The Nitric Oxide/Cyclic GMP System at the Supraspinal Site Is Involved in the Development of Acute Morphine Antinociceptive Tolerance,

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via Google Scholar

Google Scholar

	Articles by Xu, J. Y.
	Articles by Bidlack, J. M.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Xu, J. Y.
	Articles by Bidlack, J. M.

Vol. 284, Issue 1, 196-201, 1998

The Nitric Oxide/Cyclic GMP System at the Supraspinal Site Is Involved in the Development of Acute Morphine Antinociceptive Tolerance¹^,²

Jimmy Y. Xu, Kevin P. Hill and Jean M. Bidlack

Department of Pharmacology and Physiology, The University of Rochester, School of Medicine and Dentistry, Rochester, New York

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

The role of the supraspinal nitric oxide (NO)/cyclic GMP system in the development of acute morphine antinociceptive tolerancewas investigated by use of the mouse 55°C warm-water tail-flicktest. A single intracerebroventricular (i.c.v.) pretreatment ofmice with morphine (3 nmol, 140 min before testing) produced anacute antinociceptive tolerance to subsequent i.c.v. doses ofmorphine, as demonstrated by a 120-fold rightward shift of themorphine dose-response curve. When co-administered with morphine(140 min before testing), the NO synthase inhibitors: N-nitro-L-argininemethyl ester (L-NAME), 3-bromo-7-nitroindazole, 7-nitroindazoleand N^G-monomethyl-L-arginine, attenuated the development of morphinetolerance. All four NO synthase inhibitors completely blockedthe rightward shift of the morphine dose-response curve causedby i.c.v. morphine pretreatment (3 nmol, 140 min before testing).This effect was partially antagonized by L-arginine, but not D-arginine,in a dose-dependent manner. Also, D-NAME did not block the developmentof tolerance. Like the NO synthase inhibitors, LY-83,583, a guanylylcyclase inhibitor, blocked the development of tolerance, whichsuggests that NO acting through the cyclic GMP pathway is involvedin the development of acute antinociceptive tolerance. The effectsof increased NO production on acute morphine antinociceptive tolerancewere also studied. When co-administered with morphine (140 minbefore testing), neither L-arginine (100 nmol) nor the NO donors,sodium nitroprusside (5 nmol) and isosorbide dinitrate (10 nmol),had any effect on the magnitude of morphine antinociceptive tolerance.These results suggest that NO, acting through the cyclic GMP pathway,mediates the development of acute antinociceptive tolerance, butthat NO production does not alter the magnitude of antinociceptivetolerance.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

NO has been implicated as a biological messenger molecule in the central nervous system (Moncada et al., 1989; Garthwaite,1991; Bredt and Snyder, 1992). NO is derived from one of two equivalentguanidino nitrogens of the amino acid L-arginine by the enzymeNOS, yielding NO and L-citrulline, as a coproduct. NOS is amongthe largest and most complicated of enzymes, and as many as eightisoforms of NOS have been identified from neurons, macrophagesand endothelial cells (Nathan and Xie, 1994; Murad, 1994). Theseisoforms have been classified as either constitutive or inducible.The neuronal NOS is constitutive and calmodulin-dependent (Bredtand Snyder, 1992). Activation of NOS and release of NO stimulatesthe soluble form of guanylyl cyclase, which results in an increasein cyclic GMP levels within the target cells (Deguchi, 1977; Bredtand Snyder, 1992).

