimulation by (Nle-7)-CCK at a concentration of 1 µM. Results are from three to five individual determinations.

Effets of Nle/Met Exchange in CCK and Met-121 Mutations in CCK1R-- In all our studies regarding mapping of the CCK1R binding sites including the current one, we used a CCK analogue in whichMet-7 was replaced by a Nle residue because of its high stabilitycompared with Met in terms of possible oxidation on handling (19).The use of this analogue was supported by previous findings thatconfirmed its full biological potency. This was also confirmedin the present study, as shown in Fig. 2, where replacement ofMet-7 with Nle was found to be without any effect on affinityand activity of the ligand. According to the three-dimensionalmodel of the CCK1R·CCK complex, Nle (or Met) of CCK is insertedinto a hydrophobic pocket including residues Leu-50, Ile-51, Leu-53,Cys-94, Met-121, Val-125, Ile-352, and Leu-356. To analyze whetherthe biological efficacy of mutated receptors was dependent onthe presence of Met-7 in CCK, a series of experiments was performed.Both competition binding and inositol phosphate production assaysclearly demonstrated that (Met-7)-CCK bound to and stimulatedall the mutants in a manner identical to that for the (Nle-7)-CCKanalogue (data not shown), except for (M121V)-CCK1R and (M121A)-CCK1R.Indeed, (M121V)-CCK1R, which was unable to induce production ofinositol phosphates upon (Nle-7)-CCK stimulation, responded toa (Met-7)-CCK stimulation with a maximum that reached 33% of thatobtained with the (WT)-CCK1R, and with a potency that was only12.5-fold decreased (EC₅₀: 12.4 ± 1.1 nM versus 1.0 ± 0.1 nM,n = 3) (Fig. 5). Interestingly, in a competition binding assaywith ¹²⁵I-BH-(Thr,Nle)-CCK-9, the affinity of (Met-7)-CCK for (M121V)-CCK1Rwas very similar to that of (Nle-7)-CCK (IC₅₀: 25.4 ± 0.2 nM versus19.0 ± 1.3). Moreover, (M121A)-CCK1R was found to couple to productionof inositol phosphates upon (Met-7)-CCK stimulation with a higherefficacy than it did upon (Nle-7)-CCK stimulation (70% versus48% relative to (WT)-CCK1R, not illustrated). Therefore, doubleexchange of Met tor Nle in CCK and Met-121 to Val in CCK1R yieldedan inactive CCK1R·CCK complex. On the other hand, the presenceof Met-7 in CCK was required for functional coupling of (M121V)-CCK1Rand enhanced that of the (M121A)-CCK1R mutant.

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Fig. 5. Effects of Nle/Met exchange in CCK and Met-121 mutations in CCK1R on CCK1R-mediated production of inositol phosphates. Inositol production assays were conducted as described under "Experimental Procedures." Results from all the CCK1R·CCK complexes are expressed as percentage of maximal inositol phosphate production obtained in COS-7 expressing the wild-type CCK1R after stimulation by (Nle-7)-CCK. Potency (D₅₀) and efficacy (E_max) for the different complexes were: (WT)-CCK1R·(Nle-7)-CCK, D₅₀: 1.3 ± 0.1 nM, E_max:100; (WT)-CCK1R·(Met-7)-CCK, D₅₀: 1.0 ± 0.1 nM, E_max: 100; (WT)-CCK1R·(Gln-7)-CCK, D₅₀: 12.5 ± 2.4 nM, E_max: 95; (M121V)-CCK1R·(Nle-7)-CCK, E_max: 0; (M121V)-CCK1R·(Met-7)-CCK, D₅₀: 12.4 ± 1.1 nM, E_max: 33; (M121V)-CCK1R·(Gln-7)-CCK, D₅₀: 22.0 ± 4.5 nM, E_max: 44; (M121Q)-CCK1R·(Nle-7)-CCK, D₅₀: 1.8 ± 1.5 nM, E_max: 95. Results are from three to five individual determinations.

