Inhibition of Nitric Oxide Synthase Enhances Antinociception Mediated by Mu, Delta and Kappa Opioid Receptors in Acute and Prolonged Pain in the Rat Spinal Cord

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Pain

Vol. 282, Issue 2, 977-984, 1997

Inhibition of Nitric Oxide Synthase Enhances Antinociception Mediated by Mu, Delta and Kappa Opioid Receptors in Acute and Prolonged Pain in the Rat Spinal Cord¹

Halina Machelska, Dominika $L$ abuz, Ryszard Przew $l$ ocki and Barbara Przew $l$ ocka

Department of Molecular Neuropharmacology, Institute of Pharmacology, Polish Academy of Sciences, Cracow, Poland

	Abstract

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Our study was designed to determine involvement of nitric oxide (NO) in the antinociception mediated by mu, delta and kappaopioid receptors in acute and prolonged pain in the rat spinalcord. The effect of intrathecally (i.t.) injected NO synthaseinhibitors and opioid receptor agonists was evaluated in acutepain using a tail-flick and a paw pressure tests, and in prolongedpain by quantification the pain-related behavior after peripheralformalin injection. It was found that the neuronal NO synthaseinhibitor 7-nitroindazole (50-400 µg), used in inactive doses,dose-dependently enhanced antinociception induced by morphine(0.5 µg) in the tail-flick and paw pressure. Moreover, coadministrationof N^G-nitro-L-arginine methyl ester (50 µg) another NO synthase inhibitor,with morphine (0.05-0.5 µg) as well as with specific agonistsof mu ([D-Ala²,N-Me-Phe⁴,Gly-ol⁵]enkephalin 0.1-2.5 ng) and delta ([D-Pen^2,5]enkephalin 0.02-0.5 µg) opioid receptors, enhanced dose-dependentantinociception in the tail-flick and paw pressure. Coadministrationof N^G-nitro-L-arginine methyl ester with specific kappa opioid receptoragonist 3,4-dichloro-N-methyl-N-[2-(1-pyrrolidinyl)cyclohexyl]-benzenacetamide(10-100 µg), produced antinociception in the paw pressure only.Additionally, N^G-nitro-L-arginine methyl ester (100 µg) profoundly potentiatedthe antinociception induced by [D-Ala²,N-Me-Phe⁴,Gly-ol⁵]enkephalin (0.5, 15 ng) and [D-Pen^2,5]enkephalin (2, 10 µg) in the dose-related manner in the formalintest. N^G-nitro-L-arginine methyl ester (100 µg) also enhanced the antinociceptioninduced by 3,4-dichloro-N-methyl-N-[2-(1-pyrrolidinyl)cyclohexyl]-benzenacetamide(10-100 µg) but only at the last two time points of the secondphase of the formalin test. These data show that inhibition ofthe spinal NO synthase potentiates the mu-, delta- and to a lesserextent, kappa-mediated spinal antinociception in both acute andprolonged pain.

	Introduction

Top Abstract Introduction Methods Results Discussion References

Despite many years of research, the mechanisms involved in the analgesic action of opioids have yet to be identified. Someprevious evidence has suggested that EAAs are involved in nociceptivetransmission, and that opioid peptides modulate responses to glutamateand its analogs, especially in the spinal cord. It was found thatthe spinal NMDA-induced hyperalgesia was abolished by i.t. injectedopioids (Aanonsen and Wilcox, 1987), and that NMDA receptor antagonistscoadministered with morphine facilitated antinociception at alevel of the spinal cord (Chapman and Dickenson, 1992). It wasalso observed that the release of glutamate and aspartate fromrat spinal cord slices was attenuated by opioids (Kangrga andRandi $c'$ , 1991). These results are supported by immunohistochemicaland autoradiographic data showing the existence of glutamate,aspartate (De Biasi and Rustioni, 1988) and opioid peptides (Khachaturianet al., 1993), as well as NMDA (Kus et al., 1995) and opioid receptors(Yaksh, 1993) in the substantia gelatinosa of the rat spinal cord.It appears that many of the NMDA effects are mediated by NO thatis synthetized from amino acid L-arginine after stimulation ofNO synthase by Ca⁺⁺that fluxes into the cell subsequently to NMDA receptor activation.The consequences of NO production are activation of soluble guanylatecyclase and elevation of the cGMP level (Garthwaite et al., 1988;Bredt and Snyder, 1992; Bruhwyler et al., 1994; Garthwaite andBoulton, 1995). Accordingly, in the spinal cord, NO synthase wasfound predominately in superficial layers of the dorsal horn andaround the central canal, i.e., regions preferentially involvedin the sensory transmission (Dun et al., 1993), and an increasedexpression of NO synthase and/or NADPH-diaphorase a histochemicalmarker of NO synthase, in the dorsal horn of the spinal cord wasobserved after noxious stimulation of the rat hind paw (Solodkinet al., 1992; Fiallos-Estrada et al.,1993; Herdegen et al., 1994,Lam et al., 1996). Moreover, it was found that the NMDA-inducedrelease of NO from the rat spinal cord was blocked by NO synthaseinhibitors (Ping et al., 1994), and the spinal NMDA-induced hyperalgesiawas reduced by i.t. administered inhibitors of NO synthase andguanylate cyclase (Kitto et al., 1992; Meller et al., 1992; Melleret al., 1996). Recent evidence suggests involvement of NO in opioid-mediatedeffects. Thus it was found that the inhibition of NO synthaseattenuates tolerance to the antinociceptive action of morphine(Kolesnikov et al., 1992; Majeed et al., 1994; Bhargava and Zhao,1996) and enhances the spinal morphine-induced antinociceptionin the rat (Przew $l$ ocki et al., 1993). Summing up, the data presentedabove suggest a possible interaction between NO and opioid systems.