The phenomenon of opioid tolerance and dependence has been investigated for many years, but its mechanism is still not completelyunderstood. This phenomenon involves changes of a variety of nonopioidsystems, such as adrenergic and cholinergic neurotransmission(Satoh et al., 1976; Schulz and Herz, 1977; Llorens et al., 1978;Hamburg and Tallman, 1981), in addition to the changes in opioidsystems, such as the changes in affinity and number of opioidreceptors (Puttfarcken et al., 1988), and desensitization of opioid-mediatedinhibition of adenylyl cyclase activity (Sharma et al., 1975).The NMDA receptor has been implicated in the development of opioid-inducedtolerance and dependence because several NMDA antagonists, suchas MK-801, inhibited morphine tolerance and dependence (Trujilloand Akil, 1991; Marek et al., 1991; Tiseo and Inturrisi, 1993).NO produced by the constitutive neuronal NOS has been linked tothe NMDA complex. The activation of NMDA receptors has enhancedthe entry of extracellular Ca⁺⁺, thus stimulating enzymatic production of NO, which in turn increasesthe formation of cyclic GMP by activating guanylyl cyclase (Deguchi,1977; Bredt and Snyder, 1992). Therefore, the NO/cyclic GMP systemhas been postulated to be involved in the development of morphinetolerance and dependence. Indeed, NOS inhibitors, such as L-NAMEand L-NOARG, prevented morphine tolerance and dependence afterchronic morphine administration in rodents (Adams et al., 1993;Kolesnikov et al., 1992; Kimes et al., 1993; Cappenkijk et al.,1993). Systemic administration of L-NAME and L-NOARG have beenreported to attenuate the development of tolerance to the systemicmorphine administration (Elliott et al., 1994; Kolesnikov et al.,1992; 1993; Majeed et al., 1994). Other studies suggest that L-NAMEhas little effect on morphine tolerance and withdrawal at thespinal site (Dunbar and Yaksh, 1996). Therefore, we speculatedthat the NO/cyclic GMP system at supraspinal site might play animportant role in morphine tolerance. In most studies reportedso far, tolerance was induced by chronic and systemic administrationof morphine. However, acute morphine antinociceptive tolerancehas been observed after a single i.c.v. injection of morphine(Jiang et al., 1995). An advantage of studying acute antinociceptivetolerance, induced by a single i.c.v. injection of morphine, isthat the subsequent morphine dose-response line is shifted bymore than 30-fold, after a single pretreatment of mice with 3nmol morphine, at 120 min before the second injection of morphine(Jiang et al., 1995). The study reported here focused on the roleof supraspinal NO/cyclic GMP system in the development of acutemorphine antinociceptive tolerance. The results demonstrate thatinhibition of NO production and inhibition of guanylyl cyclaseactivity blocked the development of acute morphine antinociceptivetolerance.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Animals. Male, ICR mice (25-30 g, Harlan Sprague Dawley, Inc., Indianapolis, IN) were used for all experiments. Mice were kept in groupsof nine in a temperature-controlled room with a 12-hr light-darkcycle (lights on 7:00 A.M. to 7:00 P.M.). Food and water wereavailable ad libitum until the time of the experiment.

Injection techniques. Intracerebroventricular injections were made directly into the lateral ventricle according to the modified method of Haleyand McCormick (1957). The mouse was lightly anesthetized withether, an incision was made in the scalp and the injection wasmade 2 mm lateral and 2 mm caudal to bregma at a depth of 3 mmwith a 10-µl Hamilton microliter syringe. The volume of all i.c.v.injections was 5 µl.

Tail-flick assay. The thermal nociceptive stimulus was 55°C water with the latency to tail flick or withdrawal taken as the endpoint (Vaughtand Takemori, 1979). After determining control latencies, themice received graded i.c.v. doses of opioid agonists or antagonistsat various times. Morphine was given as a single i.c.v. injectionwith testing taking place 20 min after the injection, at whichtime the maximal response had been established in the preliminarystudy. A cut-off time of 15 sec was used; if the mouse failedto display a tail flick, the tail was removed from the water andthat animal was assigned a maximal antinociceptive score of 100%.Mice, showing no response within 5 sec in the initial controltest, were eliminated from the experiment. Antinociception ateach time point was calculated according to the following formula:% antinociception = 100 × (test latency $-$ control latency)/(15 $-$ control latency).

