CP-96,345, which Inhibits [3H] Substance P Binding, Selectively Inhibits the Behavioral Response to Intrathecally Administered N-Methyl-D-Aspartate, but not Substance P, in the Mouse

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Vol. 281, Issue 3, 1231-1237, 1997

CP-96,345, which Inhibits [³H] Substance P Binding, Selectively Inhibits the Behavioral Response to Intrathecally Administered N-Methyl-D-Aspartate, but not Substance P, in the Mouse¹

Rubén A. Velázquez, Kelley F. Kitto and Alice A. Larson

Department of Veterinary PathoBiology, University of Minnesota, Saint Paul, Minnesota

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

((2S,3S)-[cis-2-(diphenylmethyl)-N-[(2-methoxyphenyl)-methyl]-1-azabicyclo[2.2.2]octan-3-amine]) (CP-96,345) noncompetitivelyinhibits substance P (SP) binding at the neurokinin-1 (NK-1) siteand has been widely used to determine the extent of NK-1 activityin nociception. To test the selectivity of this compound in vivoregarding other putative nociceptive transmitters, such as excitatoryamino acids, we compared the actions of CP-96,345 to those of((2R,3R)-[cis-2-(diphenylmethyl)-N-[(2-methoxyphenyl)-methyl]-1-azabicyclo[2.2.2]octan-3-amine]),a less active isomer, on behavioral responses induced by SP, N-methyl-D-aspartate(NMDA) and kainic acid (KA) injected intrathecally in mice. Wheninjected intrathecally, SP, NMDA or KA produce a caudally directedbiting and scratching behavior that lasted for approximately 60to 90 sec. At a dose as high as 2 nmol, CP-96,345 had no effecton responses induced by a single injection of 22.5 pmol of SP.In contrast, NMDA-induced behaviors were inhibited by CP-96,345in a dose-related fashion beginning at a dose as low as 0.02 nmol.There was also an inhibitory effect of CP-96,345 on KA-inducedactivity that was not dose related. The more potent inhibitorof [³H] SP binding, (+)-(2S,3S)-3-(2-methoxybenzylamino)-2-phenylpiperidine(CP-99,994), was approximately 10 times more potent in inhibitingNMDA-induced activity than CP-96,345. CP-99,994 also inhibitedNMDA-induced activity at doses that failed to inhibit SP-inducedbehavior. Also attenuated by CP-96,345 was the development ofsensitization to the behavioral effects produced by repeated injectionsof KA and desensitization to repeated injections of SP, phenomenalinked to an action of the N-terminus of SP. NMDA-induced behaviorsand sensitization to KA were found to be sensitive to verapamil,consistent with their mediation by calcium. These results indicatethat either CP-96,345 and CP-99,994 do not inhibit NK-1-inducedactivity in the mouse spinal cord, or that exogenously administeredSP does not induce behavioral responses by an interaction withNK-1 receptors. Whether CP-96,345 acts by a mechanism that involvesinhibition of calcium channels and/or SP N-terminal activity requiresfurther testing.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

The peripheral and central roles of SP in nociceptive transmission have been extensively studied. SP and EAAs are coexpressedin small diameter primary afferent fibers (Battaglia and Rustioni,1988; DeBiasi and Rustioni, 1988) and are thought to be involvedin nociception (Cruwys et al., 1995; Levine et al., 1993; Melleret al., 1992; Mjellem-Jolly et al., 1992; Aanonsen and Wilcox,1987; Hylden and Wylcox, 1981). SP has a high affinity for NK-1receptors that are present in abundance in the superficial layersof the dorsal horn of the spinal cord (Liu et al., 1995; Mantyhet al., 1995). SP is released into the cerebrospinal fluid afterstimulation known to depolarize primary afferent nociceptors (Levineet al., 1993). Activation of NK-1 sites by i.t. injection of SPresults in a transient hyperalgesia (Radhakrishnan et al., 1995)although inhibition, using various SP antagonists, results inantinociception (Ohkubo et al., 1990).

