MEN 11270,鼦 Novel Selective Constrained Peptide Antagonist with High Affinity at the Human B2 Kinin Receptor

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Vol. 289, Issue 3, 1250-1256, June 1999

MEN 11270, A Novel Selective Constrained Peptide Antagonist with High Affinity at the Human B₂ Kinin Receptor

Stefania Meini, Laura Quartara, Anna Rizzi, Riccardo Patacchini, Paola Cucchi, Alessandro Giolitti, Girolamo Calò, Domenico Regoli, Marco Criscuoli and Carlo A. Maggi

Department of Pharmacology, Menarini Ricerche S.p.A., Florence, Italy (S.M., R.P., P.C., M.C., C.A.M); Department of Chemistry, Menarini Ricerche S.p.A., Florence, Italy (L.Q., A.G.); Department of Experimental and Clinical Medicine, Section of Pharmacology, University of Ferrara, Italy (A.R., G.C., D.R.)

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

We investigated the pharmacological profile of MEN 11270, or H-D-Arg-Arg-Pro-Hyp-Gly-Thi-c(Dab-DTic-Oic-Arg)c(7 $gamma$ -10 $alpha$ ), aconformationally constrained derivative of the B₂ kinin receptorantagonist Icatibant. MEN 11270 bound with high-affinity to theB₂ kinin receptor constitutively expressed by WI38 human fibroblasts,inhibiting ³H-bradykinin (BK) with a pK_i value of 10.3 ± 0.08 (n = 5). Therank order of affinity of several peptide and nonpeptide antagonistswas also assessed: Icatibant (pK_i = 10.6) $approx$ MEN 11270 (pK_i = 10.3) $approx$ B9430 (pK_i = 10.0) > B9858 (pKi = 8.0) > FR173657 (pK_i = 7.6)> WIN64338 (pK_i = 7.2) > Lys-[des-Arg⁹,Leu⁸]-BK (pK_i < 6) > [des-Arg⁹,Leu⁸]-BK (pK_i < 5). MEN 11270 showed a low affinity in inhibiting³H-Lys-[des-Arg⁹]-BK binding at the human B₁ kinin receptor constitutively expressedby the same cells (pK_i 6.0 ± 0.33; n = 3). MEN 11270 showed nobinding affinity (pIC₅₀ < 5.5) at 29 different receptors and ionchannels. In the human umbilical vein contraction assay, MEN 11270,shifted the concentration-response curve to BK to the right ina concentration-dependent manner (pA₂ 8.14 ± 0.22, n = 7). TheSchild plot was linear (slope 0.95 ± 0.11), consistent with acompetitive antagonism. In the same bioassay, MEN 11270 (10 µM)did not affect the concentration-response curve to the B₁ agonistLys-[des-Arg⁹]-BK nor the contractile responses elicited by noradrenaline orserotonin. These findings indicate MEN 11270 as an antagonistat the human B₂ kinin receptor, with potency and selectivity comparableto those of the linear peptide antagonist, supporting the hypothesisthat a constrained C-terminal $beta$ -turn conformation preserves ahigh affinity for the interaction of Icatibant with the B₂ kininreceptor.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

The nonapeptide bradykinin (H-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg-OH; BK) and related kinins, such as kallidin (Lys-BK), areproduced by the catalytic action of kallikrein enzymes on plasmaand tissue precursors termed kininogens (Bhoola et al., 1992).Kinins are potent autacoid peptides involved in various processesof physiological and pathological relevance, such as smooth musclecontraction, vasodilation, increased vascular permeability, recruitmentof inflammatory cells, induction of pain and cell division (Hall,1992).

Kinins produce their effects in mammals by stimulating two distinct receptor types, termed B₁ and B₂ receptors (Regoli andBarabé, 1980), both of which have been cloned (Eggerickx et al.,1992, Hess et al., 1992, Menke et al., 1994). The B₁ kinin receptorhas a low level of expression in normal tissues but undergoesa marked up-regulation (de novo synthesis) during tissue trauma/inflammation(Marceau, 1995). On the other hand, the B₂ kinin receptor is constitutivelyexpressed by a variety of cell types, (Regoli and Barabé, 1980)and is ready to transduce the signals delivered by newly formedkinins in plasma andtissues.