All NOS inhibitors, NO donors and guanylyl cyclase inhibitors were given by i.c.v. injection in a volume of 5 µl, except wherenoted. L-NAME was used at doses ranging from 0.1 to 10 nmol; previously,this dose range was shown to inhibit NO production (Salter etal., 1995

). L-NMMA, 7-nitroindazole and 3-bromo-7-nitroindazolewere administered by i.c.v. injection at a dose of 100 nmol. Thisdose of the NOS inhibitors has been an effective dose in blockingNO production (Salter et al., 1996

). The NO donors, SNP, L-arginineand ISDN, were administered by i.c.v injection at doses of 5 nmol,100 nmol and 10 nmol, respectively, doses that have been shownto be effective in generating NO (Gonzalez et al., 1996

). Methyleneblue and LY-83,583, guanylyl cyclase inhibitors, were administeredat a dose of 10 nmol. This dose of methylene blue and LY-83,583has been shown to inhibit guanylyl cyclase activity (Melis andArgiolas, 1995

Chemicals. Morphine sulfate was purchased from Mallinckrodt Chemical Company (St. Louis, MO). L-NAME, D-NAME, L-arginine, D-arginine,methylene blue, SNP and ISDN were purchased from Sigma ChemicalCompany (St. Louis, MO). LY-83,583, 3-bromo-7-nitroindazole, 7-nitroindazoleand L-NMMA were purchased from Alexis Corp. (San Diego, CA). DAMGOwas purchased from Bachem, Inc. (Torrance, CA). All compoundswere dissolved in distilled water just before use.

Statistics. All dose-response lines were analyzed by regression methods as described by Tallarida and Murray (1986). Regression lines,D₅₀ (dose producing 50% analgesia) values were determined witheach individual data point with use of the computer program byTallarida and Murray (1986). Statistical significance was determinedby analysis of variance, followed by Neuman-Keul's test for multiplegroup comparison. All data points shown are the mean of 8 to 12mice and error bars represent the S.E.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

The effect of NOS inhibitors on the development of acute morphine antinociceptive tolerance. When mice were given a single i.c.v. injection of 3 nmol morphine, a dose that produced 70 ± 10% antinociception, acute antinociceptivetolerance was produced and was measured as a 120-fold rightwardshift in the morphine dose-response curve at 140 min after theinitial morphine injection (fig. 1). Studies were directed atdetermining whether NO was involved in the development of acutemorphine antinociceptive tolerance. When co-injected with theinitial 3 nmol morphine, L-NAME, at a dose of 10 nmol, completelyblocked the development of acute antinociceptive tolerance (fig.1). L-Arginine, the endogenous substrate for NOS, partially inhibitedthe blockade of tolerance caused by L-NAME, which suggests thatL-NAME was producing its effect by acting as a NOS inhibitor (fig.1). Table 1 summarizes the D₅₀ values obtained for morphine-inducedantinociception in the absence and presence of pretreatment withmorphine and in the presence of NOS inhibitors. The suppressionof acute antinociceptive tolerance by L-NAME was concentration(fig. 2A) and time (fig. 2B) dependent. L-NAME reached its peakeffect when co-administered along with the 3-nmol morphine pretreatment,then its effect subsided gradually with time when it was administeredbefore the 3-nmol morphine pretreatment, and lasted less than8 hr (fig. 2B). An i.c.v. injection of 10-nmol L-NAME did notproduce any antinociception, and the same dose of L-NAME, whengiven i.c.v. either 140 min before morphine administration, orco-administered with morphine, did not alter antinociception,induced by i.c.v. morphine (data not shown). L-Arginine, in adose-dependent manner, partially blocked effect of L-NAME (fig.3; table 1). However, D-arginine produced no effect, which demonstratesthe stereoselectivity of the L-arginine effect (fig. 3). Similarly,D-NAME, at a dose of 10 nmol, had no effect on the developmentof acute morphine antinociceptive tolerance (fig. 4).

View larger version (25K):
[in this window]
[in a new window]

Fig. 1. Dose-response lines for i.c.v. morphine (20 min before testing) in mice treated either alone or with morphine (3 nmol), morphine(3 nmol) plus L-NAME (10 nmol) or morphine (3 nmol) plus L-NAME(10 nmol) and L-ARG (100 nmol) for 140 min before testing in themouse 55°C warm-water tail-flick assay.

View this table:
[in this window]
[in a new window]

TABLE 1
Effect of inhibition of NO/cyclic GMP by 7-nitroindazole, 3-bromo-7-nitroindazole, L-NMMA, L-NAME, LY-83,583 and methyleneblue on antinociceptive D₅₀ values for i.c.v. morphine in micepretreated with i.c.v. morphine for 140 min before testing
Pretreatment consisted of administering morphine and the compounds to mice by i.c.v. injection at 120 min before the subsequentmorphine injection. Varying doses of morphine were then injectedi.c.v. and tail-flick response was measured 20 min thereafter,as described under "Materials and Methods." The morphine controlconsisted of varying doses of morphine administered 20 min beforetesting.

