Methocinnamox Is a Potent, Long-Lasting, and Selective Antagonist of Morphine-Mediated Antinociception in the Mouse: Comparison with Clocinnamox, beta -Funaltrexamine, and beta -Chlornaltrexamine

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MORPHINE
NALTREXONE

Vol. 294, Issue 3, 933-940, September 2000

Methocinnamox Is a Potent, Long-Lasting, and Selective Antagonist of Morphine-Mediated Antinociception in the Mouse: Comparison with Clocinnamox, $beta$ -Funaltrexamine, and $beta$ -Chlornaltrexamine¹

Jillian H. Broadbear, Tina L. Sumpter, Timothy F. Burke² , Stephen M Husbands³ , John W. Lewis, James H. Woods and John R. Traynor

Departments of Psychology (J.H.B., J.H.W.) and Pharmacology (J.R.T., T.F.B., J.H.W.), University of Michigan Medical School, Ann Arbor, Michigan; and Department of Chemistry, University of Bristol, Bristol, United Kingdom (S.M.H., J.W.L.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

The irreversible µ-opioid antagonists $beta$ -funaltrexamine ( $beta$ -FNA) and $beta$ -chlornaltrexamine ( $beta$ -CNA) are important pharmacologicaltools but have a $kappa$ -agonist activity and, in the latter case, lowselectivity. This work examines whether clocinnamox (C-CAM) andthe newer analog, methocinnamox (M-CAM), represent improved long-lastingantagonists for examining µ-opioid-mediated effects in vivo. $beta$ -FNA, $beta$ -CNA, C-CAM, and M-CAM were compared after systemic administrationin mice and in vitro. $beta$ -FNA and $beta$ -CNA were effective agonistsin the writhing assay, reversible by the $kappa$ -antagonist norbinaltorphimine.Neither C-CAM nor M-CAM had agonist activity in vivo. M-CAM wasdevoid of agonist action at cloned opioid receptors. All fourcompounds depressed the dose-effect curve for the µ-agonist morphinein the warm-water tail-withdrawal test 1 h after administration;at 48 h, recovery was evident. In the writhing assay, the dose-effectcurve for morphine was shifted in a parallel fashion in the orderM-CAM C-CAM > $beta$ -CNA $>=$ $beta$ -FNA. In comparison with their abilityto shift the dose-effect curve for bremazocine ( $kappa$ ) and BW373U86( $delta$ ), $beta$ -CNA was the least µ-selective, followed by C-CAM < $beta$ -FNA< M-CAM. M-CAM (1.8 mg/kg) produced a 74-fold increase in theED₅₀ of morphine while showing no effect on bremazocine or BW373U86dose-response curves. In binding assays, C-CAM and M-CAM were8-fold selective for µ- over $kappa$ -receptors, whereas $beta$ -FNA and $beta$ -CNAwere µ/ $delta$ -, but not µ/ $kappa$ , selective. However, ex vivo binding assaysconfirmed the µ-receptor selectivity of M-CAM. M-CAM is thus apotent, long-lasting, and specific antagonist at µ-receptors invivo that lacks confounding agonistactions.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

The role of the µ-receptor in opioid pharmacology in the mouse is best studied in knock-out animals (Matthes et al., 1996).However, in other species, it is necessary to provide completeand long-lasting blockade of the µ-opioid receptor to undertakesimilar studies. Development of the irreversible opioid antagonists $beta$ -chlornaltrexamine ( $beta$ -CNA) and $beta$ -funaltrexamine ( $beta$ -FNA; Takemoriand Portoghese, 1985) and the long-lasting, but nonalkylating,antagonist clocinnamox (C-CAM; Comer et al., 1992; Fig. 1) providedthe opportunity to study opioid agonists in the absence of a particularreceptor type (Takemori and Portoghese, 1987), the relative efficacyof opioid agonists (e.g., Adams et al., 1990; Mjanger and Yaksh,1991; Comer et al., 1992; Zernig et al., 1995a), and the meansto make inferences about opioid receptor turnover (e.g., Carusoet al., 1980; Burke et al., 1994; Zernig et al., 1994).

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Fig. 1. Structures of C-CAM, M-CAM, $beta$ -CNA, and $beta$ -FNA.

$beta$ -FNA is the most thoroughly characterized irreversible opioid antagonist (Takemori et al., 1981; Ward et al., 1982a,b; Takemoriand Portoghese, 1985; Mjanger and Yaksh, 1991); $beta$ -CNA is lessso (Caruso et al., 1980; Ward et al., 1982a; Takemori and Portoghese,1985). Although $beta$ -CNA is thought to bind irreversibly to all opioidbinding sites with similar affinity (Ward et al., 1982a), theirreversible antagonist effects of $beta$ -FNA are mediated almost entirelyvia µ-receptors (Takemori et al., 1981; Ward et al., 1982b; Liu-Chenand Phillips, 1987). A drawback to both irreversible antagonistsis a reversible $kappa$ -agonist activity that initially coincides withantagonist effects (Takemori et al., 1981; Ward et al., 1982a,b).Because $beta$ -FNA and $beta$ -CNA are generally used for their antagonistproperties, an extended pretreatment time is required in vivoto allow the reversible agonist effect to subside (Ward et al.,1982b; Zimmerman et al., 1987; Broadbear et al., 1994). It canbe inferred, however, that both agonist and antagonist activityoccur simultaneously, so it is possible that the agonist effectsof $beta$ -FNA and $beta$ -CNA may alter their subsequent antagonist activity.Furthermore, $beta$ -FNA alkylates only 50% of µ-opioid receptors (Franklinand Traynor, 1991; Martin et al., 1993). This may be due to differentialalkylation of putative subtypes or to different affinity statesof the µ-opioid receptor (Tam and Lui-Chen, 1986; Franklin andTraynor, 1991). Also, a dichotomy exists between the recoveryof binding and the more rapid recovery of µ-opioid pharmacologicaleffects after $beta$ -FNA administration, such as the recovery of heroinself-administration in rats (Martin et al., 1995). Thus, thereis a need for additional long-acting µ-opioid antagonists to studytheseproblems.