When injected i.t., SP also produces a series of behaviors characterized by biting and scratching of the hindlimbs (Hyldenand Wilcox, 1981). This behavior can also be elicited by administrationof KA, NMDA and capsaicin (Sun and Larson, 1991), compounds thoughtto activate receptors involved in nociception. Caudally directedbiting and scratching behavior has been suggested to reflect activationof a variety of pathways including neurons involved in the transmissionof pain resulting from a local, spinally mediated mechanism (Pierceyet al., 1981). Although it is still unclear whether this behaviorreflects pain perception, the number of these behaviors permitsa reproducible and quantifiable measure of the degree of activationof receptor populations believed to be involved in nociception(Hornfeldt et al., 1994).

CP-96,345 has been found to be a potent inhibitor of SP binding (Snider et al., 1991). Although originally proposed to actas a competitive antagonist at NK-1 sites, CP-96,345 interactswith a site on the NK-1 receptor that has been found to be distinctfrom the binding site for the C-terminus of SP (Fong et al., 1992b).Because of the difference among species in the amino acid sequenceat residues 116 and 290 of the NK-1 receptor, some species aresignificantly more or less susceptible to the antagonistic actionof CP-96,345 at NK-1 sites relative to its nonselective abilityto inhibit calcium channels (Fong et al., 1992a). The guinea pigis the most sensitive to CP-96,345, although the rat and mouseeach have only a 10-fold difference in the concentration of CP-96,345that inhibits SP binding and the concentration that produces anonstereoselective inhibition of calcium channels (Schmidt etal., 1992). Whether CP-96,345 produces its effects in vivo viainhibition of SP or inhibition of calcium flux is dependent onthe model tested.

Compared to CP-96,344, its 2R,3R enantiomer, CP-96,345 has been found to inhibit a variety of phenomena associated with nociceptivetransmission, including late responses to noxious thermal stimulationand iontophoretically applied SP in the cat spinal cord (Radhakrishnanand Henry, 1991), SP-mediated slow excitatory postsynaptic potentialsin cat dorsal horn neurons (De Koninck and Henry, 1991), latedischarges of superficial dorsal horn neurons carrying nociceptiveinput in the rat spinal cord (Toda and Hayashi, 1993), SP-inducedplasma extravasation in the guinea pig skin (Nagahisa et al.,1992), plasma extravasation induced by antidromic C-fiber stimulationin the rat hindpaw (Xu et al., 1992) and SP-induced excitationof locus ceruleus neurons in the guinea pig (McLean et al., 1991).CP-96,345 and CP-96,344 are equally effective in their inhibitionof carrageenin-induced foot edema, carrageenin-induced hyperalgesiaand the second phase response of the formalin-induced paw lickingin the rat (Nagahisa et al., 1992), suggesting a possible involvementof calcium channel activity rather than inhibition of the NK-1receptor.

Although the selectivity of CP-96,345 on NK-1 vs. NK-2 and NK-3 receptor binding has been well studied (McLean et al., 1991;Snider et al., 1991), its selectivity with respect to other receptors,including EAAs receptors, has not. The goal of our study was toexamine the selectivity of the inhibitory effect of CP-96,345on the behavioral response produced by i.t. injections of SP comparedto that produced by NMDA and KA. The effect of CP-96,345 was thencompared to that of CP-96,344 and verapamil, compounds that inhibitcalcium channel activity with less or no affinity to inhibit NK-1receptors, respectively. We also used CP-99,994, a newer and morepotent NK-1 antagonist than CP-96,345, for comparison to the effectsof CP-96,345.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Animals. Male Swiss-Webster mice (15-20 g, Sasco Inc., Omaha, NE) were housed four per cage in animal facilities with controlled temperatureand 12-hr light and dark cycles. This facility is cleaned daily.Animals were allowed free access to food and water, allowed toacclimate for at least 24 hr before use and always used duringthe light period of the cycle. Animals were used strictly in accordancewith the Guidelines of the University of Minnesota Animal Careand Use Committee and those prepared by the Committee on Careand Use of Laboratory Animals of the Institute of Laboratory AnimalResources, National Research Council [DHEW Publication (NIH) 78-23,revised 1978].

