Nonopioid Motor Effects of Dynorphin A and Related Peptides: Structure Dependence and Role of the N-Methyl-D-aspartate Receptor

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Vol. 283, Issue 2, 604-610, 1997

Nonopioid Motor Effects of Dynorphin A and Related Peptides: Structure Dependence and Role of the N-Methyl-D-aspartate Receptor¹

Vijay K. Shukla, Jyoti A. Prasad and Simon Lemaire

Department of Pharmacology, Faculty of Medicine, University of Ottawa, Ottawa, Ontario, Canada

	Abstract

Top Abstract Introduction Methods Results Discussion References

Dynorphin (Dyn) A and related opioid and nonopioid peptides were tested for their ability to produce motor effects in mice.Central (intracerebroventricular) administration of Dyn A in miceproduced marked motor effects characterized by wild running, jumping,circling and/or barrel rolling with an ED₅₀ value of 14.32 (95%confidence limits, 10.09-20.32) nmol/mouse. The order of potencyof the various Dyn A-related peptides and fragments in producingmotor effects was Dyn A $sime$ Dyn A-(1-13) > [Ala¹]Dyn A-(1-13) $sime$ Dyn A-(2-13) > $alpha$ -Neo-End > Dyn A-(1-8) $sime$ Dyn B $sime$ Dyn A-(2-8) >>> Dyn A-(3-8). Dyn A-(1- 5) (or Leu-Enk) and DynA-(6-10) displayed no motor effect at doses up to 100 nmol/mouse.The potencies of Dyn A and Dyn A-(2-13) were not affected by preadministrationof naloxone (5 mg/kg s.c.), but the motor effects of Dyn A-(1-13)(20 nmol/mouse i.c.v.) were significantly reduced by coadministrationof low doses (0.2-0.6 nmol/mouse) of the N-methyl-D-aspartate(NMDA) receptor antagonists dextrorphan, MK-801 and CPP. Dyn Awas also a potent inhibitor of the binding of the phencyclidinereceptor ligand, [³H]MK-801, to rat brain membranes, with a K_i value of0.41 µM. However, the order of potency of the various Dyn A-relatedpeptides and fragments in inhibiting [³H]MK-801 binding did not correlate with their ability to producemotor effects. On the other hand, Dyn A and related peptides produceda significant potentiation of the binding of the competitive NMDAantagonist [³H]CGP-39653 to rat brain membranes, an effect that correlatedwell (r = 0.91) with their potency in producing motor effects.These results indicate that the nonopioid motor effects of DynA and related peptides are structure dependent, with Dyn A-(2-8)being the minimal core peptide for motor activity. In addition,these effects most likely involve the participation of the excitatoryamino acid binding domain on the NMDA receptor complex.

	Introduction

Top Abstract Introduction Methods Results Discussion References

Dyn A is an endogenous peptide possessing high binding affinities for all opioid receptor types and some binding selectivityfor the kappa site (Garzon et al., 1984). Dyn A-related peptides(see fig. 1 for structures) also bind to nonopioid sites (Dumontand Lemaire, 1993; Smith and Lee, 1988). Various pharmacologicaland/or pathophysiological effects of Dyn A and related peptidesare not antagonized by the opiate antagonist naloxone and aremimicked by nonopioid fragments of the peptide (Dumont and Lemaire,1997; Shukla and Lemaire, 1994). In rat heart synaptosomal preparations,Dyn A and related peptides inhibit the uptake of [³H]norepinephrine, and a good correlation exists between the abilityof the peptides to inhibit [³H]norepinephrine uptake and compete with the binding of [³H]Dyn A-(1-13) to nonopioid sites (Dumont and Lemaire, 1994a).

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Fig. 1. Structures of Dyn A and related peptides.