View larger version (23K):
[in this window]
[in a new window]

Fig. 2. Dose (A) and time (B) response of the effect of L-NAME on antinociception induced by i.c.v. morphine (10 nmol, 20 min beforetesting) in mice pretreated with a single i.c.v. pretreatmentof morphine (3 nmol, 140 min before testing) in the mouse 55°Cwarm-water tail-flick assay. **P < .01 in comparison with thegroup of mice pretreated with i.c.v. morphine (3 nmol, 140 minbefore testing) only.

View larger version (23K):
[in this window]
[in a new window]

Fig. 3. Effect of L-arginine (L-ARG) and D-arginine (D-ARG) on the inhibition of morphine antinociceptive tolerance by L-NAME. Micewere pretreated with either morphine (3 nmol, 140 min before testing)alone, or morphine (3 nmol, 140 min before testing) and L-NAME(10 nmol, 140 min before testing) or morphine (1 nmol, 140 minbefore testing) and varying doses of L-ARG and D-ARG. A secondi.c.v. injection of morphine (10 nmol) was given 20 min beforetesting in the mouse 55°C warm-water tail-flick assay. *P < .05,**P < .01 in comparison with the group of mice pretreated withi.c.v. morphine (3 nmol) plus L-NAME (10 nmol) for 140 min beforetesting.

View larger version (20K):
[in this window]
[in a new window]

Fig. 4. Dose-response lines for i.c.v. morphine (20 min before testing) in mice treated alone or pretreated with either i.c.v. morphine(3 nmol) or i.c.v. morphine (3 nmol) and i.c.v. D-NAME (10 nmol)for 140 min before testing in the mouse 55°C warm-water tail-flickassay.

To further demonstrate that L-NAME was producing its effect by acting on NOS, three other NOS inhibitors were tested to determinewhether they blocked the development of acute morphine antinociceptivetolerance. As shown in table 1, the NOS inhibitors, 3-bromo-7-nitroindazole,7-nitroindazole and L-NMMA, in addition to L-NAME, completelyblocked the development of acute tolerance.

Determining whether cyclic GMP was involved in the development of acute morphine antinocieptive tolerance. The target action of NO is to activate soluble guanylyl cyclase and increase the production of cyclic GMP. To determine whetherinhibition of guanylyl cyclase activity would also affect thedevelopment of morphine tolerance, the effects of LY-83,583 andmethylene blue, two guanylyl cyclase inhibitors, were studiedby use of the same protocol. LY-83,583, at a dose of 10 nmol,completely blocked the development of acute morphine antinociceptivetolerance when LY-83,583 was co-administered with the initialinjection of 3 nmol morphine (fig. 5 and table 1). Methyleneblue, at a dose of 10 nmol, when co-administered with the 3-nmolmorphine pretreatment, partially blocked the rightward shift ofthe morphine dose-response line caused by the morphine pretreatment(table 1).

View larger version (20K):
[in this window]
[in a new window]

Fig. 5. Dose-response lines for i.c.v. morphine (20 min before testing) in the absence and presence of i.c.v. morphine (3 nmol) andi.c.v. morphine (3 nmol) plus i.c.v. LY-83,583 (10 nmol) given140 min before testing in the mouse 55°C warm-water tail-flickassay.

Determining whether NO production would enhance the development of acute morphine antinociceptive tolerance. Babey et al. (1994) suggested that L-arginine, a NO precursor, when co-administered chronically with morphine, acceleratesthe development of morphine tolerance Therefore, we were interestedin determining whether L-arginine, or the NO donors, such as SNPand ISDN, which are able to release NO without the presence ofNOS, would affect the acute morphine antinociceptive tolerance.To reveal the possible potentiating effect of these compoundson morphine tolerance, mice were pretreated i.c.v. with a lowerdose of morphine (1 nmol), so that only 6-fold of the rightwardshift of morphine dose-response line was observed, which indicatesa lower magnitude of the morphine tolerance (fig. 6). NeitherL-arginine (100 nmol), SNP (5 nmol) nor ISDN (10 nmol), when co-administeredwith the 1-nmol morphine pretreatment for 140 min, affected themagnitude of the morphine antinociceptive tolerance (fig. 6, table2). The effect of chronic and systemic pretreatment of L-arginineon the morphine tolerance was also investigated. As shown in figure7, L-arginine, when given i.p. 200 mg/kg daily for 3 days, didnot alter the magnitude of the morphine antinociceptive tolerance.These results suggest that increased production of NO did notaffect the magnitude of acute morphine antinociceptive tolerance,but that NO was required for the development of acute antinociceptivetolerance.