Owing to the putative role of kinins in mediating pain and inflammation, there is a remarkable interest in developing potentand selective kinin receptor antagonists. These efforts have beenespecially successful in the case of the B₂ kinin receptor. Afirst generation of B₂ receptor antagonists was obtained throughthe insertion of D-Phe at position 7 of the BK sequence (Vavrekand Stewart, 1985). In the early 1990s, the introduction of nonnaturalamino acids led to the discovery of a very potent linear peptideantagonist Hoe 140 or Icatibant ([D-Arg⁰,Hyp³,Thi⁵,DTic⁷,Oic⁸]-BK) (Hock et al., 1991; Wirth et al., 1991). Because of itspotency, metabolic stability and suitability for in vivo investigations,Icatibant has been an instrumental tool in assessing the pathophysiologicalrole of B₂ kinin receptors in both animals and humans. In particular,clinical studies with Icatibant have proven a role of the endogenouskinins, acting via B₂ receptors in regulating coronary circulation(Groves et al., 1995) and in the pathophysiology of allergic reactions(Austin et al., 1994), rhinitis (Proud et al., 1995), and asthma(Akbary et al., 1996). Potent analogs of Icatibant, such as thelinear peptide antagonist B9430 ([D-Arg⁰,Hyp³,Igl⁵,DIgl⁷,Oic⁸]-BK), have also been developed by other groups (Stewart et al.1996). More recently, nonpeptide B₂ kinin receptor antagonistshave also been discovered, such as WIN64338 ({[4-[[2[[bis(cyclohexylamino) methylene]amino]-3-(2-naphthalenyl)-1-oxopropyl]amino]phenyl]methyl]tributyl phosphonium chlorideHCl} (Salvino et al., 1993, Sawutz et al., 1994) and, more recently,FR173657 [(E)-3-(6-acetamido-3-pyridyl)-N-[N-[2,4-dichloro-3-[(2-methyl-8-quinolinyl)oxymethyl]phenyl]-N-methylaminocarbonylmethyl]acrylamide](Aramori et al., 1997; Asano et al., 1997) and LF 16.0335 (1-[[3-[2,4-dimethylquinolin-8-yl)oxymethyl]-2,4-dichloro-phenyl]sulfonyl]-2(S)-[[4-[4-aminoiminomethyl)phenyl-carbonyl]piperazin-1-yl]carbonyl]pyrrolidine)(Pruneau et al., 1998).

Although the discovery of nonpeptide ligands offers some advantages in the development of kinin receptor antagonists suitablefor treatment of human diseases, the unprecedented level of potencyof Icatibant for the human B₂ kinin receptor has not yet beenachieved with nonpeptide ligands. Therefore, a proper structuralknowledge of the bioactive conformation of Icatibant could beof great help in the rational design of novel nonpeptide kininreceptor antagonists. Interestingly, it has been proposed thatthe C-terminal tetrapeptide of Icatibant undergoes a $beta$ -turn arrangementfor the interaction with B₂ kinin receptors (Guba et al., 1994).With the aim of probing this hypothesis, we designed a seriesof Icatibant analogues in which the C-terminal region of the moleculehas been cyclized to constrain it to the $beta$ -turn conformation.In the present study, we describe the pharmacological profileof MEN 11270 or H-D-Arg-Arg-Pro-HypGly-Thi-c(Dab-DTic-Oic-Arg)c(7 $gamma$ -10 $alpha$ ),a cyclized analog of Icatibant, by performing radioligand bindingstudies and comparing its affinity and selectivity at the humanB₂ kinin receptor with that of a number of other ligands (agonistsand antagonists). The antagonist activity of MEN 11270 was assessedin the human umbilical vein, an in vitro preparation which issuitable for functional characterization of B₁ and B₂ kinin receptorantagonists (Gobeil et al., 1996).

	Experimental Procedures

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Materials. ³H-BK (specific activity, 114 Ci·mmol¹) and ³H-Lys-[des-Arg⁹]-BK (specific activity, 92 Ci·mmol¹) were provided by DuPont NEN (Hertfordshire, UK). BK, Lys-[des-Arg⁹]-BK, and Lys-[des-Arg⁹,Leu⁸]-BK were obtained from Peninsula (St. Helens, UK), whereas [Hyp³,Tyr(Me)⁸]-BK and [des-Arg⁹]-BK were obtained from Novabiochem (Läufelfingen, Switzerland).All B₂ receptor antagonists used were synthesized at MenariniRicerche (Florence, Italy). Leupeptin was obtained from BoehringerMannheim (Mannheim, Germany) and DL-2-mercaptomethyl-3-guanidoethylthiopropanoicacid was obtained from Calbiochem (La Jolla, CA). L-glutamine,trypsin plus EDTA, and HEPES were obtained from Gibco Ltd. (Paisley,Scotland). GF/B glass fiber filtermats were provided by Brandel(Semat, Gaithersburg, MD). All other material and culture reagentswere obtained from Sigma (St. Louis,MO).