In vivo, Dyn A-(1-13) and related peptides produce a wide variety of nonopioid effects, such as hindlimb paralysis (Stevensand Yaksh, 1986), loss of tail flick reflex (Caudle and Isaac,1987), decreases in spinal cord blood flow (Long et al., 1987),neuroanatomic damage (Long et al., 1988), antagonism of morphineanalgesia (Walker et al., 1983) and suppression of naloxone-precipitatedopioid withdrawal and tolerance (Takemori et al., 1993). The minimalcore peptides that produced motor dysfunctions and suppressedopioid withdrawal and tolerance were Dyn A-(3-13) and Dyn A-(2-8),respectively (Stevens and Yaksh, 1986; Takemori et al., 1993).Other studies have also demonstrated that i.c.v. injection ofDyn A and related peptides in mice and rats produce motor effects,such as wild running, jumping, circling, barrel rolling and ataxia,through nonopioid mechanisms (Herman et al., 1980; Nakazawa etal., 1989; Walker et al., 1982). The Dyn A analog Dyn A-(1-13)-Tyr-Leu-Phe-Asn-Gly-Pro(Dyn Ia, i.c.v.), is one of the most potent peptides that producedmotor effects in mice, and such effects were blocked by the noncompetitiveNMDA receptor antagonists metaphit, dextromethorphan and ketamine(Shukla et al., 1992).

A particular role for the NMDA receptor in the nonopioid effects of Dyn A was first suggested by Faden (1992). The NMDA receptoris an inotropic excitatory amino acid receptor involved in centralkey functions that include synaptic plasticity, learning and memoryprocesses as well as neurodegeneration (Collingridge and Bliss,1995; Malenka and Nicoll, 1993; Wong and Kemp, 1991). This receptorcomprises various binding domains for compounds that modulateits activity (MacDonald and Mowak, 1990; Wong and Kemp, 1991).Glycine and polyamines exert positive modulatory actions on thestimulation of the receptor by the excitatory amino acids glutamicacid and aspartic acid, whereas PCP, Mg⁺⁺ and Zn⁺⁺ negatively modulate the receptor. Competitive NMDA antagonists,such as CGP 39653 (Sills et al., 1991), interact directly on theexcitatory amino acid binding domain and compete with glutamicacid and aspartic acid to block their activity. On the other hand,noncompetitive NMDA antagonists, such as MK-801 [(+)-5-methyl-10,11-dihydro-5H-dibenzo[a,d]cyclohepten-5,10-iminemaleate] (Sircar et al., 1987), bind to the PCP site located insidethe NMDA receptor-linked ion channel and block its activity ina use-dependent manner (MacDonald and Mowak, 1990). Dyn A andrelated peptides have already been shown to interact with bothexcitatory amino acid and PCP binding domains on the NMDA receptorcomplex by their potentiation of [³H]CGP 39653 binding (Dumont and Lemaire, 1994b) and inhibitionof [³H]MK-801 binding (Hunter et al., 1994; Shukla et al., 1992), respectively.The possible involvement of any one of these two sites in thenonopioid motor effects of these peptides remains to be established.

The present study was aimed at investigating (1) the structure-activity relationship of the motor effects of Dyn A and relatedpeptides in mice, (2) the blockade of the motor effects with competitiveand noncompetitive NMDA receptor antagonists and (3) the structuralrequirement for the interaction of Dyn A and related peptideswith the glutamic acid and PCP binding domains on the NMDA receptorcomplex. A close correlation was made between the abilities ofthe peptides to enhance [³H]CGP 39653 binding and to produce motor dysfunction.

	Methods

Top Abstract Introduction Methods Results Discussion References

Animals. Male Swiss Webster mice [(SW)f BR] weighing between 20 and 25 g were housed five per cage in a room with controlled temperature(22 ± 2°C), humidity and artificial light (6:30 a.m. to 7:00 p.m.).A minimum of 10 animals were used per group. The animals had freeaccess to food and water and were used after a minimum of 4 daysof acclimation to the housing conditions. To avoid the diurnalvariations, all experiments were conducted between 9:00 a.m. and5:00 p.m. All experiments were authorized by the animal care committeeof the University of Ottawa in accordance with the guidelinesof the Canadian Council on Animal Care.

