Antinociceptive Profile of 3-alpha -tropanyl-(2-Cl)-acid phenoxybutyrate (SM-21): A Novel Analgesic with a Presynaptic Cholinergic Mechanism of Action

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Vol. 282, Issue 1, 430-439, 1997

Antinociceptive Profile of 3- $alpha$ -tropanyl-(2-Cl)-acid phenoxybutyrate (SM-21): A Novel Analgesic with a Presynaptic Cholinergic Mechanism of Action¹

Carla Ghelardini, Nicoletta Galeotti, Fulvio Gualtieri, Cristina Bellucci, Dina Manetti, Alberto Giotti , Petra Malmberg-Aiello, Alessandro Galli and Alessandro Bartolini

Department of Pharmacology (C.G., N.G., A.G., P.M.A., A.G., A.B.), University of Florence and Department of Pharmaceutical Sciences (F.G., C.B., D.M.), University of Florence, Florence, Italy

	Abstract

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The antinociceptive effect of (±)-3- $alpha$ -tropanyl-(2-Cl)-acid phenoxybutyrate (SM-21) (10-40 mg kg¹ s.c., 10-30 mg kg¹ i.p., 20-60 mg kg¹ p.o., 3-20 mg kg¹ i.v. and 5-20 µg per mouse i.c.v.) was examined in rodents andguinea pigs by using the hot-plate, abdominal constriction, tail-flickand paw-pressure tests. The antinociception produced by (±)-SM-21was prevented by atropine, pirenzepine and hemicholinium-3 butnot by quinpirole, R-( $alpha$ )-methylhistamine, [1-[2(methylsufonyl)amino]ethyl]-4-piperidinyl]methyl-5-floro-2-methoxy-1H-indole-3-carboxylatehydrochloride, N⁶-cyclopentyladenosine, 1-(2-methoxyphenyl)-4-[4-(2-phthalimido)butyl]piperazinehydrobromide, naloxone, 3-aminopropyl-diethoxy-methyl-phosphinicacid or reserpine. On the basis of the above data, it can be postulatedthat (±)-SM-21 exerted an antinociceptive effect mediated by acentral potentiation of cholinergic transmission. Affinity profilesof (±)-SM-21 for muscarinic receptor subtypes, determined by functionalstudies (rabbit vas deferens for M₁, guinea pig atrium for M₂,guinea pig ileum for M₃ and immature guinea pig uterus for putativeM₄) have shown a selectivity ratio M₂/M₁ of 4.6 that, althoughvery low, might be responsible for the antinociception inducedby (±)-SM-21 through an increase in ACh extracellular levels.In the antinociceptive dose range, (±)-SM-21 did not impair mouseperformance evaluated by the rota-rod and hole-board tests.

	Introduction

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Ghelardini et al. (1990) have reported that the antimuscarinic compound atropine, at very low doses, was able to induce acentral cholinergic antinociception in rodents regardless of theroute of administration and the noxious stimulus applied. Furthermore,this antinociceptive activity was not accompanied by the typicalcholinergic symptomatology. The atropine-induced increase in thepain threshold was attributable to the R-(+)-enantiomer of atropine,R-(+)-hyoscyamine, because S-( $-$ )-hyoscyamine was ineffective inall antinociceptive tests used (Ghelardini et al., 1992). Morerecently, Bartolini et al. (1994), investigating the antinociceptiveeffect of atropine, demonstrated, using microdialysis techniques,that R-(+)-hyoscyamine, at analgesic doses, produced an increasein the release of ACh from the rat cerebral cortex in vivo. Onthe bases of the above-mentioned results, the racemate (Gualtieriet al., 1994) and the enantiomers (Romanelli et al., 1995) ofthe compound labeled SM-21 (fig. 1), which is structurally relatedto atropine, have been synthesized in order to obtain a new cholinergicamplifier endowed with more intensive antinociceptive activitythan atropine but as lacking as atropine in cholinergic side effects.To this end, we investigated (±)-SM-21 antinociceptive propertiesby using the hot-plate, abdominal constriction, paw-pressure andtail-flick tests, and the incidence of behavioral side effectswas detected by the rota-rod and hole-board tests.

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Fig. 1. Chemical structure of SM-21 racemate and its enantiomers.

	Materials and Methods

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Animals. Male Swiss albino mice (23-30 g), Wistar rats (200-300 g) from Morini (San Polo d'Enza, Italy), Fisher 344 rats (200-300)from Charles River (Calco, Italy) and guinea pigs (150-200 g)from Rodentia (Bergamo, Italy) breeding farms were used. Fifteenmice and four rats or guinea pigs were housed per cage. The cageswere placed in the experimental room 24 h before the test foracclimatization. The animals were kept at 23 ± 1°C with a 12-hlight/dark cycle, light on at 7 A.M., with food and water ad libitum.All experiments were carried out according to the guidelines ofthe European Community Council.