Cell Culture and Membrane Preparation. WI38 fibroblasts (American Type Culture Collection, Rockville, MD) were used up to passage number 23 and were grown to confluencein minimum essential Eagle's medium with 0.1 mM nonessential aminoacids, 1.0 mM sodium pyruvate, 2 mM L-glutamine, and 10% fetalbovine serum. Cells were cultured in 175-cm² flasks and maintained in a humidified atmosphere at 37°C with5% CO₂. The cells were subcultured every 4 to 6 days at a ratioof 1:2 by using 0.25% trypsin and 1 mM EDTA to detachthem.

For the membrane preparation, WI38 cells were washed out of the medium by PBS without calcium and magnesium, and harvestedby incubating at 37°C with Hanks' balanced salt solution (pH 7.4)containing HEPES (10 mM), 1 mM EDTA, and a cocktail of peptidaseinhibitors: 1,10-phenanthroline (1 mM), HEPES (10 mM), captopril,leupeptin, soybean trypsin inhibitor, DL-2-mercaptomethyl-3-guanidoethylthiopropanoicacid (1 µM each), chymostatin (3.3 µM), phenylmethylsulfonyl fluoride(0.1 mM), and bacitracin (140 µg·ml¹). Cells were then washed in N-tris[hydroxymethyl]methyl-2-aminoethanesulfonicacid (10 mM, pH 7.4, at 4°C) containing the above-described peptidaseinhibitor cocktail and homogenized with a Polytron (PT 3000; KinematicaGmBH, Luzern, Switzerland) set at 10,000 rpm for 30 s. The homogenatewas centrifuged at 18,000 rpm for 20 min. The pellet was washedand homogenization and centrifugation were repeated as described.The pellet was resuspended to obtain a 2-mg·ml¹ membrane protein concentration and frozen immediately into 1-mlaliquots by immersion in liquid nitrogen, and then stored at $-$ 80°Cuntiluse.

The protein concentration was determined by the method of Bradford (1976)

with a Bio-Rad kit (Bio-Rad, Hercules, CA) usingBSA as a reference standard. Immediately before use, the frozenmembrane aliquots were thawed in binding buffer (see below) andmixed to give a homogeneous membranesuspension.

Binding Experiments. The buffer used for binding experiments was N-tris[hydroxymethyl]methyl-2-aminoethanesulfonic acid (10 mM, pH 7.4) containing1,10-phenanthroline (1 mM), bacitracin (140 µg·ml¹), and BSA (1 g·l¹). The binding assay was performed in polypropylene tubes usinga final volume of 0.5 ml. Nonspecific binding was defined as theamount of labeled ligand bound in the presence of 1 µM Lys-[des-Arg⁹]-BK or BK. Membrane concentrations of 60 µg·ml¹ and 30 µg·ml¹ were chosen for binding experiments with ³H-Lys-[des-Arg⁹]-BK and [³H]-BK, respectively. At these protein concentrations, the specificbinding was approximately 75 to 90% of the total binding for ³H-Lys-[des-Arg⁹]-BK and 80 to 90% of the total binding for ³H-BK. Two to 3% of the total added radioactivity was bound tothe membranes for each radioligand. An incubation time of 60 minat 4°C (unless stated otherwise) was used for both radioligandsthroughout the study (saturation and competition studies) (Phagooet al., 1996). With every batch of membranes, a saturation curveto the tritiated agonist was performed to allow for a correctelaboration of competition studies. The chosen radioligand concentrationwas 0.3 nM both for B₁ and B₂radioligands.

All incubations were terminated by rapid filtration through Whatman GF/B glass fiber filtermats that had been presoaked forat least 2 h in 0.6% polyethylenimine using a Brandel 48-cellharvester. The tubes and filters were then washed 4 times with3-ml aliquots of Tris buffer (50 mM, pH 7.4, 4°C). Filters weresoaked in CytoScint scintillation fluid (ICN Biomedicals, Inc.,Costa Mesa, CA) overnight, and bound radioactivity was countedby a beta scintillation counter (2200 CA; Packard Instrument Co.,Inc, Meriden,CT).