Drugs. Dyn A and related peptides used in the study were synthesized by solid-phase procedure (Merrifield, 1963) as described previously(Lemaire et al., 1986). The peptides were cleaved from the resinand deprotected with liquid hydrogen fluoride at 0°C in the presenceof anisole (10% v/v). The synthetic material was then purifiedby chromatography on Sephadex G-10 (medium size) and HPLC on NucleosilC18. The product (280 nm detection) obtained from HPLC was lyophilizedto give a final recovery of 20% to 25% (based on the startingBoc amino acid-resin). The identity and purity of the syntheticpeptides were verified by thin-layer chromatography, analyticalHPLC on Zorbax ODS C18 (0.3 × 25 cm column, Dupont) and aminoacid analysis of acid hydrolysates.

Naloxone hydrochloride (Endo Laboratories, Garden City, NY) was dissolved in sterile water just before use and injected s.c.in a volume of 10 ml/kg. Dextrorphan (Research Biochemicals, Natick,MA), MK-801 (Research Biochemicals) and CPP [(±)3-(2-carboxypiperazine-4-yl)-propyl-1-phosphonicacid; Tocris Neuramin, Essex, UK] were dissolved in water andcoinjected i.c.v. with Dyn A-(1-13).

Motor dysfunction assay. The procedure used to assay motor dysfunction is the same as that described previously (Shukla et al., 1992). Groups of 10mice each were injected i.c.v. with different doses of Dyn A orrelated peptides. The animals were observed during 30 min formotor effects, characterized by wild running, popcorn jumping,circling, barrel rolling and ataxia. The motor activity beganwithin 5 min and lasted for 1 to 2 min. In some animals, particularlyat higher doses of the peptides, episodes of motor activity wererecorded intermittently during the observation period. The animalswere scored as showing motor activity when one or more of theabove-mentioned responses were present. In each group, the numberof animals showing these behavioral signs of motor activity wasrecorded. The dose producing motor dysfunction in 50% mice (ED₅₀)and the potency ratios with 95% CL values were calculated accordingto the method of Litchfield and Wilcoxon (1949) using procedure47 of the computer program of Tallarida and Murray (1987). Theprotective effects of dextrorphan, MK-801 and CPP against DynA-(1-13) (20 nmol/mouse)-induced motor effects were analyzed byFisher's exact test using the GraphPAD INSTAT program (GraphPADSoftware, San Diego, CA).

Preparation of rat brain membranes. Six male Wistar rats were decapitated, and their whole brains were rapidly removed and homogenized in ice-cold Tris·HCl (5mM, pH 7.4; buffer A) with a glass-Teflon homogenizer. The homogenatewas centrifuged at 27,000 × g for 30 min. The pellet was resuspendedin buffer A and centrifuged at 27,000 × g for 30 min. The resultingpellet was homogenized and incubated on ice in a total volumeof 1.0 liter of buffer A supplemented with 0.3 M KCl for 60 min(Lee et al., 1982). The suspension was then centrifuged at 27,000× g for 30 min, and the pellet was resuspended in buffer A. Thiswashing procedure was repeated an additional three times, andthe final membrane pellet was resuspended in buffer A at a concentrationof 2.0 mg protein/ml (Lowry et al., 1951) and kept frozen at $-$ 90°C.

[³H]MK-801 binding assay. Rat brain membranes (0.8 mg) were incubated in 2 ml of buffer A and enzyme inhibitors bestatin (30 µM), bacitracin (25 µM),captopril (10 µM) and thiorphan (0.3 µM) and 5.0 nM [³H]MK-801 at 22°C for 30 min in the absence and presence of theindicated concentration of Dyn A or related peptides. Bindingwas terminated by rapid filtration over Whatman GF-93488 filters.The filters were washed four times with 3 ml of ice-cold bufferA, placed in vials containing 10 ml of Ecolume and counted ina Beckman Beta counter LS 7800 at 40% efficiency. The specificbinding was evaluated using the difference between the countsin the presence and absence of 10 µM MK-801. The concentrationsof the peptides that produced 50% inhibition of the binding oftritiated ligand (IC₅₀) were derived using the nonlinear regressioncurve-fitting program GraphPAD INPLOT. K_i values were calculatedusing the equation of Cheng and Prusoff (1973), and results areexpressed as the mean ± S.E.M. of five duplicated sets of experiments.Statistical significance was measured by the Student's t test.