We have previously reported on the novel, systemically active long-lasting opioid antagonist clocinnamox (C-CAM; Comer etal., 1992). In the mouse warm-water tail-withdrawal test, C-CAMsuppresses the antinociceptive effect of fentanyl such that themaximal effect is not achieved and completely abolishes the responseto morphine, even up to lethal doses (Comer et al., 1992). Thisnoncompetitive nature to the antagonism mediated by C-CAM andthe long duration of antagonist activity that lasts for up to8 days led to the conclusion that C-CAM acts via a nonequilibriummechanism. Indeed, a number of in vitro and ex vivo studies haveprovided additional evidence that C-CAM and related compoundsbind with high affinity to the µ-receptor and dissociate veryslowly (Burke et al., 1994; Jiang et al., 1994; Zernig et al.,1994, 1995b; McLaughlin et al., 1999).

This study provides a more detailed characterization of C-CAM and in particular its close analog methocinnamox [M-CAM; 14p-(4'-methylcinnamoylamido)-7,8-dihydro-N-cyclopropylmethyl-normorphinonemesylate, Fig. 1] and compares them functionally with $beta$ -FNA and $beta$ -CNA as tools for the long-lasting blockade of systemically administeredµ-opioid agonists. The compounds were evaluated in vivo usingthe warm-water tail-withdrawal and acetic acid-induced writhingprocedures in mice, and the binding of each of the antagoniststo opioid receptors was examined in mouse brain using both invitro and ex vivo methods. The results confirm that C-CAM andM-CAM are devoid of agonist effects both in vitro and in vivoand provide a long-lasting and, in the case of M-CAM, a highlyselective blockade of µ-opioidreceptors.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Animals

Male NIH Swiss mice weighing 20 to 32 g (Harlan Sprague-Dawley, Indianapolis, IN) were housed in standard laboratory cages(8-12/cage) in a temperature-controlled colony room maintainedon a 12-h light/dark cycle. Food (Purina Rodent Chow; Purina Mills,St. Louis, MO), and water were available ad libitum until testing.Each animal was used only once and was sacrificed by an overdoseof pentobarbital immediately after use. Studies were carried outin accordance with the Declaration of Helsinki and with the Guidefor the Care and Use of Laboratory Animals as adopted and promulgatedby the National Institutes of Health. The University of MichiganUniversity Committee on the Use and Care of Animals approved theexperimentalprotocols.

Chemicals and Drugs

[³H][D-Ala²,N-Me-Phe⁴,Gly⁵-o1]-Enkephalin ([³H]DAMGO; 40.7Ci/mmol) was purchased from Amersham (Arlington Heights, IL). [³H]U69,593 ([³H](5 $alpha$ ,7 $alpha$ ,8 $beta$ -(+)-N-methyl-N-[7-(I-pyrrolidinyl)-1-oxaspiro[4,5]dec-8-yl]benzeneacetamide;47.9 Ci/mmol) and [³H][D-Pen²,D-Pen⁵]-enkephalin ([³H]DPDPE; 30 Ci/mmol) were obtained from New England Nuclear (Boston,MA). $beta$ -CNA was purchased from Research Biochemicals International(Natick, MA). Morphine sulfate was obtained from Mallinckrodt(St. Louis, MO). DAMGO, DPDPE, fentanyl, naloxone, and U69593were obtained from Sigma Chemical Co. (St. Louis, MO). Naltrindole(NTI) and norbinaltorphimine (nor-BNI) were gifts from Dr. B.de Costa (National Institutes of Health, Bethesda, MD). BW373U86[(±)-[1(S*),2, $alpha$ ,5 $beta$ ]-4-[[2,5-dimethyl-4-(2-propenyl)-1-piperazinyl]-(3-hydroxyphenyl)methyl]-N,N-diethylbenzamide]was a gift from Burroughs Wellcome (Research Triangle Park, NC).Bremazocine was a gift from Sandoz (Basel, Switzerland). SNC80[(+)-4-[( $alpha$ -R)- $alpha$ -[(2S,5R)-4-allyl-2,5-dimethyl-1-piperazinyl]-3-methoxybenzyl]-N,N-dimethylbenzamide]was a gift from Dr. K. C. Rice (National Institutes of Health,Bethesda, MD). $beta$ -FNA and C-CAM were synthesized in our laboratoriesas previously described (Portoghese et al., 1980; Lewis et al.,1988). M-CAM was synthesized by acylation of 14-aminodihydrocodeinonewith p-methoxycinnamoyl chloride followed by 3-O-demethylationas follows. p-Me-cinnamic acid (201 mg, 1.24 mmol) in anhydroustoluene was refluxed with oxalyl chloride (0.77 ml, 8.8 mmol)for 1 h. The toluene and excess oxalyl chloride were then removedin vacuo, and CH₂Cl₂ (10 ml), 14-aminodihydrocodeinone (350 mg,1.0 mmol), and triethylamine (0.16 ml, 1.1 mmol) were added. Stirringwas continued overnight before adding a saturated solution ofNaHCO₃ and extracting with CH₂Cl₂. The organic layer was collected,dried (Na₂SO₄), and evaporated to a fawn powder. Silica gel chromatography(95:4:1, CH₂Cl₂/MeOH/NH₃) yielded 3-methoxymethocinnamox (MM-CAM)as a white solid; 410 mg (84%) calculated for C₃₁H₃₄N₂O₄·MeSO₃H·1.5H₂O, CHN. MM-CAM (200 mg, 0.4 mmol) was cooled to $-$ 30°C in CH₂Cl₂(5 ml) before adding BBr₃ (1 M in CH₂Cl₂, 2.4 ml, 2.4 mmol). Thesolution was allowed to warm to room temperature over 1 h beforepouring into a 1:1 mixture of ice/conc. NH₃. The organic phasewas collected, and the aqueous layer was extracted with CH₂Cl₂(3 × 5 ml). The organic layers were combined and washed with brine(15 ml), dried over Na₂SO₄, and evaporated in vacuo to leave adark foam. Silica gel chromatography (95:4:1, CH₂Cl₂/MeOH/NH₃)yielded M-CAM as a white solid. 100 mg (52%), $delta$ H (DMSO) 2.33(3 H, s, Ar-CH₃), 2.95 (1 H, d, J = 18.3 Hz, 10 $beta$ -H), 4.88 (1 H,s, 5-H), 6.54 (1 H, d, J = 8.1 Hz, 1-H), 6.59 (1 H, d, J = 8.1Hz, 2-H), 6.88 (1 H, d, J = 15.6 Hz, COCH==CHAr), 7.24 (2 H, d,J = 8.0 Hz, 3'- and 5'-H), 7.42 (1 H, d, J = 15.6 Hz, COCH==CHAr),7.52 (2 H, d, J = 8.1 Hz, 2'- and 6'-H); calculated for C_3OH₃₂N₂O₄·HCl·H₂O,CHN.