Opioid drugs exert their antinociceptive effect by interacting with three types of receptors, i.e., mu, delta and kappa. Theantinociceptive effect of mu and delta receptor agonists afteri.c.v., as well as i.t., administration has been demonstrated(Porreca and Burks, 1993; Yaksh, 1993), but there is some controversyabout the kappa-mediated antinociception. In contrast to antinociceptionin the spinal cord, lack of an antinociceptive action of kappareceptor agonists was found at supraspinal sites (Walker et al.,1982). However, the activation of spinal kappa receptors was reportedto be less effective in eliciting antinociception in comparisonwith the activation of spinal mu and delta receptors (Yaksh, 1993).Moreover, some of the kappa receptor-induced effects appearedto be mediated in a nonopioid manner (Przew $l$ ocki et al., 1983).Antinociceptive effects of exogenously applied opioid receptoragonists were also observed after prolonged noxious stimulation(Porro and Cavazzuti, 1993), which is associated with long-lastingtissue damage, inflammation or neuropathologies and results froma number of complex changes in nociceptive pathways, being probablymodulated in the central nervous system in a different way thanthe pain elicited by short-lasting stimuli (Dray et al., 1994).There is a growing body of evidence that endogenous opioid peptidesystems reveal differential and tissue-specific alternations intheir activity on long-term noxious stimulation. An enhanced activityof the proenkephalin system is elicited by noxious stimulationof a limited duration, whereas an increase in the biosyntheticactivity of the prodynorphin system evokes a most striking andprotracted response to chronic pain, especially in the spinalcord (Przew $l$ ocka et al., 1992; Millan, 1993).

In view of differential involvement of opioid peptides in nociceptive transmission and influence of NO on opioid-mediatedeffects, the aim of our study was to find out to which extentNO is involved in antinociceptive effects of multiple opioid receptoragonists at a level of the rat spinal cord in both acute and prolongedpain.

	Methods

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Animals

Male Wistar rats (300-400 g) from Laboratory Animals Breeding Center (Rembertow, Poland), were used. The rats were housedin single cages lined with sawdust, on a standard 12 hr/12 hrlight-dark cycle (8.00 A.M./8.00 P.M.), with food and water adlibitum.

The rats were chronically implanted with i.t. catheters under hexobarbital anaesthesia. They were placed in the David Kopfstereotaxic table, and an incision was made in the atlanto-occipitalmembrane. A catheter (PE 10, Clay Adams) was carefully introducedto the subarachnoid space at the rostral level of the spinal cordlumbar enlargement according to Yaksh and Rudy (1976). Only animalswith a normal motor function were used. Intrathecal injectionstudies were carried out 5 to 14 days after the surgery. Drugswere dissolved in distilled water and were injected in a volumeof 5 µl (single injections) or 10 µl (coadministration), followedby an injection of 10 µl of distilled water to flush the catheter.In different experiments used in this study, control animals wereinjected i.t. with distilled water and were tested according tothe same time schedule as described below for the experimentalgroups. After completing the experiment, the animals were killedwith an overdose of pentobarbital (i.p.).

Analgesia Testing

Acute pain. Antinociceptive effects were evaluated using TF and PP tests. The TF test was carried out using an Analgesia Meter apparatus(mod 33, IITC Inc., Landing, NJ). The animal was gently restrainedby hand, and radiant heat was directed onto the animal's tail.The cut-off time was 8 or 16 sec (the latter in experiments withU50,488H). The PP threshold (Randall-Selitto test), necessaryto elicit paw withdrawal, was determined using an automatic gauge(Ugo Basile). The animal was gently restrained and an incrementalpressure was applied via a piston onto the dorsal surface of thehind paw. The cut-off pressure was 480 g. TF and PP measurementswere taken three times at 15- or 10-sec intervals, respectively,and their mean was used for calculations.