[³H]CGP-39653 binding assay. The ability of Dyn A and its analogs to potentiate the binding of [³H]CGP-39653 to rat brain membranes was measured as described previously(Dumont and Lemaire, 1994b). The rat brain membranes were preparedas described by Sills et al. (1991). [³H]CGP-39653 (5 nM) binding was performed in 2 ml of Tris·HCl (5mM, pH 7.7; buffer B) at 4^o for 60 min, containing 30 µM bestatin, 25 µM bacitracin, 10 µMcaptopril, 0.3 µM thiorphan and 0.8 mg of rat brain membranes.The binding was stopped by filtration as described above. Specificbinding was defined as the difference between the total radiolabelbound and that bound in the presence of 10 µM CPP. The potentiationof [³H]CGP-39653 binding by Dyn A and its analogs (10 µM) was expressedas the percent increase over the control binding activity in theabsence of the peptide. Experiments were repeated five times induplicate, and results are the mean ± S.E.M. values. Statisticalsignificance was determined using one-way analysis of variancefollowed by the Newman-Keuls test.

	Results

Top Abstract Introduction Methods Results Discussion References

Motor effects of Dyn A and related peptides. The i.c.v. administration of Dyn A (5-30 nmol/mouse), Dyn A-(1-13) (5-30 nmol/mouse), Dyn A-(1-8) (10-60 nmol/mouse), DynB (20-100 nmol/mouse) and $alpha$ -Neo-End (5-100 nmol/mouse) showeddose-dependent motor effects characterized by wild running, jumping,circling and barrel rolling (fig. 2A). Dyn A (ED₅₀ = 14.32 nmol/mouse)and Dyn A-(1-13) (ED₅₀ = 14.40 nmol/mouse) were equipotent inproducing motor effects (table 1). $alpha$ -Neo-End (ED₅₀ = 32.97 nmol/mouse),Dyn A-(1-8) (ED₅₀ 42.08 = nmol/mouse) and Dyn B (ED₅₀ = 45.01nmol/mouse) were significantly less potent compared with Dyn Ain producing motor effects. Leu-Enk (20-100 nmol/mouse) did notshow any motor activity (table 1).

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Fig. 2. Dose-response curves for the motor effects of i.c.v. administration of Dyn A and related opioid (A) and nonopioid (B) peptides.

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TABLE 1
Relative potencies of Dyn A and related peptides in producing motor effects in mice

The nonopioid fragments [Ala¹]Dyn A-(1-13) (10-60 nmol/mouse), Dyn A-(2-13) (10-60 nmol/mouse) and Dyn A-(2-8) (10-100 nmol/mouse)also showed dose-dependent motor effects after i.c.v. administration(fig. 2B). [Ala¹]Dyn A-(1-13) (ED₅₀ = 26 nmol/mouse), Dyn A-(2-13) (ED₅₀ = 28.82nmol/mouse) and Dyn A-(2-8) (ED₅₀ = 47.01 nmol/mouse) were significantlyless potent than Dyn A-(1-13) and Dyn A in producing motor effects(table 1). Dyn A-(3-8) showed motor effects in 33% of mice atthe dose of 100 nmol/mouse. Dyn A-(6-10) (20-100 nmol/mouse) didnot show any motor effect (table 1). The overall rank order ofpotency of the different Dyn A-related peptides was Dyn A $sime$ DynA-(1-13)> [Ala¹]Dyn A-(1-13) $sime$ Dyn A-(2-13) > $alpha$ -Neo-End > Dyn A-(1-8) $sime$ Dyn B $sime$ Dyn A-(2-8) >>> Dyn A-(3-8). Pretreatment of mice with naloxone(5 mg/kg s.c.) did not affect the potencies of Dyn A and Dyn A-(2-13)(table 2).