The intent of the mutation of Met-121 to Val was to disturb the hydrophobicity pattern within the pocket surrounding Nle ofCCK. This mutation, which was expected to decrease the bindingaffinity of the CCK1R for CCK, effectively caused a 16-fold dropin the affinity of the receptor for the ligand and, surprisingly,made activation of that receptor dependent on the presence ofMet-7 in CCK. To further explore the role of residue 121 of theCCK1R and of Met-7 of CCK, the (M121Q)-CCK1R mutant was expressedand a (Gln-7)-CCK analogue was synthesized. Competition bindingto (WT)-CCK1R revealed that substitution of Met-7 residue by Glnin the ligand affects only weakly the affinity of the peptide(K_d(1): 12.5 ± 2.4 nM, K_d(2): 332 ± 78 nM, n= 3, not shown). In agreement with this high binding affinity,(Gln-7)-CCK was found to stimulate inositol phosphates with highpotency (D₅₀: 13.8 ± 2.2 nM) (Fig. 5). Furthermore, the mutant(M121Q)-CCK1R binds ¹²⁵I-BH-(Thr,Nle)-CCK-9 at two classes of binding sites with bindingparameters similar to those of the (WT)-CCK1R (K_d(1):0.8 ± 0.6 nM, K_d(2): 120 ± 50 nM, not illustrated) andthis binding is coupled to the production of inositol phosphatesat a potency similar to the (WT)-CCK1R upon (Nle-7)-CCK stimulation(EC₅₀: 1.8 ± 0.6 nM, E_max: 95% of (WT)-CCK1R). Finally, (Gln-7)-CCKstimulates the (M121V)-CCK1R mutant as did (Met-7)-CCK (Fig. 5).Altogether, this set of results excludes a direct involvementof the sulfur atoms of Met-7 of CCK and Met-121 of the CCK1R inthe mechanism of activation of the receptor. However, the presenceof a polar atom within the hydrophobic cluster surrounding thesetwo residues appears to be required for CCK1Ractivation.

Using a molecular dynamic simulated annealing procedure, three-dimensional models of the different CCK1R·CCK complexes wasgenerated. As illustrated in Fig. 6, the location of the C-terminalpart of CCK was identical in the (WT)-CCK1R·(Met-7)-CCK and (WT)-CCK1R·(Nle-7)-CCKcomplexes (Fig. 6a), which is consistent with the identical bindingand functional properties of these complexes (Fig. 2). Conversely,in the (M121V)-CCK1R·(Nle)-CCK complex, the position of the liganddiffers as shown in Fig. 6b. Indeed, in this complex, the Val-121and Nle-7 residues are in tight contact leading to a deeper insertionof the peptide into the receptor grove. As a consequence, interactionsbetween Asn-333 and the C-terminal amide of the ligand are precludedand the aromatic ring of the CCK Phe residue is moved into thedirection of the Val-121 side chain. Reintroduction of Met-7 inCCK reverses these altered docking modes in the (M121V)-CCK1R·(Nle)-CCKcomplex, and the resulting structural models of the (M121V)-CCK1R·(Met)-CCKand (WT)-CCK1R·(Nle)-CCK complexes become very similar (Fig. 6,c and d). Hence, the positioning of the C-terminal part of CCKapparently differs in the (M121V)-CCK1R·(Nle)-CCK complex as theonly inactive complex from that in the active complexes.

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Fig. 6. Molecular modeling of the effects of Nle/Met exchange in CCK and Met-121 mutations in CCK1R on the positioning of the C terminus of CCK into the CCK1R binding site. A molecular dynamic simulated annealing procedure was used to generate the models. a, the postioning of the C-terminal part of CCK was rigorously identical in (WT)-CCK1R·(Met-7)-CCK and (WT)-CCK1R·(Nle-7)-CCK complexes; b, in contrast, the positioning of CCK was affected in (M121V)-CCK1R·(Nle)-CCK complex because positioning of the peptide in the receptor grove was deeper and, as a consequence, interactions between Asn-333 and the amide were disrupted and the aromatic ring of CCK Phe fold in the direction of Val-121 side chain; c and d, re-introduction of Met-7 in CCK reversed modifications of docking seen in (M121V)-CCK1R·(Nle)-CCK complex so that (M121V)-CCK1R·(Met)-CCK and (WT)-CCK1R·(Nle)-CCK complexes are very similar.