Inhibitors of NO synthase were coadministered with opioid receptor agonists, and the measurements were carried out at 15,30, 60 min after 7-NI (50, 100, 400 µg) plus morphine (0.5 µg),at 30 min after L-NAME (50 µg) plus morphine (0.05, 0.1, 0.5 µg)and at 15 min after L-NAME (50 µg) plus DAMGO (0.1, 0.5, 2.5 ng)or DPDPE (0.02, 0.1, 0.5 µg) or U50,488H (10, 50, 100 µg).

Prolonged pain. The rats were lightly anaesthetized with ether, and 100 µl of a 12% formalin solution was injected s.c. into the dorsal surfaceof the left hind paw. The rat was then placed in a wire cage forobservation of the formalin-injected paw. The pain-related behaviorwas quantified by counting spontaneous flinches and shakes ofthe injected paw. The flinches and shakes were counted for eachanimal at several time points: at 0 to 10 min (first phase) andat 10 to 15, 25 to 30, 35 to 40, 45 to 50, 70 to 75 min (secondphase) after formalin administration.

The rats were injected i.t. with L-NAME (100, 400 µg), DAMGO (0.5, 15, 500 ng), DPDPE (2, 10, 50 µg) or U50,488H (10, 50,100 µg) at 7 min before formalin administration. In the experimentsin which the influence of the NO synthase inhibitor on the opioidreceptor agonists-induced antinociception was evaluated, L-NAME(100 µg) was coadministered with DAMGO (0.5, 15 ng), or DPDPE(2, 10 µg) or U50,488H (10, 50, 100 µg).

Drugs

DAMGO, DPDPE, U50,488H, L-NAME, 7-NI were purchased from RBI (Natick, MA); morphine was obtained from Polfa (Kutno, Poland).

Data Analysis

The results were statistically assessed by an analysis of variance. Intergroup differences were analyzed by Duncan's multiple-rangetest.

	Results

Top Abstract Introduction Methods Results Discussion References

Acute Pain

The effect of NO synthase inhibition on the antinociceptive effects of opioids, evaluated by the TF and PP tests. 7-NI (50, 100, 400 µg) used in doses which had no effect on the baseline TF and PP latencies (fig. 1), dose-dependently enhancedthe effect of morphine (0.5 µg) in both those tests (fig. 1).Morphine given in the above dose caused mild but significant antinociceptionat 15 min after injection in the TF test. The morphine-inducedeffect was significantly potentiated by 7-NI at 30 min (100 µg)and 15 to 30 min (400 µg) after their coadministration. In thePP test, morphine (0.5 µg) did not influence the pain threshold,but its coadministration with 7-NI produced antinociception whichoccurred after 15 min (50 µg) and 15 to 30 min (100, 400 µg) (fig.1).

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Fig. 1. The effect of 7-nitroindazole (7-NI; 50-400 µg) on the morphine (MOR; 0.5 µg)-induced antinociception after their i.t. coadministration,evaluated by the tail-flick (TF) and paw pressure (PP) tests inthe rat. Control animals were injected i.t. with distilled waterand were tested according to the same time schedule as experimentalgroup. 7-NI used in the above doses did not influence the baselineTF (the results were as follows: 50 µg, 3.7 ± 0.3, 3.5 ± 0.1,3.6 ± 0.4, 3.8 ± 0.6; 100 µg, 3.7 ± 0.5, 4.1 ± 0.6, 3.6 ± 0.3,3.7 ± 0.3; 400 µg, 3.7 ± 0.4, 3.6 ± 0.1, 3.8 ± 0.5, 3.8 ± 0.4after 0, 15, 30 and 60 min, respectively) and PP values (the resultswere as follows: 50 µg, 200 ± 3.8, 202 ± 3.2, 196 ± 2.4, 209 ±5.2; 100 µg, 206 ± 2.6, 209 ± 0.6, 208 ± 4.6, 208 ± 5.2; 400 µg,208 ± 4.0, 198 ± 2.2, 207 ± 5.8, 202 ± 2.4 after 0, 15, 30 and60 min, respectively). The data are presented as mean ± S.E.M.+Indicates a significant difference (P < .05) between morphineand control. *Indicates a significant difference (P < .05) between7-NI + morphine and morphine alone. The number of animals usedfor each dose was 6 to 11.