View larger version (25K):
[in this window]
[in a new window]

Fig. 6. Dose-response lines for i.c.v. morphine (20 min before testing) in the absence and presence of i.c.v. morphine (1 nmol) andin the presence of i.c.v. morphine (1 nmol) plus L-arginine (L-ARG)(100 nmol) or SNP (5 nmol) or ISDN (10 nmol) given by i.c.v. injection140 min before testing in the mouse 55°C warm-water tail-flickassay.

View this table:
[in this window]
[in a new window]

TABLE 2
Effect of increased production of NO by L-arginine, SNP and ISDN on antinociceptive D₅₀ values for i.c.v. morphine in micepretreated with i.c.v. morphine for 140 min before testing
Pretreatment consisted of administering morphine and the compounds to mice by i.c.v. injection at 120 min before the subsequentmorphine injection. Varying doses of morphine were then injectedi.c.v. and tail-flick response was measured 20 min thereafter,as described under "Materials and Methods." The morphine controlconsisted of varying doses of morphine administered 20 min beforetesting.

View larger version (20K):
[in this window]
[in a new window]

Fig. 7. Dose-response lines for i.c.v. morphine (20 min before testing) in the absence and presence of i.c.v. morphine (1 nmol, 140min before testing) in mice treated with and without i.p. L-arginine(L-ARG) (200 mg/kg daily for 3 days) in the mouse 55°C warm-watertail-flick assay.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

The mechanisms underlying the tolerance to the antinociceptive action of opioids are not clear and need to be further explored.The phenomenon of opioid tolerance and dependence may involvechanges in several opioid and non-opioid systems. Animal studieshave revealed that there are two kinds of opioid tolerance, namelyacute opioid tolerance and chronic opioid tolerance. The characteristicsof acute opioid tolerance may differ from those of chronic opioidtolerance. The present study used an acute morphine antinociceptivetolerance model, which has been well documented in this laboratory(Jiang et al., 1995). Acute antinociceptive tolerance to morphinedevelops within 2 hr after a single i.c.v. injection of morphinein mice.

The magnitude of opioid tolerance appears to be affected by the route of administration. The i.c.v. or i.t. administrationof opioid agonists produces a larger magnitude of tolerance tosubsequent i.c.v. or i.t. administration of the same opioid agonists,respectively, in comparison with the systemic administration ofopioids. For example, with the mu selective peptide DAMGO, Mattiaet al. (1991) reported a 47-fold rightward shift of the i.c.v.DAMGO dose-response curve in mice pretreated with i.c.v. injectionsof the D₉₀ dose of DAMGO twice daily for 3 days. The same protocolwith the delta selective peptide, [D-Ala²]deltorphin II, produced a greater than 37-fold shift in the i.c.v.[D-Ala²]deltorphin II dose-response curve (Mattia et al., 1991). Otherinvestigators demonstrated a robust 117-fold rightward shift inthe i.t. morphine dose-response curve by a chronic i.t. infusionof 20 nmol/hr of morphine into rats for 7 days as measured bythe hot-plate test (Stevens and Yaksh, 1989). On the other hand,a s.c. injection of 100 mg/kg of morphine produced only a 3- to6-fold rightward shift in the s.c. morphine dose-response curvewhen measured by the radiant heat tail-flick test at 3 hr afterthe initial morphine injection (Vaught and Takemori, 1979). Withuse of the acute antinociceptive tolerance model presented hereand used previously (Jiang et al., 1995), we have consistentlyobserved a 30- to 70-fold rightward shift of the i.c.v. morphinedose-response curve in mice pretreated with a single i.c.v. injectionof 3 nmol morphine for 140 min as measured by a 55°C warm-watertail-flick test. The reason why i.c.v. or i.t. administrationof opioid agonists is more effective than the systemic route ofadministration in producing tolerance is not understood. It couldbe the result of the relatively higher potency produced by systemicadministration of opioid agonists, because both supraspinal andspinal opioid receptors are activated and a multiplicative interactionbetween the two sites may occur (Roerig and Fujimoto, 1989). Thisphenomenon fits the concept proposed by Stevens and Yaksh (1989)that the potency of antinociceptive agents is inversely relatedto magnitude of tolerance after continuous infusion.