Drug administration. Except where indicated, all injections were administered i.t. in mice at approximately the L5-L6 intervertebral space usinga 30-gauge, 0.5-inch disposable needle on a 50-µl Luer tip Hamiltonsyringe (Fisher Scientific, Pittsburgh, PA). A volume of 5 µlwas used for all i.t. injections as it is readily measured andappears to elicit sensitization to repeated injection of KA thatis identical to that using 2 µl per injection (Sun and Larson,1991). SP was administered in 0.85% NaCl containing 0.01 N aceticacid (pH 3.4) to minimize absorption to synthetic surfaces (Halland Stewart, 1983). KA and NMDA were routinely administered insaline (pH 7.4). Doses of 25 pmol SP, 300 pmol NMDA and 22.5 pmolof KA were used as these doses were found to produce an intensityof behavioral responses that allows us to monitor either increasesor decreases in the response. CP-96,345, CP-96,344, CP-99,994and verapamil were diluted in normal saline (pH 7.4) and administered30 min before injection of SP or EAAs, except where indicated.

Experimental protocol for behavioral responses. Immediately after i.t. injection of KA, NMDA or SP, animals were placed in a large glass cylinder containing approximately2 cm of bedding. The total number of caudally directed bites andscratches over a 2-min interval were recorded. Injection of thesame volume of vehicle over this time interval has been shownto elicit no increase in behaviors above noninjected control miceand to have no effect on the normal exploratory behavior of themice (Sun and Larson, 1991). Four consecutive injections of KAand SP (or NMDA) were used in all experiments involving testingof sensitization and desensitization, respectively. After thefirst injection, behaviors were counted during a 2-min interval.At the end of the 2-min interval, the animal was reinjected andbehaviors counted for 2 min. The same procedure was repeated forthe third and fourth injections. Sensitization was defined asan increase in the number of behaviors measured during the 2-mininterval after the fourth injection of a compound. Desensitizationwas defined as an decrease in the number of the biting and scratchingbehavior during the 2-min interval after the fourth injection.

Drugs. CP-96,345, CP-96,344 and CP-99,994 were generously provided by Pfizer Central Research (Groton, CT). SP was purchased fromPeninsula Laboratories (Belmont, CA). KA, NMDA and verapamil werepurchased from Sigma Chemical Company (St. Louis, MO).

Data analysis. Mean (± S.E.M.) of the data are presented in all figures. Throughout the experiments, each group represents at least six mice.Statistical analysis of the number of behaviors 2 min after thefirst and fourth injection was performed using analysis of variancefollowed by the Scheffé F test of significance using the MacintoshStatView version 1.02 software. P < .05 were used as the cut offto indicate a significant difference between the test group andcontrol values.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Injection of 0.002 to 2 nmol of CP-96,345 30 min before testing, failed to inhibit the number of caudally directed bitingand scratching behaviors induced by a single injection of 22.5pmol of SP (fig. 1A), despite the sensitivity of this responseto the inhibitory effect of 1 nmol of DPDT-SP when injected 5min before SP (Mousseau et al., 1994). In contrast, pretreatmentwith CP-96,345 produced a dose-related inhibition of NMDA-inducedbehaviors (fig. 1C). KA-induced behaviors were uniformly but weaklyinhibited by all doses of CP-96,345 tested (fig. 1B). The lackof a dose-relatedness suggests a nonspecific action on this non-NMDA-inducedactivity.

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Fig. 1. Effect of CP-96,345 on SP-, KA- and NMDA-induced behaviors. CP-96,345 was injected i.t. 30 min before injection of SP or EAAs.The dotted line represents the mean number of behaviors in responseto a single i.t. injection of agonist after pretreatment withsaline. Values represent the mean (± S.E.M.) number of bitingand scratching behaviors after injection of the compound indicated,here as follows: (A) 22.5 pmol SP, (B) 25 pmol KA and (C) 0.3nmol NMDA. Asterisks represent significant differences (P < .05)between groups pretreated with saline and CP-96,345.

Whereas CP-96,345 failed to alter the number of behavioral responses to a single injection of SP, it prevented the developmentof desensitization to the behavioral effect of SP that resultsfrom repeated injections of SP. The effect of CP-96,345 was toattenuate, in a dose-related fashion, the normal decrease in theintensity of behaviors (i.e., behavioral desensitization) inducedby each injection of SP as indicated by a dose-related decreasein the response to the fourth injection of SP (fig. 2). In addition,the increased number of responses to each of four injections ofKA (i.e., behavioral sensitization) was inhibited by pretreatmentwith CP-96,345 over a dose-range similar to that preventing behavioraldesensitization to SP (fig. 2).