Analgesic Tests

Hot-plate test. The method adopted was described by O'Callaghan and Holtzman (1975). Mice were placed inside a stainless steel container thermostaticallyset at 52.5 ± 0.1°C in a precision water bath from KW MechanicalWorkshop, Siena, Italy. Reaction times (s), were measured witha stopwatch before treatment and at regular intervals up to amaximum of 60 min after treatment. The endpoint used was the lickingof the fore or hind paws. Those mice scoring below 12 and over18 s in the pretest were rejected (30%). An arbitrary cut-offtime of 45 s was adopted.

Abdominal constriction test. Mice were injected i.p. with a 0.6% solution of acetic acid (10 ml kg¹), according to Koster et al. (1959). The number of stretchingmovements was counted for 10 min, starting 5 min after aceticacid injection.

Paw-pressure test. The nociceptive threshold in the rat and guinea-pig was determined with an analgesimeter (Ugo Basile, Varese, Italy), accordingto the method described by Leighton et al. (1988). Threshold pressurewas measured before treatment and 15, 30 and 45 min after treatment.Rats and guinea-pigs scoring below 30 g or over 85 g during thetest before drug administration were rejected (25%). An arbitrarycutoff value of 250 g was adopted.

Tail-flick test. An analgesimeter from Ugo Basile (Varese, Italy) was used to perform the tail-flick test described by D'Amour and Smith (1941).The light from a project bulb situated beneath the platform wherethe animal was placed was focused through a small hole on theventral part of the tail at a point about 4 cm from the tip. Withdrawalof the tail exposed a photocell to the light, which turned offthe thermal stimulus and automatically stopped the clock. Theintensity was regulated so that the reaction time varied between2 and 4 s. The analgesia was tested before treatment and 15, 30and 45 min after treatment. Each value was derived from the meanof three consecutive readings in which the light was focused onthree adjacent points of the tail.

Anti-inflammatory Test

Carrageenan-induced paw edema. Rats paw volumes were measured using a plethysmometer (Ugo Basile, Varese, Italy). Rats received (±)-SM 21, indomethacin orsaline 90 min after a 0.1-ml injection of 0.5% carrageenan inthe right hind paw. Two hours after the injection of carrageenan,the paw volume of the right hind paw was measured and comparedwith saline-treated controls.

Additional Behavioural Tests

Hole-board test. The hole-board test consists of a 40-cm-square plane with 16 flush-mounted cylindrical holes (diameter 3 cm) distributed 4by 4 in an equidistant, grid-like manner. Mice were placed onthe center of the board one by one and left to move about freelyfor a period of 10 min each. Two electric eyes, crossing the planefrom midpoint to midpoint of opposite sides, thus dividing theplane into 4 equal quadrants, automatically signaled the movementof the animals on the surface of the plane. Miniature photoelectriccells in each of the 16 holes recorded the exploration of theholes (head plunging activity) by the mice.

Rota-rod test. The apparatus consisted of a base platform and a rotating rod 3 cm in diameter with a nonslippery surface. The rod was placedat a height of 15 cm from the base. The rod, 30 cm in length,was divided into 5 equal sections by 6 disks. Thus up to 5 micewere tested simultaneously on the apparatus, with a rod-rotatingspeed of 16 rpm. The integrity of motor coordination was assessedon the basis of the number of falls from the rod in 30 s accordingto Vaught et al. (1985). The performance time was measured beforetreatment and 15, 30 and 45 min after treatment.

In Vitro Functional Studies

Isolated rabbit vas deferens. Experiments on isolated rabbit vas deferens were performed according to the method described by Eltze (1988) and modifiedby Dei et al. (1995). The preparations were maintained at 32°C,and tissues were stimulated through platinum electrodes by square-wavepulses (2 ms, 0.1 Hz, 10-30 V). Contractions were measured isometricallyafter tissues had been equilibrated for 1 h, and then a cumulativedose-response curve for the inhibitory effect of McN-A-343 wasplotted.

Isolated guinea pig left atria. Isolated left atria were prepared according to the method described by Eltze et al. (1985) and modified by Dei et al. (1995).Bath fluid temperature was maintained at 30°C. Atria were electricallystimulated (1 Hz, 1 ms, 4-10 V) by means of two platinum electrodes.Carbachol negative inotropic effects on isometric atria contractionswere recorded before and 1 h after perfusion with antagonists.