L-NAME (50 µg) and morphine (0.05, 0.1, 0.5 µg), applied in doses that did not significantly influence nociceptive reflexes,produced dose-dependent antinociception at 30 min after theircoadministration. A statistically significant effect was observedafter coadministration of L-NAME with the highest dose of morphinein the TF test, and with all the three doses of the latter inthe PP test (fig. 2A). Similar effects were reported at 15 minafter coadministration of L-NAME (50 µg) with DAMGO (0.1, 0.5,2.5 ng) and L-NAME (50 µg) with DPDPE (0.02, 0.1, 0.5 µg), specificmu and delta opioid receptor agonists, respectively. A statisticallysignificant antinociception was evaluated after coadministrationof L-NAME with two higher doses of DAMGO, as well as two higherdoses of DPDPE in both the TF and PP tests (fig. 2, B and C).Mild, yet significant antinociception was observed in the PP testat 15 min after coadministration of L-NAME (50 µg) with the twohigher doses of U50,488H (50, 100 µg), a specific kappa opioidreceptor agonist. No significant antinociception was found afterL-NAME injected concomitantly with U50,488H in the TF test (fig.2D). DAMGO, DPDPE and U50,488H were used in doses which had noeffect on the baseline TF and PP latencies (fig. 2, B-D).

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Fig. 2. The dose-response relationship evaluated at 30 min after i.t. coadministration of L-NAME (50 µg) with morphine (0.05-0.5 µg)(A), and at 15 min after i.t. coadministration of L-NAME (50 µg)with DAMGO (0.1-2.5 ng) (B), L-NAME (50 µg) with DPDPE (0.02-0.5µg) (C) and L-NAME (50 µg) with U50,488H (10-100 µg) (D) in thetail-flick (TF) and paw pressure (PP) tests in the rat. Controlanimals were injected i.t. with distilled water and were testedaccording to the same time schedule as experimental group. Thedata are presented as mean ± S.E.M. *Indicates a significant difference(P < .05) between L-NAME coadministered with opioid receptor agonistsand L-NAME as well as opioid receptor agonists alone. The numberof animals used for each dose was 6 to 9.

Prolonged Pain

The effect of NO synthase inhibition on the antinociceptive effects of opioids, evaluated in the formalin test. L-NAME injected in a dose of 100 µg significantly suppressed the formalin-induced behavior in the first, but not the secondphase of the formalin test. L-NAME in a dose of 400 µg did notinfluence the first phase of the formalin test, but produced significantattenuation of the second phase (fig. 3).

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Fig. 3. The effect of i.t. administered L-NAME (100-400 µg) on the formalin-induced nociception in the rat. L-NAME was administered7 min before peripheral formalin administration. The labels onthe x-axis indicate the end of a 10-min period of counting flinchesand shakes in the first phase (0-10 min), and the end of 5-minperiods at several time points of the second phase (10-75 min)of the formalin test. The data are presented as mean ± S.E.M.*Indicates a significant difference (P < .05) between L-NAME andvehicle-treated control. The number of animals used for each dosewas 8 to 25.

DAMGO (0.5, 15, 500 ng), DPDPE (2, 10, 50 µg) and U50,488H (10, 50, 100 µg) produced significant, dose-dependent inhibitionof the formalin-induced behavior (fig. 4). DAMGO and DPDPE inall of the three doses tested and U50,488H in a dose of 100 µgattenuated the first phase of the formalin response. The secondphase was significantly attenuated by DAMGO, DPDPE and U50,488Hinjected in the two higher doses. Statistically significant effectswere observed at 15 to 30 min (15 ng) and at 15 to 50 min (500ng) after administration of DAMGO at 30 to 50 min after administrationof DPDPE given in doses of 10 and 50 µg and at 30 to 40 min (50µg) and at 30 to 50 min (100 µg) after administration of U50,488H(fig. 4).

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Fig. 4. The effects of i.t. administered DAMGO (0.5-500 ng), DPDPE (2-50 µg) and U50,488H (10-100 µg) on the formalin-induced nociceptionin the rat. Opioid receptor agonists were administered 7 min beforeperipheral formalin administration. The labels on the x-axis indicatethe end of a 10-min period of counting flinches and shakes inthe first phase (0-10 min), and the end of 5-min periods at severaltime points of the second phase (10-75 min) of the formalin test.The data are presented as mean ± S.E.M. *Indicates a significantdifference (P < .05) between opioid receptor agonists and vehicle-treatedcontrol. The number of animals used for each dose was 8 to 25.

No potentiation of the DAMGO- (15 ng) induced antinociception by L-NAME (100 µg) was observed in the first phase of the formalintest (fig. 5). However, L-NAME coadministered with DAMGO significantlypotentiated its antinociceptive effect in the second phase (25-50min) of the formalin response (fig. 5). When injected alone L-NAME(100 µg) did not influence the second phase of the formalin test,and DAMGO (15 ng) caused only mild, but significant, suppressionof that phase (15-30 min) (figs. 3, 4, 5). L-NAME (100 µg) didnot influence antinociception induced by DAMGO given in a doseof 0.5 ng as evaluated at 35 to 40 min after formalin injection(fig. 6).