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TABLE 2
Effect of preadministration (15 min) of naloxone (5 mg/kg s.c.) on the potencies of Dyn A-(1-13) and Dyn A (2-13) in producingmotor effects in mice

To verify the possible involvement of the NMDA receptor in the motor effects of Dyn A-(1-13), the peptide was coadministeredwith competitive or noncompetitive NMDA antagonists (fig. 3).Coinjection of Dyn A-(1-13) (20 nmol/mouse i.c.v.) with dextrorphan(0.2, 0.3 and 0.6 nmol/mouse i.c.v.) or MK-801 (0.3 and 0.4 nmol/mousei.c.v.) or CPP (0.3 and 0.4 nmol/mouse) produced significant (P< .05) blockades of its motor effects. Coinjection of the peptidewith higher doses of the NMDA antagonists showed some decreasein protective activities (fig. 3).

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Fig. 3. Percent protection of different doses of the NMDA antagonists dextrorphan, MK-801 or CPP against the motor effects of DynA-(1-13). NMDA antagonists were coadministered at the indicateddoses with Dyn A-(1-13) (20 nmol/mouse i.c.v.)., which alone producedmotor effects in 90% of tested mice. P < .05 was considered significant.

Competition with [³H]MK-801 binding to rat brain membranes. Various Dyn A-related peptides were also tested for their ability to compete with the binding of [³H]MK-801 to rat brain membranes (fig. 4; table 3). Dyn A-(1-13)was 2-fold more potent than Dyn A in inhibiting the binding of[³H]MK-801 (5 nM), with a K_i value of 0.21 µM compared with 0.41µM for Dyn A. The order of potency of the various Dyn A-relatedpeptides in the binding assay was distinct from that mentionedabove for the production of motor effects: Dyn A-(1-13) > DynA > [Ala¹]Dyn A-(1-13) > Dyn A-(1-9) > Dyn B > $alpha$ -Neo-End > Dyn A-(1-8).Dyn A-(2-13), Dyn A-(3-13), Dyn A-(2-8) and Dyn A-(1-5) were inactiveat concentrations up to 10 µM. In addition, the ability of DynA-(1-13) to displace [³H]MK-801 binding was not affected by 10 µM naloxone (fig. 4).

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Fig. 4. Concentration-dependent inhibition of [³H]MK-801 binding with Dyn A-(1-13) in the absence ( $open circle$ ) or presence of 10 µM of naloxone( $diamond$ ). The results are expressed as the mean ± S.E.M. of five experimentsconducted in duplicate.

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TABLE 3
Relative potencies of Dyn A and related peptides and fragments in competing with the binding of [³H]MK-801 to rat brain membranes

Potentiation of [³H]CGP-39653 binding. Dyn A-(1-13) was previously shown to potentiate the binding of the NMDA receptor antagonist [³H]CGP-39653 to rat brain membranes (Dumont and Lemaire, 1994b).Figure 5 illustrates the effects of Dyn A and various relatedpeptides on such binding activity. Among the opioid peptides,Dyn A and Dyn A-(1-13) (10 µM) were equipotent and caused a 2.9-foldincrease in [³H]CGP-39653 binding, followed by $alpha$ -Neo End and Dyn A-(1-8), whichshowed 2.3- and 1.4-fold increases, respectively. Dyn B, Dyn A-(3-8)and Leu-Enk showed no significant potentiation (fig. 5). The nonopioidDyn A-related peptides Dyn A-(2-13) and [Ala¹]Dyn A-(1-13) were also able to enhance the binding of [³H]CGP-39653, displaying 2.4- and 2.3-fold stimulations, respectively.However, Dyn A-(2-8) was less potent and showed only a 1.4-foldincrease in the binding activity. Comparison between the potenciesof the various peptides in producing motor effects (table 1)and potentiating the binding of [³H]CGP-39653 (fig. 4) provided a good correlation with an r valueof 0.91 (fig. 6). The potentiation of [³H]CGP-39653 binding by Dyn A-(1-13) (10 µM) was nonopioid, beingnot affected by naloxone (10 µM; data not shown).