Guinea pig isolated ileum. Isolated ileum fragments were prepared according to Eltze and Figala (1988). Bath fluid temperature was maintained at 37°C.Isotonic ileum contractions induced by ACh were recorded beforeand 1 h after perfusion with antagonists.

Guinea pig isolated uterus. Experiments on isolated immature guinea pig uterus were performed according to Dörje et al. (1990). The preparations weremaintained at 30°C, and after a 1-h equilibration period, isotoniccontractions to carbachol were recorded. Initially the tissueswere exposed to a single-concentration of carbachol (3 nmol l¹) to check the responsiveness to the agonist, and a dose-responsecurve for carbachol was obtained.

Determination of antagonist affinities. After a stabilization time of 30 to 60 min, agonist concentration-response curves were plotted before and after equilibrationwith antagonists. In separate control experiments, no significantchanges in tissue sensitivity to the agonist were observed overthe period required for the determination of two concentration-responsecurves. The antagonists were allowed to equilibrate for 60 min.No more than two concentrations of antagonist were tested in thesame preparation. Agonist EC₅₀ values in the absence and presenceof antagonists were determined graphically for the calculationof dose ratios.

AChE activity. AChE activity was assayed according to Ellman et al. (1961), using 0.5 mM acetylthiocholine iodide as substrate. The (±)-SM-21inhibitory effect was tested at various concentrations on a purifiedpreparation of AChE from the electric eel.

Drugs. SM-21 racemate was prepared according to Gualtieri et al. (1994); R-(+)-SM-21 and S-( $-$ )-SM-21 were prepared according to Romanelliet al. (1995); R-(+)-hyoscyamine was prepared according to Gualtieriet al. (1991). Also used were altropine sulfate, carbamylcholinechloride, carrageenan, physostigmine hemisulfate and yohimbinehydrochloride (Sigma, Milan, Italy), HC-3, pirenzepine dihydrochloride,naloxone hydrochloride, quinpirole hydrochloride, (R)- $alpha$ -methylhistaminedihydrochloride, indomethacin, N⁶-cyclopentyladenosine, NAN 190, McN-A-343 (R.B.I., Milan, Italy);ACh chloride (Merck, Florence, Italy); GR 125487 (Boehringer Ingelheim,Milan, Italy); morphine hydrochloride (U.S.L. 10/D, Florence,Italy), diphenhydramine hydrochloride and AFDX-116 (De Angeli,Milan, Italy); clomipramine hydrochloride (anafranil), CGP 35348and reserpine (Ciba Geigy, Basel, Switzerland); (+)-amphetaminesulfate (Recordati, Rome, Italy). Other chemicals were of thehighest quality commercially available. All drugs were dissolvedin isotonic (NaCl 0.9%) saline solution or dispersed in sodiumcarboxymethylcellulose 1% immediately before use, except reserpine,which was dissolved in a 20% solution of ascorbic acid, and R-(+)-hyoscyamine,which was dissolved in 0.1 M HCl and then diluted with saline(1:10). Drug concentrations were prepared in such a way that thenecessary dose could be administered in a volume of 10 ml kg¹ by s.c., i.p., and p.o. route or 5 ml kg¹ by i.v. route. Intracerebroventricular administration was performedunder ether anaesthesia using isotonic saline as solvent, accordingto the method described by Haley and McCormick (1957) for miceand that we adapted for rats. Briefly, during anaesthesia, miceand rats were grasped firmly by the loose skin behind the head.A hypodermic needle 0.4 mm in external diameter, attached to a10-µl syringe, was inserted perpendicularly through the skullat a depth of no more than 2 mm into the brain of the mouse and4 mm into the brain of the rat, where 5 µl (mice) or 10 µl (rats)were then administered. The injection site was 1.5 mm (mice) or2.5 mm (rats) from either side of the midline on a line drawnthrough to the anterior base of the ears. To ensure that the drugswere administered exactly into the cerebral ventricle, some miceand rats were injected i.c.v. with 5 to 10 µl of diluted 1:10Indian ink and their brains examined macroscopically after sectioning.Intraplantar injections of carrageenan were performed by injecting100 µl of a suspension in sterile saline solution of 0.5% carrageenanin the rat hind paw.

Statistical analysis. Results are given as the mean ± S.E.M.; analysis of variance (ANOVA), followed by Fisher's PLSD procedure for post-hoc comparison,was used to verify the significance of the difference betweentwo means. P values of less than .05 were considered significant.Data were analyzed with the StatView for the Macintosh computerprogram (1992).