All compounds were dissolved in distilled water and administered in volumes of 10 ml/kg for in vivo experiments. C-CAM, dueto its limited solubility, was administered in a volume of 32ml/kg to obtain the 32-mg/kgdose.

Acetic Acid-Induced Writhing Assay

The antinociceptive effects and antagonist selectivity of each of the drugs used in this study were assessed using a modificationof the acetic acid-induced writhing assay as previously described(Traynor et al., 1999). Mice were injected i.p. with 0.4 ml of0.6% acetic acid and placed in individual Plexiglas boxes (18× 28 × 23 cm) for observation. Five minutes later, a 5-min observationperiod was initiated, during which the number of writhes was recorded.Each writhe typically consisted of a wave of contraction of theabdominal musculature followed by extension of the hind legs.Test drug or vehicle was administered either s.c. (agonists) ori.p.(antagonists) at various times before acetic acidadministration.

Agonist Activity. C-CAM (10 mg/kg) and M-CAM (32 mg/kg) were tested for antinociceptive effects at 15, 30, and 60 min after administration. $beta$ -FNA (32 mg/kg) was tested at a number of time points rangingfrom 10 min to 24 h after administration. The effect of the $kappa$ -selectiveantagonist nor-BNI (32 mg/kg i.p.; 24-h pretreatment) was examinedat the time agonist effect was at its maximum. Due to limitedavailability, single-dose experiments with $beta$ -CNA (32 mg/kg) wereperformed 1 h afteradministration.

Antagonist Activity. The antagonist activity of $beta$ -CNA, $beta$ -FNA, C-CAM, and M-CAM was tested against morphine (µ-agonist), BW373U86 ( $delta$ -agonist), andbremazocine ( $kappa$ -agonist) using doses and pretreatment times ofthe antagonists that produced a 5- to 10-fold shift in the morphinedose-effect curve. If no antagonism of either bremazocine or BW373U86was observed, higher doses of the antagonist weretested.

The number of writhes for each mouse was expressed as a percentage of the control number of writhes per mouse. The controlnumber of writhes per mouse was defined as the mean number ofwrithes per mouse when s.c. injection of sterile water was administered15 min before the acetic acid injection. Individual percentagecontrol values for mice in the treatment group were averaged,and the S.E.M. value was calculated. Each data point representsthe results from six mice, unless otherwise noted, and each mousecontributed to only one condition in a dose-effectevaluation.

Warm-Water Tail-Withdrawal Assay

The antinociceptive effect of morphine in the presence or absence of $beta$ -FNA, $beta$ -CNA, C-CAM, and M-CAM was measured using thewarm-water tail-withdrawal procedure as modified for mice (Burkeet al., 1994). Each mouse was restrained in a cylindrical plasticcontainer (Harvard Apparatus, South Natick, MA) that allowed thetail to protrude. The tail was immersed to up to half its lengthin 55.0 ± 0.2°C water, and the latency to tail withdrawal wasmeasured using a stopwatch. A cumulative dosing procedure formorphine was used whereby testing and injection of the next concentrationof morphine took place every 30 min. The initial measurement (baselinelatency) was determined 25 min after an injection of sterile water.All injections were given i.p. This injection-testing procedurecontinued until either the mouse failed to remove its tail after15 s of immersion (designated as "100% analgesia") or toxic effectsof high doses (e.g., convulsions and/or death) interfered withthemeasurements.