The binding affinity of MEN 11270 for a range of 20 different receptors and for Na⁺, Ca²⁺, K⁺, and Cl channels (see Results) was measured according to methods establishedby Cerep (Le Bois L'Evrque BP 1, 86600 Celle l'Evescault,France).

Analysis of Binding Data. Saturation and competition data were processed according to the method of Munson and Rodbard (1980), initially by means ofthe EBDA software and then by LIGAND, to determine the maximumbinding site density (B_max), affinity constant (K_D), equilibriuminhibition constants (K_i) and to test the significance of thebinding site models. All values are given as mean ± S.E.M. forthe stated number of experiments (n). Each experimental determinationwas obtained in duplicate on a different batch of membranepreparation.

Human Isolated Umbilical Vein. Human umbilical cords (n = 13) from healthy women, 22 to 40 years old, were collected after spontaneous delivery at term andplaced in cold (4°C) Krebs' solution. The lapse of time betweenthe delivery and the experiment was on average 4 h (1-10 h). Inthe laboratory, the middle segment of the cord (7-8-cm long) wasplaced in Krebs' solution at room temperature and, within 30 min,the vein was dissected free of surrounding tissue. The endotheliumwas rubbed off using a cotton swab. The tissues were cut intospiral strips (2-cm long, 3-mm wide) and suspended in 10-ml organbaths containing warm (37°C), oxygenated (95% O₂, 5% CO₂) Krebs'solution (118 mM NaCl , 4.7 mM KCl , 2.5 mM CaCl₂ , 0.5 mM MgCl₂,1.2 mM KH₂PO₄, 1.2 mM MgSO₄, 25 mM NaHCO₃, and 10 mM glucose).The human umbilical vein strips were stretched to a resting tensionof 2g. Changes in tension were measured isometrically with GrassFT03 force transducers (Grass Instruments, Quincy, MA) and recordedon a Linseis (model L2005) multichannel chart recorder (LinseisInc., Princeton Jct., NJ). In all experiments, the kininase IIinhibitor captopril was added to the Krebs' solution at a 1 µMconcentration. Before testing any agent, the tissues were allowedto stabilize for 120 to 150 min, resting tension was readjustedevery 15 min. The experiments began with the application of 100mM KCl to measure the responsiveness of the preparations. Theantagonist activity of MEN 11270 was evaluated by measuring thecumulative concentration-response curves to BK or Lys-[des-Arg⁹]-BK in the absence and presence of the antagonist. The antagonistwas applied 15 min before theagonist.

The nature of the interaction of MEN 11270 with the B₂ receptor was studied by performing the Schild analysis (Arunlakshanaand Schild, 1959

), and the apparent affinity of MEN 11270 wasexpressed in terms of pA₂. pEC₅₀ ( $-$ log EC₅₀) values were calculatedby linear regression and 95% CLs were calculated (cf. 95%CLs).

Furthermore, the activity of MEN 11270 was measured toward contractions evoked by single and repeatable administrations ofnoradrenaline or serotonin (both at 1 µM). The control responseand the response in the presence of the antagonist were obtainedfor each agonist in the same strip preparation. The antagonistwas applied 15 min before theagonist.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Binding Studies at the Human Kinin B₂ Receptor. ³H-BK (0.02-5 nM) saturation isotherm was fitted according to a one-site model with a K_D of 123 ± 17 pM (Hill slope, 0.92 ±0.03, n = 7) and a B_max of 485 ± 78 fmol·mg¹ of protein. In competition experiments, the binding of a panelof kinin receptor-selective agonists and antagonists indicatedthat the binding sites labeled by ³H-BK correspond to a classic B₂ kinin receptor (Fig. 2a; Table1). In fact, a high-affinity binding was detected with BK andthe selective B₂ kinin receptor agonist [Hyp³,Tyr(Me)⁸]-BK, whereas only a negligible binding affinity was measuredfor [des-Arg⁹]BK and Lys-[des-Arg⁹]-BK.

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TABLE 1
Competition studies at the B₁ and B₂ kinin receptor in WI38 fibroblasts membranes

With regard to antagonists, MEN 11270 (Fig. 1) showed subnanomolar affinity for the human B₂ kinin receptor natively expressedin WI38 cells (Fig. 2b; Table 1). Its affinity was comparableto that obtained with Icatibant (Fig. 2b; Table 1) and the otherlinear peptide B₂ kinin receptor antagonist B9430 (Fig. 2b; Table1), whereas the nonpeptide antagonists FR 173657 and WIN 64338showed much lower (about 3 order of magnitude) affinity values(Fig. 2b; Table 1).