	Results

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Antinociceptive activity of SM-21. (±)-SM-21, as shown in figure 2, produced a dose-dependent increase in the pain threshold in the mouse hot-plate test afters.c. (10-40 mg kg¹; panel A), i.c.v. (5-20 µg per mouse; panel B), p.o. (20-60 mgkg¹; panel C) and i.v. (3-20 mg kg¹; panel D) administration. The antinociceptive effect of (±)-SM-21peaked 15 min after s.c. and i.c.v. administration and then slowlydiminished. (±)-SM-21, after p.o. and i.v. administration, reachedits maximum analgesic effect respectively 30 and 10 min afterinjection. Figure 3 (panels A and B) illustrates the analgesiceffect of (±)-SM-21 in the mouse acetic acid abdominal constrictiontest. (±)-SM-21 induced an increase in the pain threshold in adose-dependent manner starting from the dose of 10 mg kg¹ s.c. (fig. 3, panel A). (±)-SM-21 showed antinociceptive propertiesalso after the injection of 1 and 5 µg per mouse i.c.v., reachingits maximum effect between 15 and 30 min after administration(fig. 3, panel B).

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Fig. 2. Dose-response curves of (±)-SM-21 administered s.c. (panel A), i.c.v. (panel B), p.o. (panel C) and i.v. (panel D) in themouse hot-plate test. The doses are expressed as mg kg¹ s.c., p.o. and i.v. and as µg per mouse i.c.v. Vertical linesshow S.E.M. P < .05; * P < .01 in comparison with saline controls. Each pointrepresents the mean of at least 10 mice.

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Fig. 3. A) Dose-response curves of (±)-SM-21 administered s.c. and effect of both HC-3 (1 µg per mouse i.c.v.) and reserpine (2 mgkg¹ i.p.) pretreatments on antinociception induced by (±)-SM-21 (10mg kg¹ s.c.) in the mouse abdominal constriction test induced by aceticacid 0.6%. The nociceptive responses were recorded 15 min after(±)-SM-21 administration. HC-3 was injected 5 h and reserpine48 and 24 h before testing. (B) Time course of (±)-SM-21 administeredi.c.v. The nociceptive responses were recorded 15, 30, 45 and60 min after (±)-SM-21 administration. Vertical lines show S.E.M. P < .05; * P < .01 in comparison with saline controls. ° P <.01 in comparison with (±)-SM-21 (10 mg kg¹ s.c.). Numbers inside the columns indicate the number of mice.

(±)-SM-21 was able to produce an increase in the pain threshold not only in mice but also in rats and guinea pigs. In thepaw pressure test (±)-SM-21 administered i.p. at the dose of 20-30mg kg¹ in the rat, and 20 mg kg¹ in guinea pigs, induced antinociception starting 15 min afterinjection, reaching a maximum after 30 min and persisting up to45 min (table 1). The analgesic profile of (±)-SM-21 was alsoinvestigated in Wistar and Fisher 344 rat strains by using thetail flick test (fig. 4). In both rat strains used (±)-SM-21 exhibiteda similar antinociceptive activity 30 min after i.p. injectionof 20-30 mg kg¹ (fig. 4).

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TABLE 1
Antinociception exerted by (±)-SM-21 in the paw-pressure test: in the rat (A) and in the guinea pig (B) and antagonism byatropine and HC-3 on (±)-SM-21 antinociception in the rat

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Fig. 4. Antinociceptive effect of (±)-SM-21 in the rat tail-flick test. Nociceptive responses were recorded 30 min after drug administration.Vertical lines show S.E.M. * P < .01 in comparison with salinecontrols. Numbers inside the columns indicate the number of mice.

The analgesic effect of the two enantiomers of (±)-SM-21, R-(+)-SM-21 and S-( $-$ )-SM-21, was evaluated in the mouse hot-platetest (fig. 5, panels A and C) and in the acetic acid abdominalconstriction test (fig. 5, panels B and D). Both enantiomers dose-dependentlywere able to increase the pain threshold, even if R-(+)-SM-21was slightly more effective than S-( $-$ )-SM-21.

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Fig. 5. Dose-response curves of R-(+)-SM-21 (panels A and C) and S-( $-$ )-SM-21 (panels B and D) in the mouse hot-plate test and abdominalconstriction test. The doses are expressed as mg kg¹ s.c. Vertical lines show S.E.M. P < .05; * P < .01 in comparison with saline controls. Numbersinside the columns are the number of mice.

The areas under the curve of the antinociception induced by (±)-SM-21 (30 mg kg¹ i.p.), R-(+)-hyoscyamine (5 µg kg¹ i.p.), morphine (8 mg kg¹ i.p.), diphenhydramine (20 mg kg¹ i.p.) and clomipramine (25 mg kg¹ i.p.) are reported in figure 6. The doses of the analgesic drugschosen were the highest that did not impair rota-rod performance.

