Characterization of I2 Imidazoline and sigma  Binding Sites in the Rat and Human Stomach

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Vol. 285, Issue 1, 170-177, April 1998

Characterization of I₂ Imidazoline and $sigma$ Binding Sites in the Rat and Human Stomach

Gerhard J. Molderings, Kurt Donecker, Maria Burian, W. Alexander Simon, Detlev W. Schröder and Manfred Göthert

Institute of Pharmacology and Toxicology (G.J.M., K.D., M.B., M.G.), University of Bonn, Bonn, Germany, Byk Gulden Lomberg GmbH (W.A.S.), Konstanz, Germany and Evangelisches Krankenhaus (D.W.S.), Bonn, Germany

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Radioligand binding experiments were carried out to identify and characterize nonadrenoceptor [³H]idazoxan binding sites and [³H](1,2-di-(2-tolyl)guanidine) binding sites in the rat and humanstomach. Furthermore, we examined two selected aspects of theirpotential functional significance. Binding of [³H]idazoxan (K_d = 11.1 nM and 12.4 nM, respectively) and [³H]DTG (K_d = 932 nM and 242 nM, respectively) to cell membranesfrom rat and human stomach was rapid, reversible, specific andsaturable. In rat stomach, binding of the radioligands was inhibitedby imidazolines and by nonimidazoline $sigma$ -site ligands, respectively,at different rank orders of affinity, which suggests the existenceof I₂-imidazoline binding sites as well as $sigma$ ₂-sites. In two functionalmodels, the direct effects of I₂-site ligands and $sigma$ ₂-site ligandson gastric smooth muscle and glands were investigated. (1) Cirazoline,clonidine and 4-chloro-2-(2-imidazolin-2-ylamino)-isoindoline(BDF 6143) failed to contract the longitudinal muscle of the ratstomach fundus; BDF 6143 also failed to induce relaxation of thispreparation when it was precontracted with 30 mM KCl. (2) Clonidine,idazoxan, BDF 6143, 1,2-di-(2-tolyl)guanidine, agmatine and (R)-3-(3-hydroxyphenyl)-N-propylpiperidineup to 100 µM did not induce acid secretion from rabbit isolatedgastric glands. Our data provide evidence that the rat stomachis endowed with $sigma$ ₂ sites and I₂ binding sites in addition to thepreviously identified non-I₁/non-I₂ [³H]clonidine binding sites. Our experiments also offer basic evidenceof the existence of I₂ and $sigma$ binding sites in the human stomach.Neither the I₂ and [³H]clonidine binding sites nor the $sigma$ sites in rat stomach are directlyrelated to a postsynaptic effect on gastric smooth muscle or toacid release from isolated gastric glands.

	Introduction

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Nonadrenoceptor IBS are recognized with high to moderate affinity by imidazolines and related compounds, but not by catecholamines.At least two classes of IBS exist, I₁-IBS and I₂-IBS, which canbe labeled by [³H]clonidine and [³H]idazoxan, respectively (for review, see Regunathan and Reis,1996; Molderings, 1997). Binding experiments with [³H]clonidine and [³H]idazoxan in membranes from guinea pig (Houi et al., 1987), rabbit(Tesson et al., 1992) and rat gastric tissue (Molderings et al.,1995) provided basic evidence that IBS are also present in thestomach. Interestingly, it has been shown that in the rat stomach, $sigma$ -receptor ligands exhibited a remarkably high affinity for nonadrenoceptor[³H]clonidine binding sites (Molderings et al., 1995). Moreover, $sigma$ -like sites were recently identified in the porcine gastric mucosa(Harada et al., 1994), but not in rat and human gastric tissue.

On the basis of these findings, the first aim of the present study was to identify and characterize [³H]idazoxan and [³H]DTG binding sites in the rat and human stomach and to investigatewhether a relationship exists between nonadrenoceptor [³H]clonidine and [³H]idazoxan binding sites on the one hand and $sigma$ binding sites onthe other. Therefore, we determined and compared the affinityof key ligands for IBS and $sigma$ sites in rat stomach membranes labeledwith [³H]clonidine, [³H]idazoxan or [³H]DTG (a radioligand for $sigma$ sites; Weber et al., 1986).