Data are presented as percentage maximum effect (MPE) = [(test latency $-$ baseline latency)/(cutoff time $-$ baseline latency)]× 100, where cutoff time was 15 s, and baseline latency is thedelay from immersion until withdrawal of the tail from 55°C waterafter an injection of vehicle (sterile water). The results formice in a particular group were averaged, and the S.E.M. valuewas calculated. The dose-effect curves consist of data from atleast five mice; each mouse contributed to only oneexperiment.

Binding Assays

In Vitro. Homogenates of mouse cerebral cortex were prepared and ligand-binding assays were performed essentially as previously described(Burke et al., 1994). The relative affinities of C-CAM, M-CAM, $beta$ -FNA, and $beta$ -CNA were determined in competition studies using[³H]DAMGO (0.5 nM) to label µ-sites, [³H]U69,593 (1.5 nM) to label $kappa$ -sites, and [³H]DPDPE (1.5 nM) to label $delta$ -sites. Each assay included 0.5 mghomogenate protein (Lowry et al., 1951), radiolabeled ligand,and various concentrations of unlabeled drug in a total volumeof 0.525 ml in 50 mM Tris-HCl buffer. Incubations were performedat 25°C for 80 min ([³H]DAMGO), 40 min ([³H]U69,593), or 70 min ([³H]DPDPE). Specific binding was defined in the presence of an excess(10 µM) of the corresponding unlabeled ligand. Reactions wereterminated by rapid filtration through glass-fiber disks (WhatmanGF/C) treated with water that had been saturated at room temperaturewith N-amyl alcohol ([³H]DAMGO or [³H]DPDPE assays) or 0.05% polyethyleneimine ([³H]U69,593 assays). Filters were rapidly washed three times with3 ml ice-cold 50 mM Tris-HCl, pH 7.4, and the radioactivity retainedon the filters was determined by liquid scintillationcounting.

Ex Vivo. Mice were treated s.c. with M-CAM (1.8 mg/kg) or sterile water. Then, 1 h later, the mice were sacrificed, and the brainswere rapidly removed. Homogenates of brain (minus cerebellum)were prepared in 10 volumes Tris-HCl (pH 7.4, 50 mM) and centrifugedat 18,000g for 20 min. The resultant pellet was resuspended inTris-HCl buffer, warmed to 37°C for 20 min to dissociate looselybound ligands, and then recentrifuged. The final pellet was resuspendedin Tris-HCl buffer for binding assays. The specific binding of[³H]DAMGO (1.6 nM), [³H]DPDPE (2.6 nM), and [³H]bremazocine (1 nM in the presence of 1 µM DAMGO and 1 µM DPDPEto block binding to µ- and $delta$ -receptors) was determined at 25°Cfor 60 min, as earlier, using naloxone (10 µM) to define nonspecificbinding.

[³⁵S]Guanosine-5'-O-(3-thio)triphosphate (GTP $gamma$ S) Assays

C6 glioma cells stably transfected with either the rat cloned µ-opioid (C6µ; Alt et al., 1998) or $delta$ -opioid receptor (C6 $delta$ ;Clark et al., 1997), and CHO cells expressing the human $kappa$ -opioidreceptor (CHO-hkor; Zhu et al., 1997) were cultured in Dulbecco'smodified Eagle's medium (C6 cells) or Dulbecco's modified Eagle'smedium/F-12 (CHO-hkor cells), with 10% fetal calf serum and 1.0to 0.2 mg/ml geneticin. Cells were grown in monolayers to confluencyat 37°C in a humidified 5% CO₂ atmosphere. Cells were harvestedin HEPES (20 mM, pH 7.4)-buffered saline containing 1 mM EDTA,dispersed by agitation, and collected by centrifugation at 500g.The cell pellet was suspended in a buffer of 20 mM HEPES, pH 7.4,100 mM NaCl, and 10 mM MgCl₂·6H₂O (buffer A) and homogenized usinga tissue tearor (Biospec Products). The resultant homogenate wascentrifuged at 50,000g, and the pellet was collected, washed inbuffer A, and recentrifuged. The pellet was finally resuspendedin buffer A to give a protein concentration of 100 to 200 µg/ml(Lowry et al., 1951) and stored at $-$ 80°C. All procedures wereperformed at 4°C.

Membranes (approximately 50 µg protein) were incubated in buffer A containing [³⁵S]GTP $gamma$ S (80 pM), GDP (3 µM), and varying concentrations of testcompound in a total volume of 1 ml for 60 min at 30°C as describedpreviously (Traynor and Nahorski, 1995). Nonspecific binding wasdefined using unlabeled GTP $gamma$ S (10 µM). Bound and free [³⁵S]GTP $gamma$ S were separated by vacuum filtration through GF/B filtersand quantified by liquid scintillation counting. Specific bindingwas 90 to 95% of total binding. Maximal stimulation of [³⁵S]GTP $gamma$ S was determined using 10 µM fentanyl (C6µ), 10 µM SNC80(C6 $delta$ ), and 10 µM U69593 (CHO-hkor).

Data Analysis

Behavioral Assays. ED₅₀ values for agonists in the absence and presence of antagonist were calculated as described by Tallarida and Murray (1987).Shifts in ED₅₀ values were determined to be statistically significantif there was no overlap in the 95% confidenceintervals.