The present study demonstrated that supraspinal administration of four different NOS inhibitors attenuated the developmentof acute morphine antinociceptive tolerance in a dose- and time-dependentmanner. A dose of 10 nmol L-NAME completely blocked the acutemorphine antinociceptive tolerance induced by a pretreatment ofmice with 3 nmol morphine for 140 min. This action of L-NAME waspartially antagonized by L-arginine but not D-arginine, whichindicates the stereoselectivity of the L-arginine effect. Thisstereoselectivity of L-NAME effect was further supported by theineffectiveness of the D-NAME in attenuating morphine tolerance.These results strongly suggest that inhibition of supraspinalNO production resulted in an inhibition of acute morphine antinociceptivetolerance. This finding is in line with studies reported by othersthat systemic administration of NOS inhibitors attenuates thedevelopment of tolerance to systemic morphine administration (Kolesnikovet al., 1992, 1993; Babey et al., 1994; Majeed et al., 1994).Recently, i.t. administration of L-NAME has also been reportedto have little effect in attenuating tolerance to i.t. morphine(Dunbar and Yaksh, 1996). Taken together, these studies suggestthat NO at supraspinal but not the spinal site may play an importantrole in the mediation of morphine antinociceptive tolerance.

Studies by others suggest that L-NAME exhibits antinociceptive activity in the mouse (Moore et al., 1991; Malmberg and Yaksh,1993). In those studies, the antinociceptive activity of L-NAMEwas demonstrated in the formalin-induced paw licking test, aswell as the acetic acid-induced writhing test and hot-plate testafter L-NAME was administered by i.p. injection. Also, L-NAMEproduced antinociception in the formalin-induced paw licking testafter i.c.v. or oral administration (Moore et al., 1991). Przewlockiet al. (1993) reported that i.t. L-NAME potentiated i.t. morphine-inducedantinociception. Based on these findings, it is logical to suspectthat the reversal effect of L-NAME on morphine-induced antinociceptionafter the development of tolerance might be caused by the additiveor synergistic actions between the possible L-NAME-induced antinociceptiveeffect and morphine-induced antinociceptive effect. However, wewere able to exclude this possibility for the following reasons.First, in the mouse 55°C warm-water tail-flick test, L-NAME atdoses up to 10 nmol, when given i.c.v., did not produce a significantantinociceptive effect. Second, L-NAME at 10 nmol, when givenalong with, or 140 min before i.c.v. morphine injection, did notaffect morphine-induced antinociception (data not shown). Theseresults are consistent with the study reported by Xu and Tseng(1995), which demonstrated that L-NAME is not effective in modulatingmorphine-induced antinociception in the tail-flick test at thesupraspinal site.

One of the actions of NO is to activate soluble guanylyl cyclase, thus increasing the level of cyclic GMP (Deguchi, 1977;Bredt and Snyder, 1992). This action of NO can be inhibited byLY-83,583 and methylene blue, which are inhibitors of guanylylcyclase. In the present study, we found that LY-83,583, when givenalong with the i.c.v. morphine pretreatment, completely attenuatedthe development of morphine antinociceptive tolerance. Methyleneblue, which is not as selective for guanylyl cyclase as LY-83,583,partially blocked the development of tolerance. These resultssuggest that the cyclic GMP system may also participate in themediation of the morphine tolerance. There may be both cyclicGMP-dependent and -independent mechanisms involved in the effectof NO on the development of tolerance. Indeed, NO has been demonstratedto modulate certain neuronal proteins through a cyclic GMP-independentprocess. For example, Hess et al. (1994) reported that exogenousand endogenously generated NO resulted in the modification ofcysteine residues on neuronal proteins. In particular, exposureof synaptosomes to NO inhibited subsequent thiol-linked ADP-ribosylationof the heterotrimeric G-protein by pertussis toxin.