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Fig. 1. Chemical structure of MEN 11270 [H-D-Arg-Arg-Pro-Hyp-Gly-Thi-c(Dab-DTic-Oic-Arg)c(7 $alpha$ -10 $gamma$ )].

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Fig. 2. Inhibition of ³H-BK binding to WI38 membranes by a range of B₁- and B₂-selective ligands. Specific ³H-BK binding was plotted against increasing concentration of agonists (a): BK ( $open circle$ ), [Hyp³, Tyr(Me)⁸]-BK (

), Lys-[des-Arg⁹]-BK ( $black-triangle$ ), and [des-Arg⁹]-BK ( $black-diamond$ ); antagonists (b): Icatibant ( $black-square$ ), MEN 11270 (

), B9430 ( $black-triangle$ ), B9858 (×), FR173657 ( $down-triangle$ ), and WIN 64338 (*). [³H]-BK (0.3 nM) and WI38 membranes (30 µg·ml¹) were incubated as described in Experimental Procedures in the presence of increasing concentrations of displacer. The data shown represent the mean ± S.E.M. of at least three separate determinations in duplicate.

Competition studies with the B₂ kinin receptor antagonists Icatibant, MEN 11270, and FR 173657 were also carried out at atemperature of 20°C (incubation time, 60 min). Under these conditions,there was no significant difference in the saturation analysisof ³H-BK (data not shown). The affinity of Icatibant or MEN 11270was not influenced by temperature: Icatibant's pK_i was 10.6 ±0.02 (n = 4) and 10.7 ± 0.06 (n = 3) at 4 and 20°C, respectively(Fig. 3a), and the pK_i values of MEN 11270 were 10.3 ± 0.08 (n= 5) and 10.2 ± 0.07 (n = 3) at 4 and 20°C, respectively (Fig.3b). In sharp contrast, raising the temperature of the assay determineda sizable increase (about 10-fold) in the estimated affinity ofthe nonpeptide antagonist FR 173657 (Fig. 3c). In fact, pK_i valuesof 8.6 ± 0.07 (n = 3) and 7.6 ± 0.04 (n = 6) were estimated forthis ligand at 20°C and 4°C, respectively.

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Fig. 3. Icatibant (a), MEN 11270 (b), and FR173657 (c) displacement curves of the ³H-BK binding (0.3 nM) to WI38 membranes performed at 4°C ( $open circle$ ) or 20°C (

]). The data shown represent the mean ± S.E.M. of at least three separate determinations in duplicate.

Binding Studies at the Human Kinin B₁ Receptor. ³H-Lys[des-Arg⁹]-BK (0.03-3 nM) bound to WI38 cell membranes in a specific and saturable manner. The Scatchard transformationof the specific binding was consistent with a one-site bindingmodel. The experiments indicated a K_D value of 175 ± 40 pM (n= 5) with a B_max of 104 ± 8 fmol·mg^¹ of protein and a Hill slope of 1.02 ± 0.05.

Competition studies confirmed the selectivity of ³H-Lys-[des-Arg⁹]-BK in labeling the B₁ kinin receptor (Fig. 4; Table 1). Withregard to the agonists, Lys-[des-Arg⁹]-BK inhibited the ³H-Lys-[des-Arg⁹]-BK binding with the highest affinity, whereas [des-Arg⁹]-BK showed a negligible binding affinity for this site (Table1). The selective B₁ kinin receptor antagonist Lys-[Leu⁸,des-Arg⁹]-BK inhibited the ³H-Lys[des-Arg⁹]-BK binding with a high affinity, whereas MEN 11270 showed alow affinity comparable to that obtained with Icatibant (Fig.4; Table 1).

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Fig. 4. Inhibition of ³H-Lys-[des-Arg⁹]-BK binding to WI38 membranes. Specific ³H-Lys-[des-Arg⁹]-BK binding was plotted against increasing concentrations of Lys-[des-Arg⁹]-BK ( $open circle$ ), Lys-[Leu⁸,des-Arg⁹]-BK (

), Icatibant ( $black-square$ ), MEN 11270 (

), and BK ( $star$ ). ³H-Lys-[des-Arg⁹]-BK (0.3 nM) and WI38 membranes (60 µg·ml¹) were incubated as described in Experimental Procedures in the presence of increasing concentrations of displacer. The data shown represent the mean ± S.E.M. of three separate determinations in duplicate.