In previous in vivo studies, imidazolines such as clonidine exerted a dual action on gastric acid secretion; at low concentrations,these compounds reduced acid secretion (Del Tacca et al., 1982;Bhandare et al., 1991; Blandizzi et al., 1995; Carlisle et al.,1995; Glavin and Smyth, 1995). This inhibitory effect on acidsecretion was prevented by alpha-2 adrenoceptor antagonists (DelTacca et al., 1982; Bhandare et al., 1991; Blandizzi et al., 1995),which suggests that it is mediated mainly by activating presynapticalpha-2 adrenoceptors on cholinergic nerves innervating the stomach.Additionally, evidence has been presented that peripheral I₁-imidazolinereceptors might also contribute to the antisecretory and antiulcereffects of imidazoline derivatives (Carlisle et al., 1995; Glavinand Smyth, 1995). At higher concentrations, several imidazolinesand agmatine stimulated acid secretion in vitro and in vivo (Medgettand McCulloch, 1979; Del Tacca et al., 1982; Houi et al., 1987;Bhandare et al., 1991; Glavin et al., 1995). The stimulatory effectwas not due to activation of alpha-2 adrenoceptors, because itwas not mimicked by the alpha-2 adrenoceptor agonist $alpha$ -methylnoradrenalineand it was not counteracted by yohimbine (Houi et al., 1987).Some have speculated that the stimulatory effect of the imidazolinesmay be due to activation of imidazoline receptors in stomach tissue(Houi et al., 1987; Bhandare et al., 1991; Glavin et al., 1995).Therefore, the second aim of this study was to investigate whetherligands with high affinity for IBS and/or $sigma$ sites could induceacid secretion from isolated rabbit gastric glands, which is thestandard preparation for investigating acid secretion in vitro.

Finally, it was demonstrated that CDS, a putative endogenous ligand at IBS (Regunathan and Reis, 1996) induced a contractionof gastric smooth muscle via an unknown mechanism of action (Felsenet al., 1987). It has been proposed that imidazoline receptorson gastric smooth muscle may be involved. Hence the third aimof the present study was to examine whether other ligands at imidazolinebinding sites mimic the effect of CDS and, if so, whether bindingof drugs at [³H]clonidine, [³H]idazoxan and [³H]DTG binding sites directly contract rat stomach smooth musclecells in a vagal nerve-independent manner. Parts of this studyhave been presented at scientific meetings.

	Materials and Methods

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Membrane preparation. Fresh stomachs were obtained from Wistar Kyoto rats immediately after killing. Segments of macroscopically normal human stomachwere obtained from male or female patients undergoing gastricsurgery. The study was approved in all respects by the local ethicscommittee. All steps of the preparation procedure were performedon ice. The rat glandular stomach and the segments of the mucosallayer from human stomach were prepared and cut into small fragmentsthat were placed in 40 ml of buffer solution containing sucrose270 mM, ascorbic acid 0.6 mM and Tris-sulfate 10 mM (pH 7.4),minced by means of an Ultraturax (five times for 20 s each) andhomogenized using a glass-Teflon homogenizer (three times for30 s each). The homogenates were centrifuged (5 min, 1200 × g,4°C). The supernatant was filtered through four layers of gauze,diluted to 420 ml with HEPES buffer (HEPES-Na⁺ 5 mM, EGTA 0.1 mM, PMSF 0.3 mM, pH 7.4; buffer I) and recentrifuged(20 min, 40,000 × g, 4°C). The pellet was washed twice and thenresuspended in buffer I, homogenized, diluted to give a proteinconcentration of about 2 mg/ml and stored at $-$ 80°C until use.Before use, the membranes were centrifuged (20 min, 40,000 × g,4°C), resuspended in the incubation buffer (HEPES-Na⁺ 5 mM, EGTA 0.5 mM, MgCl₂ 0.5 mM, ascorbic acid 0.1 mM, pH 7.4;buffer II), homogenized by ultrasonics and diluted to a finalprotein concentration of about 0.6 mg/ml.

Binding assay. A 400-µl aliquot of membranes was incubated for 55 min with [³H]idazoxan or [³H]DTG (25 µl) at 4°C in a final volume of 0.5 ml. The reactionwas stopped by rapid vacuum filtration with a Brandel cell harvesterthrough Whatman GF/C glass-fiber filters presoaked with polyethylenimine0.5 M and clonidine 0.1 mM (to reduce filter binding), followedby rapid washing (within about 5 s) of the incubation tubes andfilters with 10 ml ice-cold buffer II. Filters were placed in6 ml of scintillation fluid and shaken overnight, and the radioactivitywas determined by liquid scintillation counting at 44% efficiency.Nonspecific binding was defined as radioligand binding in thepresence of BDF 6143 100 µM ([³H]idazoxan binding) or in the presence of (+)-3-PPP 100 µM ([³H]DTG binding), and it accounted for 5% and 21% of the total radioactivityretained in the filters when [³H]idazoxan and [³H]DTG 10 nM were used in the competition experiments, respectively.Adrenaline 10 µM, which has no affinity for imidazoline bindingsites (Molderings et al., 1993, 1994) was added to the assay toprevent the radioligands from binding to alpha-2 adrenoceptors.