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Fig. 2. Effects of pretreatment (30 min) with CP-96,345 on SP desensitization and KA sensitization. Injection of KA or SP i.t. every2 min for four injections results in an increase (behavioral sensitization)or decrease (behavioral desensitization) in the response elicitedby these compounds. Desensitization to the behavioral effect ofSP is indicated by the change (decrease) in the number of behaviorsduring the 2 min after the fourth injection compared to the firstinjection of SP. Sensitization to the behavioral effect of KAis indicated by the magnitude of the change (increase), in thenumber of behaviors for 2 min after the fourth injection comparedto the first injection of each compound. Asterisks represent significantdifferences (P < .05) in the degree of sensitization or desensitizationbetween groups pretreated with CP-96,345 at the doses indicatedand vehicle-injected control mice tested on the same day.

To determine whether the effect of CP-96,345 was via its ability to inhibit calcium channels, we first examined the effectof CP-96,344, an isomer of CP-96,345, that is equal to CP-96,345in its ability to inhibit calcium channels activity, but lesspotent than CP-96,345 in its ability to inhibit NK-1 activity.Our results indicate that CP-96,344 differed only slightly fromCP-96,345, in its ability to inhibit the development of desensitizationto SP (fig. 3A), sensitization to repeated injections of KA (fig.3B) or to inhibit NMDA-induced behaviors (fig. 3C). When administeredi.p., the response to each of these isomers did not differ fromeach other in their influence on responses to four injectionsof KA (fig. 4). The magnitude of the effects produced by 40 µg/kgof CP-96,345, which is approximately 1.6 to 2 nmol per mouse,was also very similar to the effect elicited by an i.t. injectionof 2 nmol of CP-96,345 (fig. 3B).

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Fig. 3. Comparison of inhibitory effects of CP-96,344 and CP-96,345. Animals were pretreated with 2 nmol CP-96,344 or CP-96,345 30min before the first of four i.t. injections of (A) 22.5 pmolSP, (B) 25 pmol KA or (C) 0.3 nmol NMDA. Biting and scratchingbehaviors were measured during a 2-min interval after each agonistinjection. The duration of behaviors after each injection wasusually 60 to 90 sec. Values represent the mean (± S.E.M.) numberof biting and scratching behaviors after injection of the compoundindicated. Asterisks represent significant differences (P < .05)in the response to a single injection (0-2 min) and in the degreeof sensitization or desensitization (6-8 min) when compared toresponses from vehicle-pretreated animals (dotted line).

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Fig. 4. Effect of i.p. CP-96,344 and CP-96,345 on KA sensitization. Values represent the mean (± S.E.M.) number of biting and scratchingbehaviors during a 2-min interval after each of four injectionsof KA, 30 min after pretreatment with 40 µg/kg i.p. of CP-96,344or CP-96,345. Asterisks represent significant differences (P <.05) from vehicle-pretreated animals (dotted line); details asin figure 3.

To test the possibility that inhibition of calcium flux produces effects similar to the inhibitory effect of CP-96,345, wecompared its action to that of verapamil, which has no abilityto inhibit SP binding. Injected at a dose of 5 pmol 30 min beforetesting, verapamil did not inhibit the response to a single injectionof SP or to repeated injections of SP (fig. 5A). However, verapamilinhibited the development of sensitization to repeated injectionsof KA, suggesting a calcium-sensitive component in this phenomenon(fig. 5B). Verapamil also inhibited the response to a single injectionof NMDA, which is known to be brought about by activation of acalcium channel (fig. 5C).

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Fig. 5. Effect of verapamil on SP desensitization, KA sensitization and NMDA-induced behaviors. Animals were pretreated with 5 pmolof the calcium channel blocker, verapamil, 30 min before the firstof four i.t. injections of (A) 22.5 pmol SP, (B) 25 pmol KA or(C) 0.3 nmol NMDA. See "Materials and Methods" for details. Valuesrepresent the mean (± S.E.M.) number of biting and scratchingbehaviors after injection of the compound indicated. Asterisksrepresent significant differences (P < .05) from vehicle-pretreatedanimals (dotted line).