Receptor Selectivity and Ion Channel-Binding Affinity. The affinity of MEN 11270 was determined for many receptors and ion channels by using conventional radioligand-binding techniques.MEN 11270 showed no relevant binding affinity (pIC₅₀ < 5.5) atthe angiotensin 1, angiotensin 2, calcitonin gene-related peptide,interleukin-1 $beta$ , tumor necrosis factor $alpha$ , chemokine receptor type1, chemokine receptor type 2, neurokinin 1, neurokinin 2, neurokinin3, neuropeptide Y, thromboxane A₂, prostaglandin I₂, opioid-likereceptor 1, serotonin, muscarinic, neurotensin, somatostatin,bombesin, and vasoactive intestinal peptide receptors. MEN 11270had no measurable binding affinity (pIC₅₀ < 5.5) for Ca²⁺ channels (L-type: dihydropiridine, verapamil, diltiazem sites;N-type), K⁺ channels (ATP-, voltage-, and Ca²⁺-dependent), Na⁺ channel (site 2), or Cl $-$ (picrotoxinin)channel.

Organ Bath Studies. BK (0.001-100 nM) produced concentration-dependent contraction of the human umbilical vein with a pEC₅₀ value of 8.3 (cf.95% CLs, 8.0-8.5; n = 7). The administration of MEN 11270 (10-100-1000nM, contact time 15 min) did not produce any motor effect perse but, in the presence of MEN 11270, a concentration-dependentrightward shift of the curve to the agonist was observed, withoutdepression of E_max (Fig. 5a). The Schild plot was compatible withcompetitive antagonism with an extrapolated pA₂ value of 8.14± 0.22 (n = 7) with the slope being not significantly differentfrom unity (0.95 ± 0.11; Fig. 5b).

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Fig. 5. a, concentration-response curves to BK in the human umbilical vein in the absence and presence of various concentrations of MEN 11270: BK ( $open circle$ ), 10 nM MEN 11270 (

), 100 nM MEN 11270 ( $black-square$ ), and 1000 nM MEN 11270 ( $black-triangle$ ). Contact time of the antagonist was 15 min. b, Schild plot of MEN 11270 against BK. Abscissa, log of the molar concentration of the antagonist. Ordinate, log of the concentration ratio $-$ 1 (CR $-$ 1) of the agonist. Values represent the mean ± S.E.M. of seven experiments.

MEN 11270 (10 µM, contact time 15 min) had no effect on the concentration-response curve to the B₁ kinin receptor agonistLys-[des-Arg⁹]-BK (0.001-100 nM). The pEC₅₀ value of Lys-[des-Arg⁹]-BK averaged 8.5 (95% CLs, 8.4-8.6; n = 5) and 8.5 (cf. 95% CLs,8.3-8.7; n = 5) in the absence and presence of MEN 11270, respectively(Fig. 6).

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Fig. 6. Concentration-response curves to Lys-[des-Arg⁹]-BK in the human umbilical vein in the absence ( $open circle$ ) and presence (

) of 10 µM MEN 11270. Contact time of the antagonist was 15 min. Values represent the mean ± S.E.M. of five experiments.

Moreover, the contractions of the human isolated umbilical vein produced by noradrenaline (1 µM; 2.18 ± 0.49 and 2.20 ± 0.49g in the absence and presence of MEN 11270, respectively; n =4) or serotonin (1 µM; 4.43 ± 0.48 and 4.64 ± 0.54 g in the absenceand presence of MEN 11270, respectively; n = 4 each) were notmodified by MEN11270.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