In rat stomach, saturation studies with [³H]idazoxan were performed with radioligand concentrations ranging from 0.1 to 46nM to determine receptor number and affinity. Because it has beenshown that the affinity of [³H]DTG for peripheral $sigma$ sites is in the high nanomolar range i.e.,a concentration of the radioligand at which it cannot be usedbecause the cost is too high), equilibrium-saturation bindingof [³H]DTG was performed by incubating the membranes with 10 nM [³H]DTG and increasing the concentrations of unlabeled DTG for 55min at 4°C in both rat and human stomach. A similar experimentalprotocol has been used to determine the affinity and the densityof [³H]idazoxan binding sites in human stomach. This competitive protocolnot only has the advantage over saturation protocols that lessradioligand is consumed, but the contribution of nonspecific bindingis also minimized because the radioligand is used at a low concentration(DeBlasi et al., 1989

). Competition studies were done using 10nM [³H]idazoxan or [³H]DTG, respectively, and 13 different concentrations, rangingfrom 0.1 nM to 100 µM, of the unlabeled ligand under investigation.All experiments were carried out in triplicate.

Determination of gastric acid release. Gastric glands were prepared from anesthetized New Zealand rabbits by high-pressure perfusion of the stomach followed by collagenasedigestion of pieces of fundic mucosa. Gastric glands were suspendedin Krebs-Henseleit solution (NaCl 132.5 mM, KCl 5.4 mM, Na₂HPO₄5 mM, NaH₂PO₄ 5 mM, MgSO₄ 1 mM, CaCl₂ 1.2 mM) containing 2 mg/mlglucose and 0.125 µM [dimethylamine-¹⁴C]aminopyrine; pH 7.4. Glands were incubated at 37°C in the presenceof the drugs at the concentrations indicated. After 30 min, theglands were sedimented by rapid centrifugation, and the aminopyrineaccumulation ratio was determined from the relation of radioactivitybetween the glands and the supernatant (for details, see Simonet al., 1990).

Contraction of gastric smooth muscle. Gastric longitudinal muscle strips (3 × 10 mm) were obtained from Wistar-Kyoto rats. The stomach, opened along the greatercurvature, was stripped free of all mucosal tissue, and longitudinalstrips were cut at right angles to the visible circular musclebundles. In an organ bath, tissue strips were pre-equilibratedfor about 1 h at 37°C in oxygenated physiological salt solutionof the following composition (mM): NaCl 118, KCl 4.7, CaCl₂ 2.5,MgCl₂ 1.2, NaHCO₃ 25, KH₂PO₄ 1.2, glucose 10; pH 7.4. This solutioncontained 1 µM atropine, 1 µM prazosin and 3 µM rauwolscine throughoutthe experiments to mask alpha-adrenoceptors and to eliminate potentialvagal nerve influences. Cumulative concentration-response curveswere determined for the drugs under study. Time-matched controlexperiments were carried out in parallel. Contractions were monitoredisometrically using Statham force transducers under a load of1 g. After the last concentration of the test compound, the preparationwas washed twice, and then KCl was added to the organ bath (finalconcentration 85 mM) to induce maximum contraction of the smoothmuscles. The responses of the test compounds are expressed asthe ratio of the contraction evoked by the test drugs to thatcaused by 85 mM KCl.

Protein assay. Protein concentration was measured by the method of Bradford (1976) using bovine serum albumin as the standard.

Data analysis. Data from the saturation and competition experiments were analyzed using the least-squares fitting program GraphPADinPlot(GraphPad Software Inc., San Diego, CA). The significance of theimprovement of fit obtained by the two-site equation over thefit obtained by the one-site equation was analyzed by the F statistics(partial F test; De Lean et al., 1982). Receptor number and affinityfrom homologous competitive binding experiments were calculatedby formulas (3) and (5) of DeBlasi et al. (1989). Results areexpressed as mean values ± S.E. The statistical significance ofdifferences was analyzed by Student's t test for unpaired data.