Effects of CCK1R Mutations on SR-146,131-induced Production of Inositol Phosphates-- SR-146,131 is an agonist having high affinity and specificity for the CCK1R. Although of non-peptidic nature, this compoundexhibits some structural similarities with the C-terminal partof CCK docked into the three-dimensional model of the CCK1R (Fig.1). This observation raised the interesting question of whetherthese structural similarities imply an overlapping of the bindingsites for the two ligands, SR-146,131 and CCK. A way to addressthis question would be to analyze the effects on binding of SR-146,131by the mutation of those residues in the receptor which were foundto be involved in CCK binding. However, as no labeled SR-146,131was available, these effects were determined by measuring SR-146,131-stimulatedproduction of inositol phosphates. The results (Table III) revealedthat residues Met-195 and Arg-197, which were shown previouslyto interact with the sulfated tyrosine of CCK, did not affectrecognition of SR-146,131. Conversely, residues Asn-333 and Arg-336,which were demonstrated previously to pair with the C-terminalamide and the carboxylate side chain of Asp-8 of CCK, respectively,are likely involved in recognition of SR-146,131 because theirmutation caused a 120- and 126-fold decrease in potency of inositolphosphate responses, respectively. Among the residues of the receptorthat were shown to interact with the Nle/Met-7 and Phe residues,several seem to be involved in SR-146,131-induced inositol phosphateproduction. In fact, the mutants (C94L)-, (I352A)-, (L356A)-,(V125A)-, (W326A)-, (I329A)-, (I329F)-, and (F330A)-CCK1R respondedto SR-146,131 stimulation with potencies that were 2.4-, 27-,23-, 6-, 6-, 18-, 600-, and 2.3-fold lower than that of the (WT)-CCK1R.These results strongly suggest that residues of the receptor thatare in close proximity of the C-terminal moiety of CCK ligandare also involved in recognition of the non-peptide SR-146,131ligand, whereas residues such as Met-195 and Arg-197, which interactwith the sulfated tyrosine residue located within the N-terminalportion of CCK, do not contribute to recognition of SR-146,131by the receptor. Interestingly, the (M121V)-CCK1R mutant coupledto production of inositol phosphate upon SR-146,131 stimulationwith a potency and efficacy very similar to those of the (WT)-receptor.Thus, SR-146,131 behaved as an agonist on (M121V)-CCK1R as did(Met-7)-CCK and (Gln-7)-CCK. It is also worthy to note that themutants (I51A)-, (C94L)-, (M121A)-, (F218A)-, and (F330A)-CCK1R,which showed decreased efficacies upon CCK stimulation, were alsoless efficient to induce inositol phosphate production upon SR-146,131stimulation (Table III).

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Table III
Effects of CCK1R mutations on SR-146,131-induced production of inositol phosphates
Data from three to four individual experiments from different batches of transfected cells were analyzed. Results are expressed as percentage of maximal inositol phosphate production obtained in COS-7 expressing the wild-type CCK1R after stimulation by SR-146,131. Potency (D₅₀) and efficacy (E_max) for the different mutants were calculated using GraphPad Prism program (Software). The mutation factors (F_mut) were calculated as D₅₀ (mutated receptor)/D₅₀ ((WT)-CCK1R). ND, not detectable.

Docking of SR-146,131 into the CCK1R Structural Model-- On the basis of above experimental data, dynamic docking of SR-146,131 into the three-dimensional model of the CCK1R was carriedout using a molecular dynamic simulated annealing procedure describedelsewhere. Compared with the docking of CCK the positioning ofSR-146,131 exhibits some similarities. Indeed, the SR-146,131carboxylate group interacts with the guanidino function of Arg-336,and its chloro-dimethoxy aromatic ring is positioned inside thesame pocket as the Phe-9 side chain of CCK (Fig. 7). Asn-333 ofthe CCK1R is also involved in interactions with the non-peptideagonist. This interaction occurs through a possible hydrogen bondbetween the Asn-333 carboxamido group and the chlorine of theligand, which could be activated by the two O-methyl groups. Thecyclohexane moiety of SR-146,131 is positioned in proximity tothe Cys-94, Val-125, Ile-352, and Leu-356 side chains, which areinvolved in the binding site of CCK (Fig. 7). It is noteworthythat the sulfur atom and the carbonyl of SR-146,131 are positionedalmost at the same place as the sulfur atom of the CCK Met-7 inthe CCK1R·CCK complex, with the indole group of SR-146,131 occupyingthe position of CCK Trp-6-Met-7 backbone.