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Fig. 6. Area under the curve of the analgesic effect of (±)-SM-21 in comparison with R-(+)-hyoscyamine, morphine, diphenhydramineand clomipramine in hot-plate test. The nociceptive responseswere recorded from 15 min after drug injection to 90 min afterdrug administration. Numbers inside the columns indicate the numberof mice.

The potentiating effect on antinociception exerted by non-analgesic doses of physostigmine (0.05 mg kg¹ i.p.) on AFDX-116 (6.3 ng per mouse i.c.v.) and R-(+)-hyoscyamine(5 µg kg¹ s.c.) in the mouse hot-plate test is illustrated in table 2.In the same experimental conditions physostigmine was not ableto potentiate (±)-SM-21 (30 mg kg¹ i.p.) antinociception (Table 2).

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TABLE 2
Effect of physostigmine on (±)-SM-21, AFDX-116 and R-(+)-hyoscyamine antinociception in the mouse hot-plate test

Antagonism of the (±)-SM-21 induced antinociception. In the mouse hot-plate test, the antinociceptive effect of (±)-SM-21 (30 mg kg¹ s.c.) was not antagonized by naloxone (1 mg kg¹ i.p.), CGP-35348 (2.5 µg per mouse i.c.v.), (R)- $alpha$ -methylhistamine(10 mg kg¹ i.p.), quinpirole (0.1 mg kg¹ i.p.), GR-48125 (20 mg kg¹ i.p.), N⁶-cyclopentyladenosine (5 µg per mouse i.c.v.), NAN 190 (0.5 µgper mouse i.c.v.) (table 3) and, in the abdominal constrictiontest, by reserpine (2 mg kg¹ i.p.) (fig. 3). Conversely, atropine (5 mg kg¹ i.p.), pirenzepine (0.1 µg per mouse i.c.v.) and hemicolinium-3(1 µg per mouse or rat i.c.v.) were able to completely prevent(±)-SM-21 antinociception in the mouse hot-plate (table 3), abdominalconstriction (fig. 3) and the rat paw-pressure tests (table 1).All antagonists were injected 15 min before (±)-SM-21, with theexception of reserpine, injected twice 48 and 24 h before thetest, N⁶-cyclopentyladenosine, administered simultaneously with (±)-SM-21and CGP 35348, injected 5 min before (±)-SM-21.

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TABLE 3
Effects of atropine, pirenzepine, HC-3, naloxone, CGP-35348, RAMH, quinpirole, GR-48125, N⁶-cyclopentyladenosine and NAN-190 on antinociception induced by(±)-SM-21 in the mouse hot-plate test

Evaluation of the (±)-SM-21 effect in the carrageenan-induced paw edema test. (±)-SM-21 failed to suppress paw edema in response to carrageenan administration at the dose of 20 and 30 mg kg¹ i.p. The positive control, indomethacin at the dose of 1 mg kg¹ i.p., produced a significant inhibition over saline + carrageenantreated control animals (data not shown).

Evaluation of the SM-21 effect on spontaneous activity and motor coordination. The motor coordination of mice treated with (±)-SM-21, R-(+)-SM-21 and S-( $-$ )-SM-21 was evaluated by using the rota-rod test(table 4) while their spontaneous activity was investigated byusing the hole-board test. The rota-rod performance of mice treatedwith (±)-SM-21 at the dose of 30 and 40 mg kg¹ s.c. and both enantiomers at the dose of 20 and 30 mg kg¹ s.c. was not impaired in comparison with controls (table 4).On the contrary, (±)-SM-21 administered at higher doses (50 and60 mg kg¹ s.c.) produced a significant impairment of the rota-rod performance(table 4). The number of falls by control animals progressivelydecreased at every measurement since the mice learnt how to balanceon the rotating rod. The spontaneous motility and exploratorybehavior of mice was not modified by treatment with (±)-SM-21(20 and 40 mg kg¹ s.c.) as revealed by the hole-board test (data not shown).