Drugs. The following drugs were used in this study: [¹⁴C]Aminopyrine (specific activity 96.6 Ci/mmol), [³H]DTG (specific activity 35.2 Ci/mmol; NEN DuPont, Dreieich, FRG),[³H]idazoxan (specific activity 45 Ci/mmol; Amersham, England),adrenaline base (Hoechst, Frankfurt, FRG), bovine serum albumin,agmatine, naphazoline hydrochloride, haloperidol, (±)pentazocinehydrochloride (Sigma, Munich, FRG), U46619 (Biosigma, Munich,FRG), moxonidine, BDF 6143 hydrochloride (Beiersdorf, Hamburg,FRG); cirazoline hydrochloride (Synthélabo, Paris, France), clonidinehydrochloride (Boehringer, Ingelheim, FRG), (+)-3-PPP hydrochloride,(±)-ifenprodil tartrate, dizocilpine maleate, DTG (RBI, Natick,MA); histamine dihydrochloride (Merck, Darmstadt, FRG), (±)idazoxanhydrochloride (Reckitt and Colman, Hull, UK), rauwolscine hydrochloride(Roth, Karlsruhe, FRG) and ranitidine hydrochloride (Glaxo, Greeford,UK). Drugs were dissolved in the respective buffer with the followingexceptions. Stock solutions of adrenaline and haloperidol wereprepared in HCl 0.01 M, and DTG was dissolved in methanol; theywere then further diluted in the respective buffer. The vehiclesdid not change radioligand binding.

	Results

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[³H]idazoxan binding. The specific binding of [³H]idazoxan to rat and human stomach membranes was saturable. Nonlinear regression analysis revealeda reaction of [³H]idazoxan with one binding site (K_d = 11.1 ± 2.2 nM and 12.4± 4.7 nM, respectively; B_max = 139 ± 4 fmol/mg protein and 68± 14 fmol/mg protein, respectively; figs. 1 and 2).

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Fig. 1. Saturation curve for specific [³H]idazoxan binding. Rat stomach membranes were incubated for 55 min at 4°C with increasing concentrations of [³H]idazoxan. The graph shows one representative experiment out of four performed in triplicate. At 10 nM [³H]idazoxan, nonspecific binding accounted for about 5% of the total radioactivity retained in the filters.

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Fig. 2. Competition of unlabeled idazoxan with [³H]idazoxan (upper panel) and of unlabeled DTG with [³H]DTG (lower panel) for its specific binding sites in human stomach membranes. Each point is the mean of five experiments performed in triplicate. In some cases, S.E. was smaller than the symbols. At 10 nM [³H]idazoxan and at 10 nM [³H]DTG, nonspecific binding accounted for about 5% and 12%, respectively, of the total radioactivity retained in the filters.

In competition experiments, most of the compounds listed in table 1 inhibited specific binding of 10 nM [³H]idazoxan to rat stomach membranes in a concentration-dependentmanner; at this radioligand concentration, specific binding amountedto 1188 ± 106 dpm (corresponding to about 95% of total binding;n = 48). Competition of BDF 6143 with [³H]idazoxan 10 nM revealed an inhibition curve with a slope factorn_H of less than 1. Accordingly, the competition curve for thiscompound was significantly better fitted to a two-site than toa one-site model (table 1; fig. 3). With the other competitors,monophasic displacement curves were obtained (n_H was not significantlydifferent from 1.0; fig. 3). The K_i values at the high-affinitysite or the single site for all drugs investigated ranged from11 to 265,800 nM (table 1) with the following rank order of affinities:idazoxan > cirazoline = BDF 6143 > naphazoline $>>$ dicozilpine >(+)-3-PPP > (±)-ifenprodil = clonidine $>>$ (±)-pentazocine > agmatine.Histamine, rauwolscine and ranitidine at concentrations up to100 µM inhibited binding by less than 50% (table 1).

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TABLE 1
Affinities (K_i values) of imidazolines and other compounds for [³H]idazoxan binding sites in rat stomach membranes
Results from computer analysis of competition curves^a obtained by adding various concentrations of a competing ligand and a fixed concentration (10 nM) of [³H]idazoxan. The percentages of high (%_high) and low (%_low) affinity sites are given for BDF 6143, which was best resolved (partial F test, last column) into a two-site fit. In parenthesis is the number of experiments performed in triplicate.

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Fig. 3. Competition of imidazoline derivatives (upper panel) and of $sigma$ -site ligands (lower panel) with [³H]idazoxan for its specific binding sites in rat stomach membranes. $square$ idazoxan, $open circle$ BDF 6143, $bullet$ clonidine, $triangle$ (+)-3-PPP, $black-lozenge$ (±)-pentazocine, $black-square$ (±)-ifenprodil. Each point is the mean of 3 to 7 experiments performed in triplicate. S.E. amounted to up to 11% of the respective mean.

[³H]DTG binding. The specific binding of [³H]DTG to rat and human stomach membranes was saturable. Homologous displacement experiments withunlabeled DTG and [³H]DTG revealed a reaction of [³H]DTG with one binding site with K_d values of 932 ± 319 nM and242 ± 90 nM, respectively, and B_max values of 7087 ± 4024 fmol/mgprotein and 3592 ± 553 fmol/mg protein, respectively (figs. 2and 4).