In Vitro Assays. Data from binding and [³⁵S]GTP $gamma$ S assays were analyzed by nonlinear regression using Prism version 2.01 (GraphPad Software, SanDiego, CA) to give IC₅₀ values for the ligand binding and EC₅₀values for the [³⁵S]GTP $gamma$ S assays. IC₅₀ values were converted to K_i values usingthe Cheng and Prusoff (1973) equation. These data are presentedas apparent K_i values due to the likely nonequilibrium propertiesof the compounds. Data are mean ± S.E. values from at least threeexperiments performed in triplicate. Statistical significancewas determined using Student's ttest.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Antinociceptive Assays

Agonist Activity. In the acetic acid-induced writhing assay, neither C-CAM (10 mg/kg) nor M-CAM (32 mg/kg) produced a significant decrease inwrithing relative to the sterile water control at 15-, 30- (datanot shown), and 60-min pretreatment times (Fig. 2). In contrast,at 32 mg/kg, both $beta$ -CNA and $beta$ -FNA were effective in suppressingthe writhing response: $beta$ -FNA at 15 min after administration and $beta$ -CNA at 60 min after administration (Fig. 2). The antinociceptiveactivity of $beta$ -CNA and $beta$ -FNA was prevented by pretreatment withthe $kappa$ -selective antagonist nor-BNI administered as a 24-h pretreatment(Fig. 2). None of the compounds, at the doses shown in Fig. 2,showed evidence of agonist activity in the 55°C warm-water tail-withdrawalassay (data not shown).

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Fig. 2. Effects of C-CAM, M-CAM, $beta$ -CNA and $beta$ -FNA in the mouse acetic acid-induced writhing assay. Drugs were administered s.c. at the times indicated before assay. The antinociceptive activity of $beta$ -CNA and $beta$ -FNA was prevented by nor-BNI (32 mg/kg, 24-h pretreatment). Each column represents the mean ± S.E. of the writhing activity of six mice relative to sterile water controls.

Antagonist Effects. $beta$ -FNA, $beta$ -CNA, C-CAM, and M-CAM all antagonized the antinociceptive actions of morphine in the warm-water tail-withdrawal test.At 1 h after the administration of either C-CAM (1 mg/kg; Fig.3a) or M-CAM (1 mg/kg; Fig. 3b), a rightward shift in the morphinedose-effect curve was observed. A dose-related effect was evidentbecause the higher dose of 3.2 mg/kg caused a more pronouncedeffect and, in the case of M-CAM, a complete flattening of themorphine dose-response curve (Fig. 3, a and b). $beta$ -FNA and $beta$ -CNAalso showed a very strong antagonism of the antinociceptive effectof morphine in this assay (Fig. 3, c and d). The order of potencywas M-CAM > C-CAM > $beta$ -CNA > $beta$ -FNA. With all compounds, antagonismwas still evident 48 h after administration, but at this timemorphine showed recovery to a full antinociceptive effect butwith a shift to the right in the dose-effect curve.

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Fig. 3. Effects of morphine in the mouse determined in the warm-water tail-withdrawal assay. Morphine-induced antinociception was determined without or after pretreatment at the times indicated with a single doses of C-CAM (a), M-CAM (b), $beta$ -CNA (c), and $beta$ -FNA 32 (d). A temperature of 55°C was used with a cutoff time of 15 s. Each point represents the mean ± S.E. of the tail withdrawal latency for five mice.

The selectivity of C-CAM, M-CAM, $beta$ -CNA, and $beta$ -FNA for µ-, $kappa$ -, and $delta$ -opioid receptors was assessed in the writhing assay againstthe agonists morphine, bremazocine, and BW373U86, respectively.Morphine dose-dependently suppressed writhing behavior with anED₅₀ of 0.55 mg/kg s.c. (Table 1). C-CAM, M-CAM, $beta$ -FNA, and $beta$ -CNAproduced parallel, dose-dependent rightward shifts in the morphinedose-response curve, although they did so with somewhat differentpotencies in the order M-CAM

C-CAM > $beta$ -CNA $>=$ $beta$ -FNA (Table 1).For instance, a dose of 3.2 mg/kg M-CAM produced a 218-fold increasein the ED₅₀ for morphine, whereas the same dose of C-CAM resultedin only a 9.5-fold increase. In turn, C-CAM (32 mg/kg) was morepotent as an antagonist, causing a 68-fold increase in the ED₅₀for morphine than the same doses of $beta$ -CNA (22-fold increase) and $beta$ -FNA (11.5-fold increase). However, this difference may relateto the different pretreatment times of the antagonists used. A1-h pretreatment time was used for C-CAM and M-CAM, but a 24-hpretreatment time was necessary for both $beta$ -CNA and $beta$ -FNA to avoidthe confounding agonist effects of these compounds. A lower dose(3.2 mg/kg) of $beta$ -FNA neither showed an agonist effect nor antagonizedmorphine. As an alternative to overcome the initial, predominantly $kappa$ -mediated agonist effects of $beta$ -FNA, mice were pretreated withnor-BNI (32 mg/kg i.p., 24-h pretreatment). Under these conditions, $beta$ -FNA (32 mg/kg; 1-h pretreatment) produced a 35-fold shift inthe morphine dose-effect curve, resulting in an ED₅₀ for morphineof 19.1 mg/kg (confidence limits 15.1-24.2): that is three timesthe ED₅₀ measured 24 h after the same dose of $beta$ -FNA in the absenceof nor-BNI pretreatment.