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Fig. 5. The time course of i.t. administered L-NAME (100 µg) on the antinociception induced by i.t. administered DAMGO (15 ng), DPDPE(10 µg) and U50,488H (50 µg) in the formalin test in the rat.L-NAME and opioid receptor agonists were coadministered 7 minbefore peripheral formalin administration. Control animals receivedinjections i.t. with distilled water and were tested accordingto the same time schedule as experimental group. The labels onthe x-axis indicate the end of a 10-min period of counting flinchesand shakes in the first phase (0-10 min), and the end of 5-minperiods at several time points of the second phase (10-75 min)of the formalin test. The data are presented as mean ± S.E.M.*Indicates a significant difference (P < .05) between L-NAME coadministeredwith opioid receptor agonists and L-NAME as well as opioid receptoragonists alone. The number of animals used for each dose was 8to 25.

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Fig. 6. The dose-response relationship for i.t. administered L-NAME (100 µg) on the antinociception induced by i.t. administered DAMGO(0.5-15 ng), DPDPE (2-10 µg) and U50,488H (10-100 µg), evaluatedat 35 to 40 min after formalin injection to the rat. L-NAME andopioid receptor agonists were coadministered 7 min before peripheralformalin administration. Control animals received injections i.t.with distilled water and were tested according to the same timeschedule as experimental group. The data are presented as mean± S.E.M. *Indicates a significant difference (P < .05) betweenL-NAME coadministered with opioid receptor agonists and L-NAMEas well as opioid receptor agonists alone. The number of animalsused for each dose was 8 to 25.

L-NAME (100 µg) significantly potentiated the DPDPE- (10 µg) induced antinociception in the first, as well as in the secondphase (35-40 and 70-75 min) of the formalin test (fig. 5). Whenadministered alone L-NAME (100 µg) and DPDPE (10 µg) significantlysuppressed the first phase and DPDPE (10 µg) also attenuated thesecond phase (25-50 min) (figs 3, 4, 5). L-NAME (100 µg) causedmild, although not significant potentiation of the antinociceptioninduced by DPDPE given in a dose of 2 µg as evaluated at 35 to40 min after formalin injection (fig. 6).

The first phase of the formalin test was not significantly affected by coadministration of L-NAME (100 µg) and U50,488H (10,50, 100 µg) in any dose used (fig. 5). However, in the secondphase of the test, L-NAME (100 µg) potentiated the antinociceptioninduced by U50,488H given in a dose of 50 µg (fig. 5). A significanteffect was observed at the last two time points (45-75 min) ofthe second phase of the formalin test. When injected alone ina dose of 50 µg U50,488H significantly suppressed the formalin-inducedbehavior at the first two time points (25-40 min) of the secondphase (Figs. 4 and 5). L-NAME (100 µg) did not potentiate theeffect of U50,488H given in doses of 10 µg and 100 µg as evaluatedat 35 to 40 min after formalin injection (fig. 6).

	Discussion

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Our study shows that 7-NI, a specific inhibitor of neuronal NO synthase, enhances the antinociceptive effect of morphine aftertheir i.t. coadminstration to the rat in the TF and PP tests.This finding supports our previous results that showed that concomitanti.t. injection of L-NAME and morphine elicits strong and profoundantinociception in the rat (Przew $l$ ocki et al.,1993). Moreover,in our study we have found that i.t. coadministration of L-NAMEgiven in subanalgesic doses with morphine as well as with specificmu and delta opioid receptor agonists DAMGO and DPDPE, respectively,produces dose-dependent, strong antinociception in both the TFand PP tests. A similar, although weaker effect was reported aftercoadministration of L-NAME with U50,488H, a specific kappa receptoragonist, as evaluated by the PP test. Interestingly, no such effectwas observed in the TF test. Furthermore, our previous study showedpotentiation of the morphine-induced antinociception by hemoglobinthat binds the released NO (Przew $l$ ocki et al.,1993). Thus allthe above results indicate that NO in the spinal cord may be tonicallyactive in inhibiting morphine-activated nociceptive pathways.Our study is in line with the recent results of Xu and Tseng (1995)who reported that N-nitro-L-arginine, hemoglobin and methylene blue, an inhibitorof guanylate cyclase and/or NO synthase (Luo et al., 1995), injectedi.t. potentiate the antinociception induced by morphine administeredi.c.v. The above findings suggest that NO may exert a pronociceptiveaction at a level of the spinal cord. In fact, inhibition of NOsynthase in the spinal cord leads to antinociception (Meller andGebhart 1993; Przew $l$ ocki et al., 1993; Meller et al., 1996) andNO-donating substances administered i.t. produce hyperalgesiain response to acute nociceptive stimuli (Kitto et al., 1992;Shibuta et al., 1995; H. Machelska, R. Przew $l$ ocki, M. Radomskiand B. Przew $l$ ocka, unpublished data). These behavioral data aresupported by the results of biochemical studies that show thatin the spinal cord the NO donor enhances the release of substanceP and calcitonin gene-related peptide, both neuropeptides beingprincipally involved in the nociceptive transmission (Garry etal., 1994), while the NO synthase inhibitor attenuates the NMDA-inducedrelease of glutamate and citrulline a marker of NO release (Sorkin,1993). Immunohistochemical studies further confirm the pronociceptiveaction of NO, because it has been found that the c-fos expressioninduced by noxious mechanical stimuli is reduced by the NO synthaseinhibitor administered i.t. (Lee et al., 1992).