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Fig. 4. Competition of unlabeled DTG with [³H]DTG for its specific binding sites in rat stomach membranes. Each point is the mean of five experiments performed in triplicate. In some cases, S.E. was smaller than the symbols. At 10 nM [³H]DTG, nonspecific binding accounted for about 16% of the total radioactivity retained in the filters.

In competition experiments, the compounds listed in table 2 inhibited specific binding of [³H]DTG 10 nM to rat stomach membranes in a concentration-dependentmanner; at this radioligand concentration, specific binding amountedto 1206 ± 75 dpm (corresponding to 79% of total binding; n = 56).The drugs investigated as competitors of [³H]DTG revealed monophasic displacement curves (n_H was not significantlydifferent from 1; fig. 5). The K_i value of the compounds rangedfrom 0.5 to 668 µM (Table 2). The rank order of affinities wasas follows (table 2): haloperidol $>=$ (±)-ifenprodil $>=$ DTG > BDF6143 $>=$ clonidine > (+)-3-PPP > cirazoline $>=$ naphazoline > idazoxan> moxonidine > agmatine.

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TABLE 2
Affinities (K_i values) of imidazolines and other compounds for [³H]DTG binding sites in rat stomach membranes
Results from computer analysis of competition curves^a obtained by adding various concentrations of a competing ligand and a fixed concentration (10 nM) of [³H]DTG. In parentheses is the number of experiments performed in triplicate.

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Fig. 5. Competition of imidazoline derivatives (upper panel) and $sigma$ -site ligands (lower panel) with [³H]DTG for its specific binding sites in rat stomach membranes. $square$ idazoxan, $open circle$ BDF 6143, $bullet$ clonidine, $black-square$ (±)-ifenprodil, $diamond$ haloperidol, $black-triangle$ DTG. Each point is the mean of 4 to 7 experiments performed in triplicate. S.E. amounted to up to 22% of the respective mean.

Contraction of rat gastric fundus strips. In time-matched control experiments with the vehicle applied, the tension of the preparation slightly decreased by about 2%to 14% (not shown). The thromboxane analog U46619 induced a concentration-dependentcontraction of the rat gastric longitidinal muscle strips (fig.6). In contrast, the imidazolines cirazoline, clonidine and BDF6143 up to 100 µM (the highest concentration investigated, fig.6) failed to elicit a contractile response. When the smooth musclepreparation was precontracted with 30 mM KCl (a 75% effectiveconcentration) BDF 6143 up to 100 µM failed to induce a relaxationof the smooth muscles, whereas verapamil (chosen as the controlcompound) completely relaxed the preparation (n = 5; results notshown).

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Fig. 6. Contractile response to the prostanoid U46619 ( $black-square$ ) and to the imidazoline derivatives cirazoline ( $black-lozenge$ ), BDF 6143 ( $open circle$ ) and clonidine ( $bullet$ ) in the presence of 1 µM prazosin, 1 µM atropine and 3 µM rauwolscine. S.E. amounted to 2% to 12% of the respective means (n = 5-7).

[¹⁴C]aminopyrine accumulation in rabbit isolated gastric glands. In intact gastric glands from rabbits, histamine significantly increased [¹⁴C]aminopyrine accumulation (an index of acidification within theglands) in a concentration-dependent manner (fig. 7). However,the imidazolines idazoxan and BDF 6143, the guanidine agmatineand the $sigma$ -site ligands (+)-3-PPP and DTG were without effect onthe [¹⁴C]aminopyrine accumulation at concentrations up to 0.1 mM (fig.7). At this high concentration, clonidine increased [¹⁴C]aminopyrine accumulation in 2 of 4 experiments, but becauseof the scatter, the mean value did not reach the level of significance.However, the compound was without effect on [¹⁴C]aminopyrine accumulation at lower concentrations (fig. 7). Finally,BDF 6143 up to 100 µM did not alter histamine-induced [¹⁴C]aminopyrine accumulation (n = 3; results not shown).