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Fig. 5. Effect of Dyn A and related peptides (10 µM) on the binding of [³H]CGP-39653 (5 nM) to rat brain membranes. The results representthe mean ± S.E.M. of five experiments conducted in duplicate.**, P < .01, and *, P < .05 compared with control.

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Fig. 6. Correlation between the abilities of Dyn A and related peptides to produce motor effects and potentiate [³H]CGP 39653 binding. The potency ratio obtained in table 1 wasplotted in comparison with the potency ratio derived from figure5, using Dyn A for maximal effect.

	Discussion

Top Abstract Introduction Methods Results Discussion References

Dyn A and related peptides, when administered i.c.v. or into other brain regions, produce motor dysfunction such as wild running,jumping, circling, barrel rolling, ataxia and unusual contortedposture (Nakazawa et al., 1989; Walker et al., 1982). In the corticalEEG recordings, Dyn A (i.c.v.) or [des-Tyr¹]Dyn A induced large-amplitude slow-wave EEG activity in rats(Walker et al., 1982). These Dyn-induced motor effects and changesin cortical EEG activity were not antagonized by preadministrationof naloxone, suggesting the involvement of some nonopioid mechanism(Walker et al., 1982). Here, we found that i.c.v. injections ofDyn A and related peptides in mice produce dose-dependent motoreffects. The nonopioid nature of the motor effects of these peptideswas demonstrated by their insensitivity to naloxone pretreatmentand the high potencies of the nonopioid Dyn A analogs or fragments,such as [Ala¹]Dyn A-(1-13), Dyn A-(2-13) and Dyn A-(2-8). Dyn A-(2-8) was foundto be the minimal active core of the peptide. The same minimalcore peptide was previously reported for the suppression of naloxone-precipitatedopioid withdrawal syndrome in morphine-dependent mice (Takemoriet al., 1993).

There have been numerous reports concerning the involvement of the NMDA receptor complex in the central nonopioid effectsof Dyn A and related peptides (for a review, see Shukla and Lemaire,1994). We previously found that the motor effects induced by DynIa are altered by preadministration of the noncompetitive NMDAreceptor antagonists metaphit, dextromethorphan and ketamine (Shuklaet al., 1992). In the present study, the motor effects of DynA-(1-13) were almost completely blocked by coadministration ofthe peptide with a low concentration (0.3 nmol/mouse) of the noncompetitiveNMDA antagonist dextrorphan (fig. 2). The competitive and noncompetitiveNMDA antagonists CPP and MK-801 displayed significant but onlypartial blockades of Dyn A-(1-13)-induced motor activity. Thedecreased protective activity of these compounds at higher dosesmay be due to their ability to cause motor effects of their own(Koek and Colpaert, 1990).

The NMDA receptor comprises various binding domains that regulate its activity. Thus, in addition to the site for the excitatoryamino acid (glutamic acid or aspartic acid), there exists sitesfor glycine, PCP, polyamines and divalent ions (Mg⁺⁺ and Zn⁺⁺), which modulate the entry of Ca⁺⁺ and Na⁺ consecutive to the stimulation-induced opening of the receptor-linkedion channel (Wong and Kemp, 1991). To verify whether the motoreffects of Dyn A and related peptides could be due to their interactionwith the PCP receptor, we measured their ability to compete withthe binding of the specific PCP receptor ligand [³H]MK-801 to rat brain membranes (table 3). Dyn A and relatedpeptides did compete with the binding of [³H]MK-801, but their order of potency was distinct from that observedfor motor activity (table 1). Thus, the nonopioid peptides DynA-(2-13) and Dyn A-(2-8), which produced marked motor activity,did not decrease the binding of [³H]MK-801. On the other hand, Dyn B, Dyn A-(1-8) and $alpha$ -Neo-Enddisplayed <10% of the potency of Dyn A-(1-13) in the [³H]MK-801 binding assay while exhibiting >30% of the potency ofDyn A-(1-13) in the motor dysfunction assay. Hence, the interactionof Dyn A and related peptides with the PCP binding domain on theNMDA receptor complex is more likely not responsible for theirmotor activity but rather may be involved in some other nonopioideffects of the peptides, such as the nonopioid component of theiranalgesic activity (Hooke et al., 1995).