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TABLE 1
Potencies of morphine (µ), bremazocine ( $kappa$ ), and BW373U86 ( $delta$ ) in the mouse acetic acid-induced writhing assay and their antagonism by C-CAM, M-CAM, $beta$ -FNA, and $beta$ -CNA
Experiments were performed as described under Material and Methods. ED₅₀ values represent the mean obtained by linear regression from a dose-effect curve of at least three concentrations of agonist. Values in parentheses represent the 95% confidence limits.

There was no evidence of suppression of the maximal response to morphine in the writhing assay, as shown for M-CAM (Fig. 4).Morphine has agonist actions at $kappa$ -receptors in vitro (Toll etal., 1998

). To examine whether the response of morphine in thepresence of µ-receptor blockade was mediated by $kappa$ -receptors, theeffect of morphine was reexamined in the presence of M-CAM aftera 24-h pretreatment with 32 mg/kg i.p. nor-BNI. This pretreatmentwith nor-BNI did not significantly shift the dose-effect curvefor morphine alone but shifted the ED₅₀ for morphine in the presenceof M-CAM by 6.9-fold (Fig. 4). This suggested the response tomorphine observed in the presence of µ-receptor blockade by M-CAMwas mediated through a $kappa$ -receptor mechanism.

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Fig. 4. Antinociceptive effect of morphine in the writhing assay in the absence or presence of M-CAM (1.8 mg/kg, 1 h earlier) in mice pretreated 24 h previously with vehicle (closed symbols) or nor-BNI (32 mg/kg; open symbols). Each point represents the mean ± S.E. of the writhing activity of six mice relative to sterile water controls.

Antagonism by C-CAM, M-CAM, $beta$ -FNA, and $beta$ -CNA of $kappa$ - and $delta$ -mediated antinociception was also evaluated. Bremazocine, a $kappa$ -selectiveagonist in this assay (Broadbear et al., 1994

; ED₅₀ = 0.012 mg/kg),was 40 times more potent than morphine in suppressing acetic acid-inducedwrithing in the mouse, whereas the $delta$ -selective agonist BW373U86(ED₅₀ = 2.8 mg/kg) was 5-fold weaker (Table 1). Pretreatmentwith 10 mg/kg M-CAM or 32 mg/kg C-CAM produced significant, andapproximately equipotent, antagonism of the effects of both agonists(Table 1). However, with both C-CAM and M-CAM, the magnitudeof the increases in agonist ED₅₀ was smaller for the $kappa$ - and $delta$ -agoniststhan for the µ-agonist morphine. This was especially true forM-CAM, which at a dose of 1.8 mg/kg produced a 74-fold increasein the ED₅₀ of morphine but was without significant effect atthis dose in blocking bremazocine- or BW373U86-induced antinociception(Table 1). In contrast, $beta$ -FNA was ineffective at antagonizingthe $delta$ -selective agonist, even at a dose of 32 mg/kg, and at thisdose shifted only the dose-effect curve for bremazocine by 2-fold,clearly showing a preference for antagonism of morphine-mediatedantinociception. $beta$ -CNA produced similar shifts in the dose-effectcurves of morphine, bremazocine, and BW373U86 (Table 1).

Ligand-Binding Assays

In mouse brain homogenates, $beta$ -FNA and $beta$ -CNA as well as C-CAM and M-CAM had nanomolar affinity for all three opioid receptors,with limited selectivity for the µ-receptor. In the case of C-CAMand M-CAM, receptor preference was in the order µ > $delta$ > $kappa$ , althoughthe differences were not very pronounced. In contrast, $beta$ -FNA and $beta$ -CNA had similar affinity for µ- and $kappa$ -receptors but much reducedaffinity for the $delta$ -receptor (Table 2).

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TABLE 2
Affinities (apparent K_i) of C-CAM, M-CAM, $beta$ -FNA, and $beta$ -CNA for µ-, $delta$ -, and $kappa$ -receptors in mouse brain homogenates
Values were obtained from displacement curves against 0.5 nM [³H]DAMGO (µ), 1.5 nM [³H]U69,593 ( $kappa$ ), and 1.5 nM [³H]DPDPE ( $delta$ ) as described under Materials and Methods. Values represent the means ± S.E. of at least three experiments.

To study opioid binding ex vivo, mice were injected with M-CAM (1.8 mg/kg s.c.) 1 h before the removal of brains and preparationof homogenates. At radioligand concentrations approximating theiraffinities, the specific binding of [³H]DAMGO was reduced by 76% in washed brain homogenates from M-CAM-treatedanimals compared with saline-treated controls, but the bindingof [³H]DPDPE and [³H]U69593 was unchanged (Fig. 5). In experiments using nonwashed,crude homogenates in which the mice brains were simply homogenizedin 100 ml Tris-HCl buffer/75 mg brain tissue, the binding of [³H]DAMGO was reduced by 72.0 ± 17.5%, [³H]DPDPE was reduced by 25.0 ± 5.1%, and [³H]bremazocine (in the presence of µ- and $delta$ -receptor blockade)was reduced by 14.6 ± 2.6% compared with saline-treated controls.

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Fig. 5. Binding of [³H]DAMGO (µ, 1.6 nM), [³H]DPDPE ( $delta$ , 2.6 nM), and [³H]bremazocine ( $kappa$ , 1 nM in the presence of 1 µM DAMGO and 1 µM DPDPE to block binding to µ- and $delta$ - receptors) to homogenates of brains from mice pretreated 1 h before sacrifice with M-CAM (1.8 mg/kg s.c.) (hatched columns) or sterile water (open columns). *, significantly different from binding in brain homogenates from control mice (P < .002).