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Fig. 7. Influence of histamine ( $black-square$ ), of the imidazoline derivatives idazoxan ( $square$ ), clonidine ( $bullet$ ) and BDF 6143 ( $open circle$ ) and of the guanidine agmatine ( $black-lozenge$ ), as well as of the $sigma$ -site ligands DTG ( $black-triangle$ ) and (+)-3-PPP ( $triangle$ ) on [¹⁴C]aminopyrine accumulation in rabbit gastric glands. Each point is the mean of 3 to 7 experiments determined in duplicate. S.E. amounted to up to 10%, with the exception of 0.1 mM clonidine, for which S.E. was 17%. ** P < .005, *** P < .001 (compared with the corresponding controls).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

[³H]idazoxan binding. Binding of [³H]idazoxan to rat and human stomach membranes was reversible (not shown), specific, saturable and of high affinity;i.e., the criteria for the identification of a specific bindingsite are fulfilled. The K_d values of [³H]idazoxan (11 nM and 12 nM, respectively) were identical to theK_i value obtained in the competition experiments with unlabeledidazoxan in rat stomach. The values are in the range reportedin the literature for I₂-imidazoline binding sites (Wikberg etal., 1992; Regunathan et al., 1993; Miralles et al., 1993; Molderingset al., 1994).

In the competition experiments, a shallow displacement curve (n_H < 1.0) was obtained with BDF 6143, but not with the othercompounds. The curve of BDF 6143 was fitted best to two bindingsites by computer modeling. Shallow inhibition curves with Hillcoefficients significantly different from unity have also beenfound in previous studies on bovine chromaffin cells (Molderingset al., 1993

; Regunathan et al., 1993

) and on guinea pig kidney(Wikberg et al., 1992

). As an explanation, it has been proposedthat the IBS may exist in two interconvertible forms (Wikberget al., 1992

; Li et al., 1994

). Alternatively, the data mightbe explained by assuming monomer-dimer equilibria (Strange, 1994

),in which BDF 6143 would bind with different preference to themonomer or dimer of the binding site and hence would representa case of negative cooperativity. Finally, it is conceivable that[³H]idazoxan also labeled an I₁-like site and that this accountsfor the low Hill slope of BDF 6143. In this case, however, cirazolineand naphazoline, which also possess high affinity for the I₁-likesites, should also have yielded a biphasic displacement curve.That did not occur, so this explanation appears unlikely.

The present data exclude the possibility that [³H]idazoxan labeled a histamine receptor, in particular an H₂ receptor or analpha-2 adrenoceptor, because histamine and ranitidine failedto compete with high affinity for the [³H]idazoxan site, and the alpha-2 adrenoceptor antagonist rauwolscineexhibited only very low affinity for [³H]idazoxan sites. In agreement with this, the rank order of potencyof the competing drugs (table 1) differs from the rank orderexpected for binding to one of the alpha-2 adrenoceptor subtypes(Bylund et al., 1994

). Moreover, ( $-$ )-adrenaline in the high concentrationof 10 µM was included in the incubation assay to mask the alpha-2adrenoceptor population in the membrane preparation.

The pharmacological properties of the idazoxan binding sites in the rat stomach were compared with those of I₁-IBS and I₂-IBSin bovine adrenomedullary membranes (Molderings et al., 1993

,1994

) and of the nonadrenoceptor [³H]clonidine binding sites in the same tissue (Molderings et al.,1995

). The rank order of affinity of the competing drugs for theI₁-IBS, i.e., naphazoline > clonidine = cirazoline > BDF 6143> idazoxan > phentolamine (Molderings et al., 1993

), and in particularthe affinity of clonidine, are clearly different from the findingsin the present experiments (table 1). Therefore, it is unlikelythat the [³H]idazoxan binding site represents an I₁-IBS. The [³H]idazoxan binding sites are also not identical to the nonadrenoceptor[³H]clonidine binding sites previously described in the rat stomach(Molderings et al., 1995

) for two reasons: (1) The affinitiesof the imidazolines for the [³H]idazoxan binding sites were not correlated with their affinitiesfor the [³H]clonidine binding sites in the same tissue (fig. 8A). (2) $sigma$ -Siteligands, which exhibited high to moderate affinity for the [³H]clonidine binding sites in the rat stomach, possess only weakaffinity for the [³H]idazoxan binding sites. In contrast, the rank order of affinityof competing imidazolines and guanidines at I₂-IBS in bovine adrenomedullarymembranes was cirazoline $>=$ idazoxan > guanabenz > tolazoline >rilmenidine > clonidine > phentolamine (Molderings et al., 1994

)and hence conforms to the rank order found in our experiments.Accordingly, the [³H]idazoxan binding sites identified here may be characterizedas I₂-IBS.