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Fig. 7. Dynamic docking of the non-peptide agonist SR-146,131 into the CCK1R binding site. a, dynamic docking of the non-peptide agonist SR-146,131 into the CCK1R binding site. Docking was carried out on the basis of experimental data showing importance of certain amino acids for recognition of SR-146,131 in particular, Asn-333 and Arg-336. b, comparison between positions of SR-146,131 and (Nle)-CCK into CCK1R binding site. Both experimental tests of SR-146,131 on CCK1R mutants and its dynamic docking in the three-dimensional model agreed with a positioning of the non-peptide in the part of the CCK1R binding site that interacts with the C-terminal tripeptide of CCK, Met-Asp-Phe-NH₂. Note that the sulfur atom and the carbonyl group have a position similar to that of Nle/Met of CCK toward Met-121 of the CCK1R.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

The aim of the present study was to advance in the knowledge of the binding site of CCK1 receptor for CCK, by identifyingamino acid residues that interact with two crucial residues ofthe CCK, namely Met and Phe for which no receptor partner wasyet identified. For this purpose, approaches of molecular modelingand experimental site-directed mutagenesis of the CCK1R werecombined.

For modeling experiments, a structural model of the CCK1R·CCK complex was generated in which amino acid residues of the bindingsite for CCK were shown previously to be involved by pharmacologicaland functional analysis of CCK1R mutants using several peptidicand non-peptidic ligands (14-17). In this structural model, theC-terminal portion of CCK was strongly constrained in the receptorgrove because of interactions between Arg-336 and the carboxylateof the penultimate Asp residue of CCK, and between Asn-333 andthe C-terminal CCK amide. These interactions restrict considerablypossible movements of the C-terminal part of CCK within the bottomof the receptor grove. In fact, after dynamic docking, two closelylinked hydrophobic clusters appeared as likely candidates forinteractions with the Nle/Met 7 and Phe side chains of the ligand,which are so critical for binding affinity and biological potencyof theneuropeptide.

This CCK1R·CCK structural model was well supported by a large set of experimental data and their physicochemical interpretation.The observation that mutation of residues such as Leu-50, Ile-51,Leu-53, and Val-125 affect only slightly recognition of CCK bythe receptor is in full agreement with their expected low contributionto the stability of CCK1R·CCK complex. The moderate decrease inaffinity and potency (10- and 3-fold) caused by mutation of Phe-330was consistent with a T-shaped interaction between the aromaticrings of CCK Phe-9 and receptor Phe-330. The positioning of theC terminus of CCK was furthermore in agreement with the dramaticeffect of the Ile-329 $right-arrow$ Phe mutation on CCK-induced CCK1R activation,which likely results from a reduced ability of the mutant to bindCCK. Indeed, in the three-dimensional model of (I329F)-CCK1R·CCKcomplex, exchange of Ile-329 for a Phe residue causes rotationof the amide of CCK away from Asn-333, its partner in (WT)-CCK1R.Consequently, the interaction between the CCK amide and the carboxamideof Asn-333 is lost (data not shown). The similar properties of(I329F)-CCK1R and the previously characterized (N333A)-CCK1R supportthis explanation (17). Indeed, the (N333A)-CCK1R mutant mediatesCCK-induced inositol phosphate production with a 1350-fold lowerpotency than (WT)-CCK1R and with an efficacy 60% of that of (WT)-CCK1R(17). Two sets of experimental data obtained with the receptormutated at residues Ile-352 and Met-121 further validate the locationof the C-terminal portion of CCK. Exchange of Ile-352 for an Alacaused a 232-fold shift in the potency of CCK1R to induce inositolphosphates, a result that was likely the result of an importantdecrease in the binding affinity of (I352A)-CCK1R for CCK. Thisresult agrees with observations from the three-dimensional receptormodel, which suggest that, in the empty receptor, Ile-352 of TM7interacts with Ile-329 of TM6 and that, upon docking of CCK, theNle/Met-7 side chains disrupt the interaction between these tworesidues.

To confirm the existence of the hydrophobic cluster surrounding Nle/Met of CCK, we predicted that mutation of Met-121 to Valwill decrease binding affinity of the CCK1R for CCK because ofpresence of bulky isopropyl side chain of Val residue, whereasmutation of Met-121 to Ala will not significantly affect binding.Experimental data confirmed the modeling predictions because mutants(M121V)- and (M121A)-CCK1R bound CCK with affinities that were16- and 1.8-fold lower than that of the (WT)-CCK1R, respectively.Proximity between Met-121 and Met/Nle of CCK was further documentedby the set of data showing that Met-7 of CCK and Met-121 of theCCK1R were interchangeable to yield an active CCK1R·CCK complex(seebelow).