The linear decapeptide Icatibant, a potent and selective antagonist at the B₂ kinin receptor, has been previously studiedby combining NMR spectroscopy and molecular dynamic simulationsto define its conformational behavior into a hydrophilic/hydrophobicenvironment (Guba et al., 1994). The results of this analysishad suggested the presence of a $beta$ II'-turn motif in the C-terminalpart of the sequence involving the Ser-DTic-Oic-Arg segment (Gubaet al., 1994). This conformational feature was defined as beingcritical for the high-affinity interaction of Icatibant with thereceptor (Guba et al., 1994; Kyle, 1995). In our previous studiesin the field of tachykinins, we successfully used a 14-memberedcyclic lactam to constrain a $beta$ -turn conformation in a hexapeptidesequence (Pavone et al., 1995). To apply a similar strategy toIcatibant, we designed a constrained analog in which the Ser-DTic-Oic-Argsegment was fixed in its turn conformation throughout the formationof an intramolecular lactam bridge. To obtain the 14-memberedring, we substituted the serine residue with a diaminobutiric(Dab) residue, since the serine side chain of Icatibant is notcritical for high affinity at the human B₂ kinin receptor (L.Quartara, R. Ricci, S. Meini, R. Patacchini, A. Giolitti, S. Amadesi,C. Rizzi, A. Rizzi, K. Varani, P. A. Borea, C. A. Maggi, and D.Regoli, in preparation). Cyclization was performed between thecarboxyl group of the C-terminal arginine residue and the sidechain of the Dab residue. The resulting compound, MEN 11270 [H-D-Arg-Arg-Pro-Hyp-Gly-Thi-c(Dab-DTic-Oic-Arg)c(7 $alpha$ -10 $gamma$ ),Fig. 1], is a potent and selective antagonist at the human B₂kininreceptor.

WI38 human fetal lung fibroblasts constitutively express both B₁ and B₂ kinin receptors (Phillips et al., 1992; Webb et al.,1994; Phagoo et al., 1996) and are representative of several ofthe effects produced by BK, which acts almost exclusively at theB₂ kinin receptor type. It has been reported that activation ofthe B₂ receptor in these cells leads to a tyrosine kinase activity,which is involved in prostaglandin production (Jong et al., 1993)and induces interleukin-1 $beta$ expression (Pan et al., 1996).

We used membranes of WI38 cells to probe the affinity and selectivity of MEN 11270 at both the kinin receptor types, comparedto that of other peptide and nonpeptideligands.

With few exceptions, the affinity values obtained in our binding experiments with several peptide and nonpeptide antagonistsare comparable to the values reported in otherstudies.

Phagoo et al. (1996) reported a K_i of 0.021 nM for Icatibant, corresponding to a pK_i of 10.6 in competing the ³H-BK binding. In a different fibroblast cell line (CCD-16), Icatibantinhibited the binding of the radioligand B₂ receptor antagonist³H-NPC17731 with a comparable affinity (K_i of 0.05 nM, pK_i 10.3)(Zhang and Codd, 1998).

Cortech researchers have described two antagonists, B9430 and B9858, the first one possessing mixed activity at both the B₁and B₂ receptors and the second one selective for the B₁ receptor(Burkard et al., 1996; Stewart et al., 1996). These authors obtaineda pIC₅₀ of 9.6 and 7.9 for B9430 and B9858, respectively, in inhibitingthe ³H-BK binding to cells transfected with the human B₂ receptor,and apparent pA₂ values of 8.6 for B9430 and <5 for B9858 in thehuman ileum assay. Our data confirm the affinity data presentedpreviously by these authors. It was previously reported that Icatibanthad a pA₂ amounting to 8.36 in the same bioassay (Zuzack et al.,1996), comparable to the pA₂ value obtained in the human umbilicalvein by Gobeil et al. (1996).

FR 173657 has been reported to inhibit with high affinity (IC₅₀, 2.9 and 8.9 nM, respectively) the binding of ³H-BK to membranes of IMR90 fibroblasts and Chinese hamster ovarycells transfected with cDNA coding for the human B₂ kinin receptor,respectively (Aramori et al., 1997; Asano et al., 1997). In theinitial set of experiments, performed at 4°C, the estimated affinityof FR 173657 for the B₂ kinin receptor in WI38 cells was surprisinglylow (pK_i 7.6) as compared to the values reported by Aramori etal. (1997) or by Asano et al. (1997). However, these authors didnot specify at which temperature they performed the assay. Wetherefore repeated the experiments at 20°C and, quite surprisingly,observed that the binding affinity of FR 173657 for the B₂ kininreceptor was increased by about 1 log unit when the incubationtemperature was raised to 20°C. Our results are comparable tothose obtained by Gessi et al. (1997) who, working at room temperatureand after an incubation time of 60 min, reported a pK_i of 8.7for FR173657 in inhibiting the ³H-BK binding in the human umbilical veinmembranes.