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Fig. 8. (Upper panel) Lack of correlation of the pK_i values of imidazolines determined for the high-affinity [³H]clonidine binding sites in rat stomach membranes (from Molderings et al., 1995

) with their pK_i values determined for the high-affinity [³H]idazoxan binding sites in the same tissue (present study). (Lower panel) Highly significant correlation of the pK_i values of imidazolines and $sigma$ -site ligands determined for the [³H]DTG binding sites in rat stomach membranes (present study) with their pK_i values determined for the [³H]DTG binding sites ( $sigma$ ₂ sites) on N1E-115 cells (Molderings et al., 1996

). Numbers in the graph: 1, idazoxan; 2, cirazoline; 3, BDF 6143; 4, naphazoline; 5, agmatine; 6, clonidine; 7, (+)-3-PPP; 8, haloperidol; 9, (±)-ifenprodil; 10, DTG; 11, moxonidine. The dotted line is the line of identity.

[³H]DTG binding. Specific [³H]DTG binding to the rat and human stomach membranes was saturable, reversible (not shown) and of moderate affinityand high capacity. The K_d values for [³H]DTG (932 nM and 242 nM, respectively) were consistent with thevalues previously observed in rat brain and liver, in guinea pigbrain, in porcine stomach and on N1E-115 cells (McCann and Su,1990; DeHaven-Hudkins and Fleissner, 1992; Harada et al., 1994;Molderings et al., 1996).

The affinities of the compounds for the [³H]DTG binding sites determined in the competition experiments were in the micromolarto millimolar range, which is compatible with previously publishedradioligand binding studies of peripheral $sigma$ binding sites in porcinestomach (Harada et al., 1994

) and on N1E-115 cells (Molderingset al., 1996

). Comparison of the pK_i values of the drugs withtheir affinities (pK_i values) for the $sigma$ ₂ sites on N1E-115 cells(Molderings et al., 1996

) revealed a significant correlation (fig.8B). These data suggest that the [³H]DTG binding sites in the rat stomach represent $sigma$ ₂ binding sites,which is consistent with the finding of Harada et al. (1994)

inpig stomach.

Because the affinities of the imidazolines BDF 6143 and clonidine for these $sigma$ sites were in the same range as those of typical $sigma$ -site ligands such as haloperidol and DTG (table 2), and becauseit has recently been shown that nonimidazoline $sigma$ -site ligandspossess a remarkable affinity for the nonadrenoceptor [³H]clonidine binding sites in the rat stomach, a relationship betweenthe imidazoline binding sites and the $sigma$ sites in the rat stomachwas conceivable. However, there was no correlation between theaffinity of the drugs for the [³H]DTG binding sites and their affinity for the nonadrenoceptor[³H]idazoxan and [³H]clonidine binding sites in rat stomach (r = 0.15, P > 0.74 andr = 0.10, P > 0.10; seven and nine compounds included in the regressionanalysis, respectively). Hence the three binding sites appearto represent different entities.

Functional experiments. In the stomach, the functional effects of imidazolines and guanidines that have previously been observed were tentativelyascribed to an activation of imidazoline receptors. The presentstudy focused on two clearly nonadrenoceptor-mediated effects:the contraction of gastric smooth muscle and the imidazoline-inducedstimulation of gastric acid release. In particular, the questionarose whether these effects were related to one of the heretofore-describedbinding sites at the level of the effector cells.

It was previously reported that CDS, which is assumed to be an endogenous ligand at imidazoline bindings sites/receptors (Meeleyet al., 1986

; Atlas, 1991

; Piletz et al., 1995

), elicited a concentration-dependentcontraction of rat gastric fundus strips (Felsen et al., 1987

).Because the CDS-induced contraction was not counteracted by muscarine,bradykinin, serotonin, angiotensin II, vasopressin or alpha-2receptor antagonists, it was suggested that the CDS-evoked contractionwas mediated by imidazoline receptors (Felsen et al., 1987

). However,in the present study BDF 6143, clonidine and cirazoline did notmimic the effect of CDS reported previously, although the compoundspossess high affinity for I₁- and/or I₂-imidazoline binding sites/receptors.In contrast, the thromboxan analog U46619 induced a contractionof the rat gastric strips, which indicates that the smooth musclecells were viable and able to contract. Hence the binding of theligands to nonadrenoceptor [³H]idazoxan and [³H]clonidine binding sites in rat stomach did not cause a contractionof gastric smooth muscle. Because in the stomach BDF 6143 andclonidine additionally exhibited an affinity for the [³H]DTG binding sites similar to those of the typical $sigma$ -site ligands(see table 2), it is also unlikely that these $sigma$ ₂ sites are involvedin contraction of gastric smooth muscles.