Recently, we reported that the binding of the competitive NMDA receptor antagonist [³H]CGP-39653 is significantly enhanced by Dyn A and related peptides(Dumont and Lemaire, 1994b). To verify whether the motor effectsof Dyn A and related peptides were due to their interaction withthe [³H]CGP 39653 binding site (i.e., the excitatory amino acid bindingdomain on the NMDA receptor complex), we studied their abilityto potentiate [³H]CGP 39653 binding to rat brain membranes. The results indicatethat Dyn A and some related peptides, including the nonopioidpeptides [Ala¹]Dyn A-(1-13), Dyn A-(2-13) and Dyn A-(2-8), markedly increasethe binding of [³H]CGP 39653 (fig. 5), which is in good correlation with theirmotor activity (table 1). The correlation coefficient that wasobtained between the order of potency of these peptides to enhance[³H]CGP 39653 binding and display motor activity approached unity(r = 0.91; fig. 6). Thus, the motor impairment caused by Dyn Aand related peptides may be due to their interaction with theexcitatory amino acid binding domain on the NMDA receptor complex,possibly resulting in a potentiation of the action of endogenousglutamic acid or aspartic acid. These data are in accordance withprevious results that indicated that the motor effects of thiopeptideanalogs of Dyn A-(1-9) correlate well with their ability to interactwith the glutamic acid site on the NMDA receptor complex (Le etal., 1997).

Dyn A was shown to produce both stimulatory (Walker et al., 1982) and inhibitory (Wagner et al., 1993) effects on the centralnervous system. The stimulatory effects are nonopioid, whereasthe inhibitory effects involve the participation of kappa opioidreceptors. The interaction of Dyn A with the NMDA receptor hasbeen suggested to be responsible of various physiological andpathophysiological phenomena, including allodynia (Nichols etal., 1997; Vanderah et al., 1996), hyperalgesia (Dubner and Ruda,1992), blockade of morphine tolerance (Takemori et al., 1993)and sensitivity to kindling manifested by seizure (Elmer et al.,1996). The mechanism by which Dyn A may potentiate the actionof excitatory amino acids on the NMDA receptor remains to be defined,but our findings of a direct interaction of the peptide with theglutamic acid site and of a correlation between this interactionand its NMDA-mediated motor effects are supported by the previouslyobserved displacement of [³H]glutamic acid binding by Dyn A-(1-13) (Massardier and Hunt,1989) and potentiation by this same peptide of NMDA-induced bitingand scratching behavior (Skilling et al., 1992). Therefore, theinteraction of Dyn A with the excitatory amino acid binding domainon the NMDA receptor complex may potentiate the action of endogenousexcitatory amino acids and thus participate in various NMDA receptor-mediatedbehavioral and neuroplastic activities.

	Footnotes

Accepted for publication July 11, 1997.

Received for publication March 27, 1997.

¹ This work was supported by the Medical Research Council of Canada.

Send reprint requests to: Simon Lemaire, Ph.D., Department of Pharmacology, Faculty of Medicine, University of Ottawa, 451 Smyth Road, Ottawa, Ontario, Canada K1H 8M5.

	Abbreviations

i.c.v., intracerebroventricular; s.c., subcutaneous; CL, confidence limit; EEG, electroencephalographic; Dyn A, dynorphin A; Leu-Enk, Leu-enkephalin; $alpha$ -Neo-End, $alpha$ -Neo-endorphin; NMDA, N-methyl-d-aspartate; AMPA, $alpha$ -amino-3-hydroxy-5-methyl-isoxazole-4-propionate; PCP, phencyclidine.

	References

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