However, NO appears to act as a pronociceptive as well as an antinociceptive agent at supraspinal and peripheral sites. Ithas been found that L-NAME applied i.c.v. produces dose-relatedinhibition of the formalin-induced paw licking in mice (Mooreet al., 1991) and prolongation of the TF and PP latencies, whileNO donors administered i.c.v. shorten these latencies in the rat(Machelska et al., unpublished data). Conversely, NO donors havebeen also reported to exert an antinociceptive action when theyare injected both i.c.v. (Duarte and Ferreira, 1992) and i.pl.(Duarte et al., 1990; Ferreira et al., 1991). There are also someconflicting data on the influence of NO synthase inhibition onthe antinociception mediated by morphine at supraspinal and peripheralsites. It was found that the i.c.v. morphine-induced antinociceptionwas not affected by N-nitro-L-arginine, hemoglobin or methylene blue, injected i.c.v.(Xu and Tseng, 1995). In contrast, our experiments demonstratedpotentiation of the morphine-induced antinociception by L-NAMEafter their i.c.v. coadministration (data not shown). Moreover,Duarte and Ferreira (1992) found that the morphine-induced antinociceptionwas prevented by methylene blue, but not by N-iminoethyl-L-ornithine,after their i.c.v. administration as evaluated by the TF testin the rat. It was also found that the peripheral morphine-inducedantinociception was potentiated by the NO donor injected i.pl.(Ferreira et al., 1991).

Precise mechanisms underlying the opposing effect of NO on nociception are as yet unknown. However, some studies suggest thatNO may induce pronociceptive effects at low concentrations andantinociceptive ones at higher concentrations (Kawabata et al.,1994). Meller et al. (1992) demonstrated that low doses of NMDA,which possibly generate low concentrations of NO, produce hyperalgesia,whereas generation of higher levels of NO may be associated withthe antinociception produced by administration of higher dosesof NMDA. Additionally, Kawabata et al., (1993) suggested thatL-arginine, a substrate of NO, could play a dual role in the nociceptiveprocessing in the brain, depending on the pathway in which itis involved; for example, activation of the kyotorphin-Met-enkephalinpathway leads to antinociception, but activation of the NO-cGMPpathway results in hyperalgesia. Moreover, Xu and Tseng (1993)proposed that different descending nociceptive pathways couldbe involved in the supraspinal nociceptive transmission. Theyfound that the i.c.v. morphine-induced antinociception was enhancedby i.t. L-NAME, whereas the i.c.v. $beta$ -endorphin-induced antinociceptionwas potentiated by L-arginine, the latter effect being attenuatedby i.c.v. L-NAME. For that reason, those authors proposed thatstimulation of opioid receptors by $beta$ -endorphin applied supraspinallyinduced release of Met-enkephalin and subsequent stimulation ofdelta opioid receptors in the spinal cord. However, stimulationof mu opioid receptors by morphine given supraspinally activatedthe spinopetal serotonergic and noradrenergic systems and subsequentlystimulated alpha₂-adrenoreceptors and 5-HT receptors in the spinalcord (Xu and Tseng, 1993). Eventually, yet another factor to consideris, that NO may exist in a reduced or an oxidized form, eitherof which may produce distinct pharmacological effects (Lei etal., 1992; Lipton et al., 1996).