It has also been speculated that the stimulation of gastric acid release induced by high concentrations of clonidine and relatedcompounds in rat and guinea pig (for references, see the Introduction)might be due to activation of imidazoline recognition sites (Houiet al., 1987

; Bhandare et al., 1991

). Nonadrenoceptor [³H]idazoxan (Tesson et al., 1992

) and [³H]clonidine (G.J. Molderings, unpublished results) binding siteshave also been found in the rabbit stomach. Therefore, [¹⁴C]aminopyrine accumulation in isolated rabbit gastric glands wasused to investigate whether imidazolines increase acid secretionby direct activation of the gastric glands, because this is thestandard in vitro model for the study of acid secretory mechanismsof the mammalian parietal cells (Berglindh, 1977

; for review seeChew, 1994

). As expected, stimulation of H₂ histamine receptorsby histamine induced an increase of acid release within the glandsand thereby led to an accumulation of the weak base [¹⁴C]aminopyrine (fig. 7). In contrast, BDF 6143, idazoxan and theputative endogenous ligand at imidazoline sites, agmatine (Liet al., 1994

), failed to induce an increase in [¹⁴C]aminopyrine accumulation and hence obviously did not induceacid release. Clonidine at the extremely high concentration of0.1 mM inconsistently increased [¹⁴C]aminopyrine accumulation but was without effect at the lowerdrug concentrations. The latter finding is in contrast to theincrease in acid release induced by clonidine and tolazoline froma guinea pig parietal cell preparation (Houi et al., 1987

). Thisrelease was ascribed to activation of imidazoline receptors, althoughthe effect was potently inhibited by the H₂ histamine receptorantagonists cimetidine, ranitidine and famotidine (Houi et al.,1987

), which, in turn, did not compete with [³H]clonidine for the nonadrenoceptor [³H]clonidine binding sites in guinea pig stomach mucosa (Houi etal., 1987

). Because only 65% of the parietal cell preparationprepared by Houi et al. (1987)

consisted of parietal cells, aplausible (though speculative) explanation for the discrepancybetween our present results and those obtained by Houi et al.might be that the imidazolines stimulate acid release indirectly,perhaps by inducing the release of endogenous histamine. Thiswould be consistent with the observation that the imidazoline-inducedrelease of gastric acid was blocked by H₂ histamine receptor antagonists(Houi et al., 1987

). Taken together, our results make it ratherunlikely that the stimulatory effect of the imidazolines on gastricacid release observed in vivo and in whole-stomach preparationsis due to activation of nonadrenoceptor [³H]idazoxan or [³H]clonidine binding sites located on parietal cells.

For the following reasons, we also investigated whether the potent $sigma$ -site ligands (+)-3-PPP and DTG influenced gastric acidsecretion in rabbit glands. (1) $sigma$ -Site ligands possess a remarkableaffinity for the [³H]clonidine binding sites in rat stomach (Molderings et al., 1995

).(2) Imidazolines exhibit a considerable affinity for peripheral $sigma$ ₂ sites (Molderings et al., 1996

; present study). (3) $sigma$ ₂-Sitesare believed to play some role in the control of gastric function(Harada et al., 1994

). However, both (+)-3-PPP and DTG failedto increase [¹⁴C]aminopyrine accumulation and, accordingly, did not induce acidsecretion by direct stimulation of the parietal cell.

Conclusion. Our data provide evidence that, in addition to the previously identified non-I₁/non-I₂ [³H]clonidine binding sites (Molderings et al., 1995), the rat stomachis endowed with [³H]idazoxan binding sites that belong to the I₂ subclass. In addition, $sigma$ ₂ sites are present in the rat stomach. Our experiments alsoprovide basic evidence for the existence of I₂ and $sigma$ binding sitesin the human stomach. The three different binding sites appearnot to act directly on gastric smooth muscle. They also do notmediate direct stimulation of gastric acid release from parietalcells.

	Acknowledgments

The technical assistance of Mrs. D. Funccius and Mrs. M. Hartwig is gratefully acknowledged. We wish to thank the pharmaceuticalcompanies for generous gifts of drugs. The study was supportedby the Deutsche Forschungsgemeinschaft.

	Footnotes

Accepted for publication December 1, 1997.

Received for publication June 30, 1997.

Send reprint requests to: G.J. Molderings, Institute of Pharmacology and Toxicology, University of Bonn, Reuterstr. 2b, D-53113 Bonn, Germany.

	Abbreviations

U46619, 9,11-dideoxy-11 $alpha$ ,9 $alpha$ -epoxy-methano-prostaglandin F₂; BDF 6143, 4-chloro-2-(2-imidazolin-2-ylamino)-isoindoline; (+)-3-PPP, (R)-3-(3-hydroxyphenyl)-N-propylpiperidine; DTG, 1,2-di-(2-tolyl)guanidine; IBS, imidazoline binding sites; CDS, clonidine-displacing substance.

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