It is intriguing to note that the estimate of the affinities of the two peptide antagonists, MEN 11270 and Icatibant, wasunaffected by the increase in the binding temperature. This observationsuggests a different type of interaction with the human B₂ kininreceptor by peptide and nonpeptide ligands. However, the increasein affinity for FR173657, following an increase in the temperatureof binding conditions, is unique of this molecule; in fact, theaffinity of the other nonpeptide antagonist WIN64338, which alsohas quite a low affinity at the human B₂ kinin receptor, did notchange if measured at 4 and 20°C (data not shown). The fact thatFR 173657 better inhibits BK from its binding site at a highertemperature could indicate the importance of thermodynamic factorswhich enable this nonpeptide ligand to achieve the proper bioactiveconformation for its interaction with the B₂ kinin receptor. Onthe other hand, it is also known (Testa et al., 1987) that a ligandbinding in which nonpolar or lipophilic groups lose their contactwith water molecules to form new hydrophobic interactions arefavored by an increase in temperature. In this case, an entropy-drivenincrease in the binding of FR 173657, which, contrary to WIN 64338,is a lipophilic molecule with no charged groups, may be facilitatedat higher temperatures. We cannot rule out the possibility that,at low temperature, FR 173657 selects a G protein-uncoupled conformerof the B₂ receptor which is different from that selected by FR173657 at higher temperature. Experiments with a radiolabeledform of this nonpeptide antagonist are needed to answer thesequestions.

It is interesting to note that, in the human isolated umbilical vein, both peptide and nonpeptide antagonists possess a comparablecompetitive antagonist activity: Icatibant was previously reportedto have an apparent pA₂ of 8.42 (Gobeil et al., 1996), FR173657a pA₂ of 8.22 (Rizzi et al., 1997), and MEN 11270 has a pA₂ of8.14 (this study). Notably, the apparent pA₂ value of FR173657in human umbilical vein assay is in good keeping with the pK_ivalue estimated for this ligand in binding at WI38 cell membranes,whereas the pK_i values of Icatibant and MEN 11270 are at leastone order of magnitude higher than their apparent pA₂ values.The reasons for this discrepancy, which selectively affects thepeptide antagonists, are not clear at present, although the existenceof a binding paradox (higher binding affinities of kinin receptorantagonists versus their apparent affinity in functional assay)has been repeatedly reported in the literature (Hall, 1992; Ransomet al., 1992; Burkard et al., 1996; Gobeil et al., 1996; Gessiet al., 1997; Rizzi et al., 1997). Notably the binding paradox(as defined above) reported to occur in some systems for bradykininhas been shown to depend at least in part from the ionic strengthof the medium used for binding experiments (Ransom et al., 1992).Whether a similar factor could be involved in the quantitativediscrepancies between K_i and pA₂ values reported in the presentstudy remains to beestablished.

A low but sizable affinity of Icatibant at the human B₁ kinin receptor has already been observed (Menke et al., 1994; Burkardet al., 1996; Phagoo et al., 1996; Bastian et al., 1997). Thefact that MEN 11270 maintains a comparable affinity to the B₁kinin receptor indicates that the postulated C-terminal $beta$ -turnarrangement of Icatibant is also compatible with an interactionof these ligands at the B₁receptor.

Our results confirm a very low affinity of the BK derivative lacking of the C-terminal arginine as compared to the Lys-[des-Arg⁹]-BK, as already reported at both the native or cloned human B₁kinin receptor (Menke et al., 1994; Austin et al., 1997; Bastianet al., 1998).

In conclusion, in the present study we have shown that the pharmacological profile of MEN 11270 is comparable to that of Icatibant,supporting the idea that a constriction of the C-terminal sequencein a $beta$ -turn arrangement is able to preserve a high-affinity forinteraction with the human B₂ kininreceptor.

The discovery of a constrained peptide molecule, such as MEN 11270, acting as a high-affinity antagonist at the B₂ kinin receptoris a helpful starting-step for designing new low-molecular weightmolecules.

	Acknowledgments

We thank Sharon Blumenstock for her friendly and kind help in revising themanuscript.

	Footnotes

Accepted for publication February 13, 1999.

Received for publication November 13, 1998.

Send reprint requests to: Stefania Meini, Pharmacology Department, Menarini Ricerche S.p.A., via Rismondo 12A, 50131, Florence, Italy.

	Abbreviations

BK, bradykinin; B9430, D-Arg-Arg-Pro-Hyp-Gly-Igl-Ser-DIgl-Oic-Arg-OH; diaminobutiric, Dab; Icatibant, H-D-Arg-Arg-Pro-Hyp-Gly-Thi-Ser-DTic-Oic-Arg-OH; MEN 11270, H-DArg-Arg-Pro-Hyp-Gly-Thi-c(Dab-DTic-Oic-Arg)c(7 $gamma$ -10 $alpha$ ).

	References

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