A pronociceptive action of NO in the spinal cord was also observed after prolonged noxious stimulation. Our study has shownthat L-NAME administered i.t. attenuates the formalin-inducednociception in the rat. This observation is in agreement withother behavioral and electrophysiological data. It was previouslyreported that L-NAME injected i.t. reduced the responses of dorsalhorn neurons to locally injected formalin in both the first andsecond phases of the formalin test (Haley et al., 1992), and attenuatedthe formalin-induced behavior in the second phase (Malmberg andYaksh, 1993). Additionally, inhibition of the formalin-inducedpaw licking following i.c.v., i.p. or oral administration of L-NAMEto mice, mainly in the second phase (Moore et al., 1991), as wellas inhibition of the second peak of firing of dorsal horn neuronsafter i.v. injection of L-NAME to the rat (Haley et al., 1992)were observed. An antinociceptive action in the second phase ofthe formalin test was also reported for 7-NI administered i.p.to mice (Moore et al., 1993). The above results indicate preferentialinhibition of the second peak of the formalin-induced nociceptionafter the blockade of NO synthase. This effect corresponds toaction of the NMDA receptor antagonists which are effective ininhibiting the repetitive C-fiber stimulation (wind-up), whichis related to the second phase of the formalin test (Wheeler-Acetoet al., 1990; Chapman et al., 1994). A biochemical study revealedthat peripheral formalin injection resulted in a significant increasein the spinal levels of glutamate and aspartate during the firstphase only, and produced significant enhancement of the releaseof citrulline, during both the first and second phases (Malmbergand Yaksh, 1995). Thus, one can expect that stimulation of NMDAreceptors during the first phase of the formalin test leads toan increased level of NO in both phases, while blockade of NMDAreceptors and/or inhibition of NO synthase resulted in antinociceptionprincipally in the second phase.

Intrathecal injection of specific opioid receptor agonists significantly diminishes both phases of the formalin test. Theantinociceptive action of the moderately acting doses of opioidreceptor agonists is potentiated by L-NAME (i.t.) in the secondphase of the formalin test, this effect depends on the dose usedof the opioid receptor agonist. Our study corroborates other behavioraland electrophysiological data that showed that both i.t. (Chapmanand Dickenson, 1992) and i.c.v. (Calcagnetti et al., 1988) administrationof opioid receptor agonists produced analgesia in the formalintest and, that i.t. opioids inhibited the formalin-induced activityof dorsal horn neurons (Dickenson and Sullivan, 1987). In agreementwith other findings (Chapman and Dickenson, 1992; Chapman et al.,1994), our study shows that opioids (especially DAMGO and DPDPE)are more effective in inhibiting the formalin-induced nociceptionin the first phase than in the second one. This is due to thefact that i.t. opioids effectively inhibit the C-fiber-evokedinput responses of dorsal horn neurons, which contribute to thefirst phase of the formalin test (Chapman et al., 1994). In contrast,the enhanced C-fiber-evoked responses of dorsal horn neurons contributeto the second phase of the formalin test that is mediated by NMDAreceptors, and is less sensitive to i.t. opioids (Wheeler-Acetoet al., 1990; Chapman et al., 1994). Moreover, we observed thati.t. injected L-NAME potentiated the opioid-mediated antinociceptionmainly in the second, but not the first phase (except DPDPE) ofthe formalin response, which may be due to a higher efficacy ofL-NAME to inhibit the formalin-induced nociception in the secondphase of that test (as described above).

Our results suggest involvement of NO in the antinociception mediated by different types of opioid receptors in the rat spinalcord. We found that inhibition of NO synthase in the spinal cordstrongly potentiatiated the mu and delta receptor-mediated antinociception.We also observed potentiantion of the kappa mediated antinociception;however, that effect was weaker compared to the mu and delta mediatedantinociception and occurred only in the PP test and at the lasttwo time points of the formalin test. It is suggested that whenthe intensity of heat (but not pressure) stimulus is increasedthe antinociceptive efficacy of kappa agonists is diminished (Millanet al., 1989; Millan, 1990). It seems unlikely that this effectsignificantly contributes to the lack of potentiation of the U50,488Hactivity by L-NAME, because in the TF test the heat stimulus wasadjusted to the moderate/low intensity (basal latencies approx.6 sec). Moreover, relative weakness of the spinal action of kappaagonists as compared to their systemic activity in the rat wasobserved (Millan et al., 1989). This discrepancy can be explainedby the finding that injury of the spinal cord due to the cannulationmay rise the level of dynorphin in the dorsal horn (Przew $l$ ockiet al., 1988; Millan et al., 1989) which may underline a cross-toleranceto exogenous kappa agonists and their apparently lower efficacy(Millan, 1990).

Many of the commonly used NO synthase inhibitors are nonselective, and they act on neuronal as well as endothelial NO synthase.The blockade of endothelial NO synthase by L-NAME results in vasoconstrictionand a subsequent increase in blood pressure (Moore et al., 1993;Semos and Headley, 1994). However, it seems unlikely that thecardiovascular effects of NO synthase inhibitors contribute significantlyto potentiation of the opioid-mediated antinociception in thespinal cord, observed in our study. It was found that L-NAME injectedboth i.t. and i.c.v. in doses comparable (and even much higher)to those used in the present study did not significantly affectthe basal blood pressure of rats and mice (Moore et al., 1991;Haley et al., 1992). L-NAME was reported to influence also theresting cerebral blood flow, but this effect was observed afterrelatively high doses of L-NAME injected i.v. (Yang, 1996). Itwas also found that L-NAME may act as a competitive muscarinicreceptor antagonist (Buxton et al., 1993). However, the endogenousspinal cholinergic system appears to be antinociceptive (Yakshet al., 1985; Iwamoto and Marion, 1993, 1994), so if this werethe predominant effect of L-NAME, it would be expected to be pro-rather than antinociceptive. Moreover, an antimuscarinic activityof L-NAME was found in guinea pig brain (Buxton et al., 1993)but it did not exhibit any affinity for muscarinic receptors inthe rat spinal cord (Buccafusco et al., 1995). Additionally, 7-NI,the most selective inhibitor of neuronal NO synthase that neitherincreases the mean arterial blood pressure in rodents and cats(when injected i.p. or even i.v. at high doses which exceed antinociceptiveones) (Bland-Ward and Moore, 1995), nor exhibts affinity for muscarinicreceptors, also potentiated the morphine-induced antinociceptionin our studies.