The present study also provided important new data concerning the comparison between the binding site for the non-peptideagonist SR-146,131 and the binding site for CCK. Both the experimentaldata obtained with this compound and the CCK1R mutants and itsdynamic docking to the three-dimensional receptor model agreewith a positioning of the non-peptide agonist into the part ofthe CCK1R binding site that interacts with the C-terminal tripeptideof CCK, Met-Asp-Phe-NH₂. Residues from transmembrane segmentsVI (Arg-336, Asn-333, Phe-330, Ile-329) and VII (Ile-352, Leu-356)clearly appear to be involved in recognition of SR-146,131. Ourfindings are consistent with a recent report showing involvementof several of these residues, namely Asn-333, Arg-336, Ile-329,and Leu-356 in CCK1R binding site for SR-146,131, albeit the proposedmodel for the CCK1R.SR-146,131 complex differs slightly from ours(29, 30). However, in the two models, the location of SR-146,131in respect to Met-121, Leu-356, and Cys-94 is very similar. Additionalevidence for a similar location of CCK and SR-146,131 relativeto the Met-121 residue is derived from the capability of the non-peptideagonist to stimulate coupling of (M121V)-CCCK1R to phospholipase-Cas does (Met-7)-CCK. The fact that the CCK1R binding site forSR-146,131 is overlapping part of the binding site for the biologicallyessential region of CCK strongly validates docking of the C terminusof CCK into a cavity formed by the transmembrane helices V, VI,and VII. This docking mode of the C terminus of CCK into CCK1Ris further supported by an NMR study of the interactions betweenCCK and a fragment of CCK1R comprising the top portion of helixVI and the third extracellular loop (31). On the other hand,it differs from that derived from photoaffinity labeling studies(18, 32, 33). In the photoaffinity labeling experimentswith a CCK photoprobe in which the C-terminal Phe residue wasreplaced by benzophenylalanine, Trp-39 at the top of helix I wasidentified, supporting the hypothesis that the C terminus of CCKwas in close proximity of the first helix (32). Based on thesefindings, a model was proposed of the peptide-occupied CCK1R inwhich CCK resembles an hairpin lying at the receptor extracellularsurface with the C-terminal Phe of CCK being in contact with Trp-39of the receptor (18). It is very likely that the large amountof energy required to generate the covalent bond from a p-nitrophenylalanine(or benzophenone) (30 min of UV irradiation at a wavelength of300 nm) significantly affected the conformation of both the CCK1Rand CCK, leading to movement of CCK within its binding site. Onthe other hand, by definition, photoaffinity labeling using structurallymodified CCK could not identify amino acids of the receptor ininteraction with native CCK.

Finally, with the current study, we succeeded in providing the first data related to the process of CCK1R activation followingagonist binding. Indeed, we found that an exchange of Met-121for a Val residue leads to a CCK1R mutant that is unable to induceinositol phosphate accumulation upon (Nle-7)-CCK stimulation.With this mutant, 30% of biological activity is recovered uponstimulation by (Met-7)- and (Gln-7)-CCK and 84% upon stimulationby SR-146,131. From a general point of view, results with mutantsat position 121 show that ascribing a functional role to a residuemust take into account the fact that impact of mutations on pharmacologicaland functional properties of a receptor can depend on the natureof the amino acid by which a critical residue is substituted aswell as on the ligand used to analyze the mutants. Direct involvementof the sulfur atom of Met-7 of CCK or Met-121 of CCK1R in themechanism of receptor activation can be ruled out by results demonstratingthat the Gln side chain can mimic the Met side chain. However,the presence of a polar atom within the hydrophobic cluster surroundingthe Met-121/Met-7 residues seems to be required for CCK1R activation.Indeed, in terms of production of inositol phosphates, the relativeefficacies of the mutated complexes were (M121V)-CCK1R·(Nle-7)-CCK= 0, < (M121V)-CCK1R·(Met-7)-CCK < (M121A)-CCK1R·(Nle-7)-CCK <(M121A)-CCK1R·(Met-7)-CCK. The more the side chain of residuesin the vicinity of position 121 is hydrophobic, the less efficientis phospholipase C activation. In agreement with this view, efficacyof mutant M121A represents ~50% of that of (WT)-CCK1R, a valuein accordance with moderate "hydrophobic weight" of the methylof Ala relative to isopropyl of Val. The much higher efficacyof SR-146,131 compared with (Met-7)-CCK in stimulating functionalcoupling of (M121V)-CCK1R to phospholipase C can tentatively beascribed to the presence of two polar elements, i.e. a sulfuratom and a carbonyl moiety in the vicinity of position 121 ofthe receptor. Another major support for the peculiar role of theresidues in position 121 of the receptor and 7 of the ligand wasderived from molecular dynamic modeling of the different complexes,which show the importance of the amino acid side chains in thesepositions for the correct positioning of the C-terminal part ofCCK, particularly toward Phe-330 of the CCK1R. An interactionbetween the aromatic ring of CCK Phe-9 and that of Phe-330 (T-shape)seems to be important for CCK1R full activation. This view isin line with the 60% decrease in efficacy to stimulate inositolphosphate production caused by an exchange of Phe-9 with Ala inCCK (Fig. 2). Furthermore, stimulation of inositol phosphate productionwas strongly affected by mutation of residue Phe-330, as it wasaffected by mutations of Cys-94 and Phe-218. In addition to theirrole in CCK-induced production of inositol phosphates, bindingresults also argue in favor of a role of the residues Met-121,Cys-94, Phe-218, and Phe-330 in the conformational stability ofCCK1R. Indeed, the data showed that exchange of Met-121 for aVal or an Ala converted the whole CCK1R population into a single,relatively high, affinity state as did mutation of residues Cys-94,Phe-218, and Phe-330. All these data can be interpreted by consideringthe prevailing model for G protein-coupled receptor activation,which is the allosteric ternary complex formed between the receptorR, the agonist L, and G protein(s). According to this model, inabsence of any agonist stimulation, R is believed to undergo spontaneousconformational changes, however, with the inactive conformationbeing energetically the most stable. Binding of an agonist wouldeither induce or stabilize active receptor species (R*), or both(34-36). Accordingly, Met-121, Phe-330, Cys-94, and Phe-218 wouldrepresent key residues allowing the receptor either to be stabilizedin an inactive conformation in absence of ligand and to undergoproper conformational changes for G protein(s) coupling and phospholipaseC activation in presence of theagonist.