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TABLE 4
Effect of (±)-SM-21, R-(+)-SM-21 and S-( $-$ )-SM-21 in the mouse rota-rod test

In vitro functional studies. (±)-SM-21 blocked the McN-A-343-induced inhibition of twitch contractions of the rabbit vas deferens (pK_B = 5.97 ± 0.11),antagonized the negative inotropic carbachol-induced effect inguinea-pig left atrium (pK_B = 6.63 ± 0.10), the contractile responsesto acetylcholine in guinea-pig ileum (pK_B = 6.35 ± 0.04) and tocarbachol in immature guinea-pig uterus (pK_B = 6.26 ± 0.05) asshown in table 5. Increasing concentrations of (±)-SM-21 producedparallel shifts of the agonist concentration-response curves progressivelyto the right and no appreciable change in basal tension or maximumagonist response was observed (data not shown). pA₂ values ofR-(+)-hyoscyamine and AFDX-116, used as reference drugs, are shownin table 5. The selectivity ratios for (±)-SM-21, R-(+)-hyoscyamineand AFDX-116, obtained as differences between respectively pK_Bor pA₂ values, are reported in table 5.

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TABLE 5
Affinity profiles of (±)-SM-21, R-(+)-hyoscyamine and AFDX-116 at muscarinic M₁ receptors in rabbit vas deferens, M₂ receptorsin guinea pig left atrium, M₃ receptors in guinea pig ileum andM₄ putative receptors in guinea pig uterus. The ratios of affinityconstants are given as a measure of receptor selectivity

Finally, (±)-SM-21 was shown to be endowed with a weak antiacetylcholinesterase activity, its IC₅₀ value on electrical eelacetylcholinesterase being 1.1 · 10⁴ M (data not shown).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

(±)-SM-21 was able to induce antinociception in mice, rats and guinea-pigs. Antinociception was elicited regardless of whichnoxious stimulus was used: thermal (hot-plate and tail flick tests),chemical (abdominal constriction test) and mechanical (paw pressuretest). (±)-SM-21 antinociception was obtained without producingany visible modification of animal gross behavior. Moreover, (±)-SM-21treated mice showed a complete integrity of motor coordinationon the rota-rod test, normal spontaneous motility, as well asexploratory behavior as revealed by the hole-board test.

(±)-SM-21 exerted its antinociceptive effect by acting centrally. It was, in fact, possible to reach the same intensity ofanalgesia by injecting directly into the cerebral ventricles doses(5-20 µg per mouse) of (±)-SM-21 which were one thousand timeslower than those needed parenterally. That the antinociceptiondepends on a retrodiffusion of the drug from the cerebral ventriclesto the periphery can thus be ruled out.

(±)-SM-21 antinociception was found to be dependent on central cholinergic activation since it was prevented by the non-selectivemuscarinic antagonist atropine, the M₁-antagonist pirenzepineand the ACh depletor HC-3. Taking into account that HC-3 and pirenzepinewere able to antagonize (±)-SM-21 antinociception after i.c.v.injection, this supports the hypothesis that the analgesic siteof action of (±)-SM-21 is localized in the CNS. A presynapticmechanism facilitating cholinergic transmission is involved in(±)-SM-21 antinociception as revealed by the antagonism by HC-3.A postsynaptic mechanism of action can be ruled out since, asreported by Bartolini et al. (1987; 1992), HC-3 was not able toantagonize antinociception induced by agonists of postsynapticmuscarinic receptors such as oxotremorine, McN-A-343 and AF-102B.

The hypothesis of a presynaptic cholinergic mechanism for (±)-SM-21 is in agreement with previous results demonstrating, bymicrodialysis studies, an increase in ACh release from rat cerebralcortex induced by (±)-SM-21 administration (Bartolini et al.,1994). This effect occurred in the same range of doses (10 and20 mg kg¹ i.p.) in which the above-mentioned compound exerted its antinociceptiveactivity.

(±)-SM-21, like R-(+)-hyoscyamine (see introduction), demonstrated antinociceptive properties underlying a presynaptic cholinergicmechanism, but with greater efficacy than that exerted by R-(+)-hyoscyamine.The analgesic effect of (±)-SM-21 was also compared with the analgesiainduced by some analgesic drugs such as morphine, diphenhydramineand clomipramine at the highest doses that did not impair therota-rod performances. By comparing the areas under the curve,the antinociceptive efficacy of (±)-SM-21 (30 mg kg¹ s.c.) resulted almost equal to that exerted by morphine (8 mgkg¹ s.c.), but greater than those induced by diphenhydramine (20mg kg¹ s.c.) and clomipramine (25 mg kg¹ s.c.).