We also found that pretreatment with CP-99,994, a more potent nonpeptide NK-1 antagonist, failed to inhibit biting and scratchingproduced 30 min later by a single injection of 22.5 pmol of SP(fig. 6A) but was effective in inhibiting NMDA-induced behaviorsat that time (fig. 6B).

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Fig. 6. Effect of CP-99,994 on SP and NMDA-induced behaviors. To further study the effects to responses elicited by nonpeptide NK-1antagonists to i.t. SP or NMDA, we used 0.2 nmol of the more potentNK-1 antagonists CP-99,994 30 min before the first of four i.t.injections of (A) 22.5 pmol SP and (B) 0.3 nmol NMDA. Asterisksrepresents significant differences (P < .05) between groups pretreatedwith saline and CP-99,994.

To determine if the previously reported inhibitory effect of CP-96,345 on SP-induced biting and scratching (Sakurada et al.,1994) may be due to a difference in the dose of SP or the experimentaldesign, we also examined the effects of CP-96,345 using the sametime of pretreatment, measurement interval and dose of SP as thatused previously by Sakurada's group. We coadministered 2 nmolCP-96,345 and 100 pmol SP i.t. and measured the number of behaviorsover a period of 2 and 5 min. Although 2 nmol of CP-96,345 failedto affect the behavioral response to 22.5 pmol of SP (fig. 1A),this same dose of CP-96,345 was sufficient to inhibit the numberof behaviors elicited over a 5-min interval by the higher doseof SP (fig. 7), consistent with previously reported studies ofCP-96,345 (Sakurada et al., 1994). When the same data from thefirst 2-min interval are analyzed, inhibition of SP by CP-96,345was not significant using our statistical criteria.

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Fig. 7. Effect of coadministration of CP-96,345 and SP. The effects of i.t. coadministration of 2 nmol CP-96,345 and 100 pmol of SPwere measured over a 2- and a 5-min intervals. The asterisk representssignificant differences (P < .05) between animals treated withSP alone and those coadministered with SP and CP-96,345 at thedoses indicated.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The inability of CP-96,345 to inhibit caudally directed biting and scratching produced in mice by a single i.t. injectionof SP presents an interesting paradox concerning the identityof receptors with which this compound interacts to elicit itseffects in vivo. This is especially true as the doses of CP-96,345tested readily inhibited other effects, including NMDA activity,desensitization to the behavioral effects of SP and sensitizationto KA. If SP-induced behaviors are exclusively the result of NK-1activation, CP-96,345 and CP-99,994 would be expected to inhibitthe response to SP as they are potent inhibitors of [³H]SP binding (Snider et al., 1991). Our data suggest that eitherthe response to a single injection of SP is not mediated by activationof NK-1 sites, or that CP-96,345 and CP-99,994 also bind, withan even greater affinity, to a site distinct from the NK-1 receptorto affect EAA activity.

Although it is possible that SP induces a behavioral response in mice that is not mediated by NK-1 activity (Matsumura etal., 1985), DPDT-SP, a D-analog of SP and a NK-1 antagonist, isable to inhibit the behavioral response produced by i.t. injectionsof SP (Mousseau et al., 1994). In addition, SP(5-11), a SP fragmentthat contains the tachykinin sequence homology necessary to interactwith NK receptors, mimics the behavioral effect of SP. In fact,the ability of SP(5-11) to elicit biting and scratching behaviorsis roughly equipotent to that of SP(1-11) (Igwe et al., 1990c).This is in contrast to their relative affinity at NK-1 bindingsites in vitro where increasing the length of the amino terminalsequence from SP(5-11) to SP(1-11) enhances the affinity of theSP fragment for the NK-1 peptide binding site about 1000-fold(Cascieri et al., 1992). This indicates that the amino terminalportion of SP is essential for affinity as well as selectivityof binding. However, SP N-terminal fragments, such as SP(1-7)by themselves do not compete for binding at NK-1 sites and produceno behavioral response when injected i.t. (Sun and Larson, 1991).The discrepancy between the relative potency of SP(1-11) and SP(5-11)in vivo vs. their affinity for NK-1 binding may be due to inhibitoryeffects of SP N-terminal metabolites that are believed to accumulatein vivo (Nyberg et al., 1984; Sakurada et al., 1985) and interactat distinct binding sites (Igwe et al., 1990b). SP(1-11) may havea higher affinity for NK-1 binding than SP(5-11) in vitro, however,SP(1-11) may contribute to the generation of a pool of amino terminalmetabolites that are inhibitory to NK-1-induced activity in vivo.