Further investigations are obviously required to determine precisely how certain residues such as those pointed out in thisstudy regulate affinity state and/or activation of the CCK1R.In light of recent data with rhodopsin and $beta$ ₂-adrenergic receptor,we hypothesize that these residues play a pivotal role for helixmovements upon CCK binding thereby enabling G protein(s) to efficientlycouple with previously buried region of that receptor (37, 38).Several conserved regions at the bottom of helix III (such as(D/E)-R-Y motif), helix VII (such as N-P-X-X-Y), and helix VInear the third intracellular loop boundary have been shown tobe directly involved in activation process of G protein-coupledreceptors (39-42).

To summarize, the current study has provided much information regarding positioning of the C-terminal part of CCK, which triggersthe biological activity of the peptide, in the CCK1R. SR-146,131,a non-peptide agonist, was found to occupy this critical regionof CCK1R binding site. Data showing the importance of severalamino acid residues involved in this region of CCK1R binding sitewill be used to investigate CCK1Rfunctioning.

FOOTNOTES

^* This work was supported by Association pour la Recherché sur le Cancer Grant 5481.The costs of publication of this articlewere defrayed in part by the payment of page charges. The articlemust therefore be hereby marked "advertisement" in accordancewith 18 U.S.C. Section 1734 solely to indicate thisfact.

^** To whom correspondence should be addressed: INSERM Unite 531, Centre Hospitalier Universitaire de Rangueil, Bat L3, 31054Toulouse Cedex, France. Tel.: 33-5-61-32-24-04; Fax: 33-5-61-32-24-03;E-mail: fourmyd@toulouse.inserm.fr.

Published, JBC Papers in Press, November 27, 2001, DOI 10.1074/jbc.M108563200

ABBREVIATIONS

The abbreviations used are: CCK, cholecystokinin; CCKnR, cholecystokinin receptor-n; WT, wild-type; BH, Bolton-Hunter; RP, reverse phase; HPLC, high performance liquid chromatography; ESI-MS, electrospray ionization-mass spectrometry; TM, transmembrane; GTP $gamma$ S, guanosine 5'-3-O-(thio)triphosphate.

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TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

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The Biologically Crucial C Terminus of Cholecystokinin and the Non-peptide Agonist SR-146,131 Share a Common Binding Site in the Human CCK1 Receptor EVIDENCE FOR A CRUCIAL ROLE OF MET-121 IN THE ACTIVATION PROCESS*

The Biologically Crucial C Terminus of Cholecystokinin and the Non-peptide Agonist SR-146,131 Share a Common Binding Site in the Human CCK1 Receptor

EVIDENCE FOR A CRUCIAL ROLE OF MET-121 IN THE ACTIVATION PROCESS^*