[³⁵S]GTP $gamma$ S Assays

At a concentration as high as 1 µM, M-CAM caused only a 7.2 ± 1.9% (n = 3) stimulation of [³⁵S]GTP $gamma$ binding at $kappa$ -opioid receptors expressed in CHO cells comparedwith the full agonist U69593 and a 12.7 ± 1.9% (n = 5) stimulationat µ-opioid receptors in C6 cells compared with the full µ-agonistfentanyl. These very low levels of stimulation of [³⁵S]GTP $gamma$ S binding, at concentrations many times greater than thebinding affinity of the compounds, do not lead to agonist effectsin in vitro or in vivo preparations (Traynor et al., 1999). At $delta$ -opioid receptors expressed in C6 cells, M-CAM did not stimulate[³⁵S]GTP $gamma$ Sbinding.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The aim of this work was to determine whether cinnamoylamidomorphinans such as C-CAM and M-CAM are functionally superior to $beta$ -FNA and $beta$ -CNA for blocking the µ-opioid receptor population,thereby allowing study of the physiological and pharmacologicalroles of thisreceptor.

The order of potency of the long-lasting antagonists in preventing morphine antinociception in the writhing assay and thetail-withdrawal assay was M-CAM > C-CAM > $beta$ -CNA > $beta$ -FNA. The warm-watertail-withdrawal assay cannot be used to accurately assess antagonistpotency because these agents caused a flattening of the morphinedose-effect curve, nor can the assay be used to test ligand selectivitybecause systemically administered $kappa$ - and $delta$ -selective agonistsgenerally have no antinociceptive efficacy in thermal assays (Hayeset al., 1985; Mjanger and Yaksh, 1991). In the writhing assay,however, both selectivity and antagonist potency can be determined.In the writhing assay, $beta$ -FNA showed a selective antagonism ofthe µ-receptor as expected (Takemori et al., 1981; Ward et al.,1982b). This contrasted with its binding profile, which indicateda lack of selectivity between µ- and $kappa$ -receptors. However, thisis not important in governing its antagonist selectivity in vivobecause interaction with the $kappa$ -receptor results in agonism andis reversible. In contrast, $beta$ -CNA was nonselective, producingcomparable shifts in the dose-effect curves of morphine, bremazocine,and BW373U86, in agreement with its profile in bindingassays.

C-CAM and M-CAM showed preference for µ-antagonism and were weaker but equipotent as $kappa$ - and $delta$ -antagonists. M-CAM in particularshowed a striking selectivity for µ-receptors. The selectivityand antagonist potency difference between M-CAM and C-CAM werenot expected due to the very close similarity in the structureof these compounds. Nevertheless, compounds in this series doshow very marked pharmacological variations with only small structuralchanges (Nieland et al., 1995), suggesting very subtle interactionsof the cinnamoylamido substituent with the receptor binding domain.The finding of a marked in vivo selectivity of M-CAM also contrastswith the in vitro binding data in which only a 3.7-fold selectivityof M-CAM for µ- over $delta$ -receptors and an 8-fold selectivity forµ- over $kappa$ -receptors were evident. This difference is perplexing,but there is evidence that different measures of antagonist affinitydo not always coincide with effects seen in pharmacological assays,especially when binding assays are performed in low ionic strengthTris-HCl buffer rather than in physiological medium. For example,the µ-antagonist cyprodime shows very different affinities for $kappa$ - and $delta$ -receptors in binding assays than are apparent from pharmacologicalmeasures of its affinity (Schmidhammer et al., 1995). Furthermore,the pseudoirreversible nature of the binding that occurs in vivoprovides a second recognition step that is likely to enhance selectivity(Takemori and Portoghese, 1985). Importantly, the in vivo findingswere confirmed by ex vivo binding showing that the majority ofµ-opioid binding of [³H]DAMGO was lost after the pretreatment of mice for 1 h with M-CAM,whereas no loss of $delta$ - or $kappa$ -binding was seen. In nonwashed membranes,there was some inhibition of $delta$ - and $kappa$ -binding, suggesting a reversibleinteraction with these receptors. The cinnamoylamidomorphinansdo not alkylate the µ-receptor (Zernig et al., 1995b; McLaughlinet al., 1999), so these results confirm that very high-affinity,pseudoirreversible binding develops rapidly in vivo at the µ-receptor(Piggot et al., 1995) but not at $delta$ - or $kappa$ -receptors. This is consistentwith the resistance of C-CAM binding to extensive washing (Zerniget al., 1996).