Consistent with the absence of any possible inhibitory SP N-terminal activity associated with SP(5-11), there is no desensitizationto the behavioral effects produced by repeated injections of SP(5-11).In contrast, desensitization develops readily to SP(1-11) (Igweet al., 1990a; Moochhala and Sawynok, 1984). Thus, the inabilityof CP-96,345 to inhibit the response to a single injection ofSP yet attenuate the development of desensitization to SP arguesfor a possible interaction of CP-96,345 with a site that is normallymodulated by activity of the N-terminus of SP. Based on the poorability of compounds such as SP(1-7) to compete for [³H]SP binding (Yukhananov and Larson, 1994), modulation of NK-1activity by SP N-terminal fragments likely occurs by an indirectroute involving a SP amino terminal binding site (Igwe et al.,1990b) that is distinct from the NK-1 receptor.

In support of the possibility that CP-96,345 inhibits SP N-terminal activity, CP-96,345 inhibits both SP desensitization andKA sensitization, responses that have been proposed to be mediatedby SP N-terminal activity (Sun and Larson, 1991; Larson and Sun,1992). Substance P N-terminal fragments have also been found toinhibit and potentiate NMDA-induced behaviors, depending on thetime of administration relative to injection of NMDA (Hornfeldtet al., 1994). As with CP-96,345, D-SP(1-7), the D-analog of acommonly occurring SP metabolite, prevents behavioral desensitizationto repeated injections of SP (Igwe et al., 1990c) and inhibitssensitization to KA (Larson and Sun, 1992) although SP N-terminalfragments, such as SP(1-7), inhibit SP-induced behaviors (Igweet al., 1990c) and potentiate the response to KA (Larson and Sun,1992). Thus, CP-96,345 and CP-99,994 may affect SP, KA and NMDAactivity by interfering with the mechanism by which the N-terminusof SP normally elicits its modulatory effects.

Based on the ability of verapamil to inhibit NMDA-induced activity as well as behavioral sensitization to KA, these phenomenaappear to be dependent on calcium channel activity. Binding studiessuggest that there is only a 10-fold difference in the inhibitionof NK-1 sites by CP-96,345 compared to nonselective calcium channelinhibition, as demonstrated by the use of CP-96,344. The differencebetween the effects of CP-96,345 and CP-96,344 on NMDA activityand on KA sensitization in our study and the sensitivity of thesephenomena to verapamil suggest that the majority of the effectof CP-96,345 appears to result from inhibition of calcium channels.One possibility is that SP N-terminal binding sites are directlyor indirectly linked to calcium channel activity.

Although we found no inhibition of SP-induced behaviors, a racemic mixture of (±)CP-96,345 has been previously found to inhibitresponses elicited by an i.t. injection of 200 nmol of SP in mice(Lecci et al., 1991). Results using a racemic mixture and sucha large dose of SP must be considered carefully. Because a behavioralresponse can be readily evoked by 25 pmol of SP, it is unclearwhy such a large and potentially nonspecific dose of SP (8000times the dose used in our study) was used. Sakurada et al. (1994)have also achieved a partial inhibition of SP-induced behaviorsin mice by coadministration of 2 nmol of CP-96,345 with 100 pmolof SP, a dose that is approximately four times greater than thoseused in our investigation. Although one would expect that lowerdoses of an agonist would be more readily antagonized than higherdoses, when we repeated the experiments as done by Sakurada'sgroup, testing the effect of 2 nmol CP-96,345 coadministered with100 pmol SP, CP-96,345 inhibited SP-induced behaviors evoked overa 5-min interval (fig. 7). Time of administration of CP-96,345relative to challenge with SP was not the critical factor in theability of this drug to inhibit the effect of 100 pmol of SP ascoadministration of 2 nmol of CP-96,345 with 22.5 pmol of SP,rather than as a pretreatment had no effect on SP-induced behaviors(fig. 7) and still inhibited NMDA-induced responses (data notshown). The ability of CP-96,345 to inhibit the effects of a highbut not a low dose of SP suggests that CP-96,345 may have inhibiteda nonselective action of SP or an event downstream from SP receptoractivity. Because SP can induce release of EAAs in the dorsalspinal cord (Skilling et al., 1990), the inhibitory effect ofCP-96,345 on a high, but not a low dose of SP may have been broughtabout by inhibition of NMDA-induced activity after EAA release.