Other studies with L-arginine further support the involvement of NO in morphine tolerance. L-Arginine, but not D-arginine,when given with morphine, appears to accelerate tolerance to systemicmorphine (Babey et al., 1994). L-Arginine is the natural substratefor NOS. Administration of L-arginine may increase the formationof NO and, thereby, possibly enhance the rate of development ofmorphine antinociceptive tolerance. In the present study, we focusedon the effect of L-arginine on the magnitude of morphine tolerance.We clearly demonstrated that neither L-arginine, nor NO donorssuch as SNP and ISDN, which do not require NOS to produce NO,altered the magnitude of the acute morphine antinociceptive tolerance.

In summary, we found that inhibition of supraspinal NO/cyclic GMP system prevented the development of acute morphine antinociceptivetolerance. However, increased production of NO did not affectthe magnitude of the morphine tolerance.

	Footnotes

Accepted for publication September 8, 1997.

Received for publication January 21, 1997.

¹ This work was supported by U.S. Public Health Service grants DA03742 and DA07232 from the National Institute on Drug Abuse.

² Animals used in these studies were maintained in accordance with the University Committee on Animal Resources, Universityof Rochester, and guidelines of the Committee on the Care andUse of Laboratory Animals of the Institute of Laboratory AnimalResources, National Research Council (Department of Health, Educationand Welfare, Publication No. (NIH)-23, revised 1983).

Send reprint requests to: Dr. Jean M. Bidlack, Department of Pharmacology and Physiology, P.O. Box 711, University of Rochester Medical Center, 601 Elmwood Ave., Rochester, NY 14642-8711.

	Abbreviations

NO, nitric oxide; NOS, nitric oxide synthase; L-NAME, N-nitro-L-arginine methyl ester; L-NOARG, N-nitro-L-arginine; D-NAME, N-nitro-D-arginine methyl ester; L-NMMA, N^G-monomethyl-L-arginine; LY-83, 583, 6-(phenylamine)-5,6-quinolinedione, 6-anillno-5,8-quinolinedione; NMDA, N-methyl-D-aspartate; SNP, sodium nitroprusside; ISDN, isosorbide dinitrate; DAMGO, [D-Ala²,(Me)Phe⁴,Gly(ol)⁵]enkephalin; i.c.v., intracerebroventricular(ly); i.t., intrathecal(ly); i.p., intraperitoneal(ly); s.c., subcutaneous.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