(±)-SM-21 and R-(+)-hyoscyamine have been reported to increase the extracellular levels of ACh in cortical microdialysis studies(Bartolini et al., 1994; Romanelli et al., 1995). Since ACh releasecan be increased by blocking M₂/M₄ muscarinic autoreceptors (Lapchaket al., 1989; Töröcsik and Vizi, 1991; McKinney et al., 1993;Stillman et al., 1993) and R-(+)-hyoscyamine showed a very highaffinity for the prepuberal guinea-pig uterus putative M₄ receptors(Ghelardini et al., 1993), the (±)-SM-21 affinity profile towardsmuscarinic receptor subtypes was investigated in vitro. The affinityprofile of (±)-SM-21 versus M₁ (rabbit vas deferens), M₂ (guinea-pigatrium), M₃ (guinea-pig ileum) and putative M₄ receptors (prepuberalguinea-pig uterus) was evaluated by in vitro functional studies.The M₄ muscarinic receptor subtype has been defined as putativesince it has not been confirmed that the mRNA codifying M₄ isexpressed in the prepuberal uterus tissue. However, pharmacologicaland biochemical studies show that the M₄ putative receptor ofprepuberal guinea-pig uterus has a pharmacological and biochemicalprofile identical to that of the muscarinic m₄ receptor subtypeexpressed in the rat striatum (McKinney et al., 1991; Waelbroecket al., 1992) and in NG 108-15 cells (Leiber et al., 1984; Marcet al., 1986). (±)-SM-21 showed, unlike R-(+)-hyoscyamine, a verylow M₄/M₁ muscarinic receptor subtype selectivity ratio (twice),but higher M₂/M₁ selectivity ratio (4.6 times). By comparing theaffinity profile of the M₂ muscarinic antagonists: AFDX-116 (Giachettiet al., 1986), methoctramine (Melchiorre et al., 1987) and AQRA-741(Doods et al., 1991), a selectivity ratio M₂/M₁ lower than thatshowed by (±)-SM-21 can be observed. Moreover, all the above-mentionedM₂ antagonists, like (±)-SM-21, are also endowed with cholinergicpresynaptic antinociceptive properties (Bartolini et al., 1989;Gualtieri et al., 1989; Ghelardini et al., 1991) and AFDX-116and methoctramine are able to increase the ACh release (Lapchaket al., 1989; Töröcsik and Vizi, 1991). It seems, therefore,reasonable to suppose that a selectivity ratio of 4.6, even ifsmall, may be high enough to enhance the pain threshold as a consequenceof ACh release. The antinociception induced by (±)-SM-21 may bedue to the antagonism of the M₂ muscarinic autoreceptor. The selectivityon blocking the M₂/M₄ towards M₁ was evaluated since Bartoliniet al., (1992) have demonstrated that the muscarinic postsynapticreceptor responsible for central cholinergic antinociception belongsto the M₁ subtype. The antinociceptive efficacy of (±)-SM-21 wasgreater than that of R-(+)-hyoscyamine, AFDX-116, methoctramineor AQRA-741. Therefore, we cannot exclude that other mechanismsable to potentiate the endogenous cholinergic system may be involvedin the antinociception induced by (±)-SM-21.

Both enantiomers of SM-21, R-(+) and S-( $-$ ), contrary to atropine in which the analgesic activity resides only in the R-(+)isomer (Ghelardini et al., 1992), showed very similar antinociceptiveproperties in the presence of either a thermal or chemical stimulus.However, in both analgesic tests used, R-(+)-SM-21 resulted weaklymore effective than S-( $-$ )-SM-21. Since R-(+) and S-( $-$ )-SM-21 werenot endowed with a different analgesic profile, their in vitroselectivity towards the muscarinic receptor subtypes was not consideredworth investigating.

It has been demonstrated that D₂ dopaminergic (Gorell and Czarnecki, 1986; Wedzony et al., 1988; Scatton, 1992; Imperato etal., 1993), A₁ adenosinergic (Jackisch et al., 1984; Carter etal., 1995), H₃ histaminegic (Clapham and Kilpatrick, 1992), 5-HT₄serotoninergic heteroreceptors (Consolo et al., 1994), all locatedon central cholinergic neurones, increase ACh release. The involvementof the above-mentioned heteroreceptors was, therefore, investigated.Quinpirole (D₂ agonist), N⁶-cyclopentyladenosine (A₁ agonist), R-( $alpha$ )-metylhistamine (H₃ agonist),and GR-48125 (5-HT₄ antagonist), at doses able to prevent theantinociception induced respectively by haloperidol, caffeine(Ghelardini et al., 1992), thioperamide (Malmberg-Aiello et al.,1994), BIMU 1 and BIMU 8 (Ghelardini et al., 1996), failed toprevent (±)-SM-21 antinociception. Previous data have shown thatantinociception induced by (±)-SM-21 and its enantiomers was partiallyprevented by the 5-HT₄ antagonist SDZ 205-557 (Romanelli et al.,1995). Since GR-48125 was more selective than SDZ 205-557 towards5-HT₄ receptors and was not able to antagonize SM-21 antinociception,the prevention of the SM-21 effect produced by SDZ 205-557 wasprobably not related to an antagonism of 5-HT₄ receptors. It hasalso been observed that the activation of the serotoninergic autoreceptor5-HT_1A enhances ACh release from the guinea-pig cortex (Bianchiet al., 1990). Pretreatment with the 5-HT_1A selective antagonistNAN 190 at doses which block the antinociception induced by 5-HT_1Aagonists (Ghelardini et al., 1994), did not prevent the enhancementof the pain threshold produced by (±)-SM-21 administration. Thepresent data suggest that the above-mentioned receptors, eventhough they are able to increase ACh release, are not involvedin (±)-SM-21 mechanism of analgesic action.