The exact mechanism by which inhibition of NO synthase enhances the opioid-mediated antinociception has not been clarifiedas yet. The most important aspects of the opioid-mediated antinociceptionin the spinal cord are presynaptic reduction of transmitter releasefrom C-fibers, and an increase in the membrane K⁺conductance or a decrease in the Ca⁺⁺conductance (Satoh and Kuraishi, 1991; North, 1991; Kangrga andRandic, 1991). NO is produced by NO synthase which is activatedby the Ca⁺⁺influx, mainly after NMDA receptor activation (Garthwaite, 1991).In the light of the above data it may be expected that opioidsare able to prevent activation of NMDA receptors and the subsequentNO synthesis by reducing the presynaptic release of glutamate.The latter assumption is supported by the findings that morphineproduces suppression of the formalin-evoked release of citrullinefrom the rat spinal cord (Malmberg and Yaksh, 1995). Furthermore,opioids are able to prevent the release of Ca⁺⁺from intracellular stores (mediated by inositol trisphosphate)by reducing the SP release (Collin et al., 1992). Alternatively,it is also possible that potentiation of the opioid antinociceptionby NO synthase inhibition may result from a reduced activity ofintracellular signaling in both the cGMP and cAMP pathways. Further,the inhibition of NO synthase may diminish the NMDA receptor-mediatedsynaptic efficacy after the nociceptive input and, in consequence,profoundly enhance the opioid antinociception. A direct interactionbetween NO and opioid receptors may also contribute to the observedeffect. It has been recently reported, that the NO-donor SIN-1may down-regulate the alpha subunit of Gs protein in C6 gliomacells, by increasing ADP ribosylation (Young et al., 1997). Asimilar interaction between NO and other G proteins coupled tothe opioid receptors, e.g., Gi or Go, may also take place. Itcannot be excluded, either, that the NO synthase inhibitor influencesthe metabolism of opioids or their clearance from intrathecalspace. Prolongation of the antinociceptive effect of DPDPE andU50,488H by L-NAME seems to be in line with the above suggestion.In conclusion, our study has demonstrated that inhibition of NOsynthase potentiates the mu, delta and to a lesser extent, kappareceptor-mediated spinal antinociception in both acute and prolongedpain.

	Footnotes

Accepted for publication April 25, 1997.

Received for publication January 27, 1997.

¹ This work supported by a grant for statutory activity obtained from the Committee for Scientific Research (KBN, Warsaw).

Send reprint requests to: Dr. Barbara Przew $l$ ocka, Department of Molecular Neuropharmacology, Institute of Pharmacology, Polish Academy of Sciences, Cracow, Poland.

	Abbreviations

cGMP, cyclic guanosine monophosphate; DAMGO, [D-Ala²,N-Me-Phe⁴,Gly-ol⁵]enkephalin; DPDPE, [D-Pen^2,5]enkephalin; EAA, excitatory amino acid; i.c.v., intracerebroventricular; i.pl., intraplantar; i.t., intrathecal; L-NAME, N-^G-nitro-L-arginine methyl ester; 7-NI, 7-nitroindazole; NO, nitric oxide; PP, paw pressure; TF, tail-flick; U50, 488H, 3,4-dichloro-N-methyl-N-[2-(1-pyrrolidinyl)cyclohexyl]-benzenacetamide.

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				X. Chen and J. D. Levine NOS Inhibitor Antagonism of PGE2-Induced Mechanical Sensitization of Cutaneous C-Fiber Nociceptors in the Rat J Neurophysiol, March 1, 1999; 81(3): 963 - 966. [Abstract] [Full Text] [PDF]

Inhibition of Nitric Oxide Synthase Enhances Antinociception Mediated by Mu, Delta and Kappa Opioid Receptors in Acute and Prolonged Pain in the Rat Spinal Cord1

Inhibition of Nitric Oxide Synthase Enhances Antinociception Mediated by Mu, Delta and Kappa Opioid Receptors in Acute and Prolonged Pain in the Rat Spinal Cord¹