Pain transmission is believed to involve activity along primary afferent C-fibers resulting in the release of SP and EAAs(Urban et al., 1994). Although NMDA activity is proposed to playa role in nociception (Mjellem-Joly et al., 1992) and hyperalgesia(Aanonsen and Wilcox, 1987), KA sensitization may also reflecta component of nociceptive processing. If true, KA sensitizationwould be expected to be sensitive to those compounds that inhibitpain or prevent the development of hyperalgesia. In support ofsuch a relationship, MK-801 and phencyclidine, which inhibit KAsensitization, also inhibit hyperalgesia that develops in responseto a variety of stimuli (Nishihara et al., 1995). In a similarfashion, capsaicin pretreatment in the adult animal not only preventsKA sensitization, but attenuates nociception (Cruwys et al., 1995)and prevents the development of hyperalgesia (Meller et al., 1992).The antinociceptive effects of CP-96,345 observed by numerousinvestigators (Lecci et al., 1991; Nagahisa et al., 1992; Xu etal., 1992) may thus reflect the ability of CP-96,345 to inhibitNMDA and KA activity. One might postulate that CP-96,345 attenuatesNMDA activity indirectly by inhibiting SP released in responseto activation of NMDA receptors located on primary afferent C-fibers(Liu et al., 1994). However, it remains unclear why NMDA-inducedrelease of SP would be sensitive to the inhibitory effect of CP-96,345whereas exogenously administered SP would not.

In summary, CP-96,345 produced a dose-dependent inhibition of the behavioral response to an i.t. injection of NMDA at dosesthat failed to inhibit the behavioral response to SP. CP-96,345also inhibited the development of sensitization to KA-inducedbehaviors. Thus, the inhibitory effect of CP-96,345 on the activityof NMDA and sensitization to KA may be responsible for the antinociceptiveeffect of CP-96,345. These effects may be brought about, at leastin part, by inhibition of calcium channels involved in NMDA activityand KA sensitization and perhaps by inhibition of SP N-terminalactivity. These possibilities require further investigation.

	Acknowledgments

The authors thank Pfizer Central Research for generously providing CP-96,344, CP-96,345 and CP-99,994.

	Footnotes

Accepted for publication February 28, 1997.

Received for publication September 30, 1996.

¹ This work was supported by United States Public Health Service Grant DA04090 to A.A.L. and National Research Service AwardNS09882 to R.A.V.

Send reprint requests to: Dr. Alice A. Larson, Department of Veterinary PathoBiology, University of Minnesota, 295 Animal Science/Veterinary Medicine Building, 1988 Fitch Avenue, St. Paul, MN 55108.

	Abbreviations

CP-96, 344, ((2R,3R)-[cis-2-(diphenylmethyl)-N-[(2-methoxyphenyl)-methyl]-1-azabicyclo[2.2.2]octan-3-amine]); CP-96, 345, ((2S,3S)-[cis-2-(diphenylmethyl)-N-[(2-methoxyphenyl)-methyl]-1-azabicyclo[2.2.2]octan-3-amine]); CP-99, 994, (+)-(2S,3S)-3-(2-methoxybenzylamino)-2-phenylpiperidine; DPDT-SP, [D-Pro², D-Phe⁷]-substance P; EAA, excitatory amino acid; i.t., intrathecal; KA, kainic acid; MK-801, dizocilpine or (+)-5-methyl-10,11-dihydro-5H-dibenzo[a,d]cyclohepten-5,10-imine maleate; NK-1, neurokinin-1; NMDA, N-methyl-D-aspartate; PCP, phencyclidine; SP, substance P.

	References

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