The antinociception induced by antagonists of the muscarinic autoreceptors, such as R-(+)-hyoscyamine and AFDX-116, was significantlypotentiated by pretreatment with a subliminary non-analgesic doseof physostigmine. By contrast, in the same experimental conditions,(±)-SM-21 antinociception was not modified by physostigmine pretreatment.These observations may suggest that (±)-SM-21 is endowed withvery low anticholinesterase activity, a hypothesis that seemsto be in agreement with the in vitro evaluation of the IC₅₀ valueof (±)-SM-21 (IC₅₀ = 1.1 · 10⁴ M). It is possible that (±)-SM-21 is able to amplify cholinergicneurotransmission through the antagonism of the muscarinic autoreceptorand that this effect is in its turn potentiated by its low cholinesteraseinhibitory activity.

Other neurotransmitter systems are not involved in (±)-SM-21 antinociception since the opioid antagonist naloxone, the GABA_Bantagonist CGP-35348 and the polyamine depletor reserpine, wereall unable to prevent the effect of (±)-SM-21. The doses and administrationschedules of the above-mentioned drugs were ideal for preventingantinociceptions induced respectively by morphine (Ghelardiniet al., 1992), the GABA_B agonist baclofen (Malcangio et al., 1991)and the antidepressant drugs clomipramine and amitriptyline (Galeottiet al., 1995).

(±)-SM-21 at analgesic doses failed to suppress paw edema in response to carrageenan administration, suggesting that its antinociceptionis not due to an antiinflammatory action.

In summary, our results have shown that (±)-SM-21 is able to produce dose-dependent antinociception in rodents and guineapigs, without impairing motor coordination, by potentiating endogenouscholinergic activity.

	Acknowledgments

The authors wish to thank Giba Geigy for the gift of CGP-35348.

	Footnotes

Accepted for publication March 18, 1997.

Received for publication July 16, 1996.

¹ This research was supported by grants from Fidia S.p.A. (Abano Terme, Italy) and from Ministero dell'Università e della RicercaScientifica e Tecnologia (MURST). Preliminary data were presentedat the XIII International Symposium on Medicinal Chemistry, Paris,September 19-23, 1994; at the XXVII Meeting of Italian PharmacologicalSociety, Turin, September 25-29, 1994 and at the VI InternationalSymposium on Subtypes of Muscarinic Receptors, Fort Lauderdale,Florida, November 9-12, 1994.

Send reprint requests to: Prof. Alessandro Bartolini, Department of Pharmacology, University of Florence, Viale G.B. Morgagni, 65, I-50134 Florence, Italy.

	Abbreviations

SM-21, 3- $alpha$ -tropanyl-(2-Cl)-acid phenoxybutyrate; HC-3, hemicholinium-3; NAN 190, 1-(2-methoxyphenyl)-4-[4-(2-phthalimido)butyl]piperazine hydrobromide; McN-A-343, 4-(N-[3-chlorophenyl]-carbamoyloxy)-2-butynyl-trimethylammonium chloride; GR 125487, [1-[2(methylsufonyl)amino]ethyl]-4-piperidinyl] methyl-5-fluoro-2-methoxy-1H-indole-3-carboxylate hydrochloride; AFDX-116, 11,2-(diethylamino)methyl-1-piperidinil acetyl-5,11-dihydro-6H-pyrido 2,3-b 1,4 benzodiazepine-6-one; CGP 35348, 3-aminopropyl-diethoxy-methyl-phosphinic acid; RAMH, (R)- $alpha$ -methylhistamine.

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Antinociceptive Profile of 3--tropanyl-(2-Cl)-acid phenoxybutyrate (SM-21): A Novel Analgesic with a Presynaptic Cholinergic Mechanism of Action1

Antinociceptive Profile of 3- $alpha$ -tropanyl-(2-Cl)-acid phenoxybutyrate (SM-21): A Novel Analgesic with a Presynaptic Cholinergic Mechanism of Action¹