The large, insurmountable shift caused by the antagonists in the morphine dose-effect curve in the warm-water tail-withdrawalassay and their long duration of action are further evidence thattheir interaction with the µ-opioid receptor occurs through anonequilibrium mechanism (Kenakin, 1997). In contrast, in thewrithing assay, antagonism was surmountable. The inability ofa nonequilibrium antagonist to depress agonist dose-effect curvesunder some experimental conditions has been reported previouslyusing $beta$ -FNA (Takemori et al., 1981; Ward et al., 1982b). Morphineis 30 times more potent in the writhing assay than in the tail-withdrawalassay, implying that fewer receptors have to be occupied to reachfull antinociception in the former assay, so there is a greaterµ-receptor reserve. Thus, with a reduction in the total numberof available µ-receptors, there may still be a sufficient numberremaining for a maximal response to be reached. However, it isalso feasible that with a large fraction of the µ-receptor populationblocked by antagonist, morphine can act through non-µ-opioid receptors.The present results show that when µ-receptors are depleted withM-CAM, morphine exerts its antinociceptive action through $kappa$ -receptors.A study in µ-receptor-deficient transgenic mice has suggestedthat the antinociceptive effect of low doses of morphine (up to6 mg/kg) is mediated only through µ-receptors (Matthes et al.,1996). That study used heat as the nociceptive source in the hot-plateand tail-withdrawal assays. As discussed earlier, these are likelyto be µ-selective assays, so any $kappa$ -effects of morphine would notbe apparent. In support of the present finding, morphine is knownto act through the $kappa$ -receptor in vitro in the presence of $beta$ -FNA(Ward et al., 1982a; Franklin and Traynor, 1991), and Takemoriand Portoghese (1987) showed that the agonist effects of morphinein $beta$ -FNA-treated mice are mediated by $kappa$ -opioid receptors in themouse writhingassay.

Agonist activity in a compound that is used for its antagonist properties may be a complicating factor. No agonist activitywas evident even with high doses of M-CAM or C-CAM, a findingconfirmed for M-CAM in the [³⁵S]GTP $gamma$ S assay at cloned opioid receptors. On the other hand, $beta$ -CNAand $beta$ -FNA were fully effective antinociceptive agents in the mousewrithing assay through a nor-BNI-sensitive $kappa$ -receptor mechanism,as reported previously (Takemori et al., 1981; Ward et al., 1982b),and in CHO-hkor cells, $beta$ -FNA shows partial $kappa$ -agonist activity(Zhu et al., 1997; Toll et al., 1998). Antinociception with $beta$ -FNAand $beta$ -CNA in the writhing assay was observed at doses that producedpotent antagonism of morphine at later time points. Furthermore,it is clear that both the agonist and antagonist effects of $beta$ -CNAand $beta$ -FNA occurred simultaneously as both compounds potently antagonizedmorphine 1 h after administration in the tail-withdrawal assay,a time at which they had pronounced agonist effects in the writhingassay. Because of such agonist effects, these compounds are generallygiven as a 24-h pretreatment (Zimmerman et al., 1987; Mjangerand Yaksh, 1991; Ward et al., 1992b; Martin et al., 1995).

Bidlack and colleagues have reported on compounds related to C-CAM and M-CAM that contain the 14 $beta$ -(p-nitrocinnamoylamido)group, including the metapon derivative 5 $beta$ -methyl-14 $beta$ -(p-nitrocinnamoylamino)-7,8-dihydromorphinoneand its N-cyclopropylmethyl counterpart N-cyclopropylmethylnor-5 $beta$ -methyl-14 $beta$ -(p-nitrocinnamoylamino)-7,8-dihydromorphinone(Jiang et al., 1994; McLaughlin et al., 1999). The compounds,particularly the N-methyl derivative, are selective for the µ-opioidreceptor. They show no agonist activity when given i.c.v. to themouse using the tail-flick assay but do show long-lasting antagonism.The lack of agonism is surprising given the agonist efficacy ofmetapon, but unfortunately, the compounds have not been studiedin the writhing assay, which requires much less efficacy in acompound for the manifestation of antinociception. However, takentogether, these findings suggest that this class of substituted14-aminomorphinones is devoid of agonist properties and so representssuperior long-lasting µ-opioid receptorantagonists.

In summary, M-CAM and, to a lesser extent, C-CAM have antagonist activity selectively at the µ-opioid receptor and show noevidence of any agonist activity in nociceptive tests. In contrast,both $beta$ -CNA and $beta$ -FNA have potent antinociceptive activity in thewrithing assay at doses and pretreatment times that coincide withthose that are optimal for utilization of their nonequilibriumantagonist properties. M-CAM and C-CAM are nonselective in bindingassays, suggesting an interaction in vivo that results in theformation of a high-affinity, nonwashable interaction selectivelywith the µ-receptor. The superior selectivity of M-CAM suggeststhis to be the nonequilibrium antagonist of choice for the long-termblockade of µ-opioid receptors invivo.

	Footnotes

Accepted for publication May 8, 2000.

Received for publication February 21, 2000.

¹ This work was supported by United States Public Health Service Grant DA-00254.

² Present address: Astra Merck, 3838 N. Causeway Blvd., Lakeway III, Ste. 2400, Metairie, LA70002.

³ Present address: Department of Pharmacy and Pharmacology, University of Bath, Bath BA2 7AY,UK.

Send reprint requests to: Dr. J. R. Traynor, Department of Pharmacology, University of Michigan Medical School, 1301, MSRBIII, Ann Arbor, MI 48109-0632. E-mail: jtraynor{at}umich.edu

	Abbreviations

$beta$ -CNA, $beta$ -chlornaltrexamine; $beta$ -FNA, $beta$ -funaltrexamine; C-CAM, clocinnamox; DAMGO, [D-Ala²,N-Me-Phe⁴,Gly⁵-ol]-enkephalin; DPDPE, [D-Pen²,D-Pen⁵]-enkephalin; M-CAM, methocinnamox; MM-CAM, 3-methoxymethocinnamox; nor-BNI, norbinaltorphimine; NTI, naltrindole.

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Methocinnamox Is a Potent, Long-Lasting, and Selective Antagonist of Morphine-Mediated Antinociception in the Mouse: Comparison with Clocinnamox, $beta$ -Funaltrexamine, and $beta$ -Chlornaltrexamine¹