Adams ML, Kalicki JM, Meyer ER and Cicero TJ (1993) Inhibitionof the morphine withdrawal syndrome by a nitric oxide synthaseinhibitor, N^G-nitro-L-arginine methyl ester. LifeSci 52: 245-249.
Babey AM, Kolesnikov Y, Cheng J, Inturrisi CE, Trifilletti RR and Pasternak GW (1994) Nitricoxide and opioid tolerance. Neuropharmacology 33: 1463-1470[Medline].
Bredt DS and Snyder SH (1992) Nitricoxide, a novel neuronal messenger. Neuron 8: 3-11[Medline].
Cappenkijk SL, de Vries R and Dzoljic MR (1993) Inhibitoryeffect of nitric oxide (NO) synthase inhibitors on naloxone-precipitatedwithdrawal syndrome in morphine-dependent mice. NeurosciLett 162: 97-100[Medline].
Deguchi T (1977) Endogenous activity factor for guanylylcyclase in synaptosomal soluble fraction of the rat brain. JBiochem 252: 7617-7619.
Dunbar S and Yaksh TL (1996) Effectof spinal infusion of L-NAME, a nitric oxide synthase inhibitor,on spinal tolerance and dependence induced by chronic intrathecalmorphine in the rat. NeurosciLett 207: 33-36[Medline].
Elliott K, Minammi N, Kolesnikov Y, Pasternak GW and Inturrisi CEI (1994) TheNMDA receptor antagonists, LY2764614 and MK-801, and the nitricoxide synthase inhibitor, N^G-nitro-L-arginine, attenuate analgesic tolerance to the mu-opioidmorphine but not to kappa opioids. Pain 56: 69-75[Medline].
Garthwaite J (1991) Glutamate, nitric oxide and cell-cellsignaling in the nervous system. TrendsNeurosci 14: 60-67[Medline].
Gonzalez MC, Linares JD, Santos M and Llorente E (1996) Effectsof nitric oxide donors sodium nitroprusside and 3-morpholino-sydnonimineon prolactin secretion in conscious rats. NeurosciLett 203: 167-170[Medline].
Haley TJ and McCormick WG (1957) Pharmacologicaleffects produced by intracerebral injections of drugs in the consciousmouse. Br J Pharmacol Chemother 12: 12-15.[Medline]
Hamburg M and Tallman JF (1981) Chronicmorphine administration increases the apparent number of alpha₂-adrenergicreceptors in rat brain. Nature 291: 493-495[Medline].
Hess DT, Lin L-H, Freeman JA and Norden JJ (1994) Modificationof cysteine residues with G_o and other neuronal proteins by exposureto nitric oxide. Neuropharmacology 33: 1283-1292[Medline].
Jiang Q, Seyed-Mozaffari A, Sebastian A, Archer S and Bidlack JM (1995) Preventingmorphine antinociception tolerance by irreversible mu opioid antagonistsbefore the onset of the their antagonism. JPharmacol Exp Ther 273: 680-688[Abstract/Free Full Text].
Kimes AS, Vaupel DB and London ED (1993) Attenuationof some signs of opioid withdrawal by inhibitors of nitric oxidesynthase. Psychopharmacology 112: 521-524[Medline].
Kolesnikov YA, Pick CG and Pasternak GW (1992) N^G-Nitro-L-arginine prevents morphine tolerance. EurJ Pharmacol 221: 399-400[Medline].
Kolesnikov YA, Pick CG, Ciszewska G and Pasternak GW (1993) Blockadeof tolerance to morphine but not to $kappa$ opioids by a nitric oxidesynthase inhibitor. Proc NatlAcad Sci USA 90: 5162-5166[Abstract/Free Full Text].
Llorens C, Martres MP, Baudry M and Schwarz JC (1978) Hypersensitivityto noradrenaline in cortex after chronic morphine: Relevance totolerance and dependence. Nature 274: 603-605[Medline].
Majeed NH, Przewlocki B, Machelska H and Przewlocki R (1994) Inhibitionof nitric oxide synthase attenuates the development of morphinetolerance and dependence in mice. Neuropharmacology 33: 189-192[Medline].
Malmberg AB and Yaksh TL (1993) Spinalnitric oxide synthesis inhibition blocks NMDA- induced thermalhyperalgesia and produces antinociception in the formalin testin rat. Pain 54: 291-300[Medline].
Marek P, Ben-Eliyahu S, Vaccarino AL and Liebeskind JC (1991) Delayedapplication of MK-801 attenuates development of morphine tolerancein rats. Brain Res 558: 163-165[Medline].
Mattia A, Vanderah T, Mosberg HI and Porreca F (1991) Lackof antinociceptive cross-tolerance between [D-Pen², D-Pen⁵]enkephalin and [D-Ala²]deltorphin II in mice: Evidence for delta receptor subtypes. JPharmacol. Exp Ther 258: 583-587[Abstract/Free Full Text].
Melis MR and Argiolas A (1995) Nitricoxide donors induce penile erection and yawning when injectedin the central nervous system of male rats. EurJ Pharmacol 294: 1-9[Medline].
Moncada S, Palmer RMJ and Higs EA (1989) Biosynthesisof nitric oxide from L- arginine. A pathway for the regulationof cell function and communication. BiochemPharmacol 38: 1709-1715[Medline].
Moore PK, Oluyomi AO, Babbedge RC, Wallace P and Hart SL (1991) N^G-Nitro- L-arginine methyl ester exhibits antinociceptive activityin the mouse. Br J Pharmacol 102: 198-202[Medline].
Murad F (1994) The role of nitric oxide in modulatingguanylyl cyclase. Neurotransmissions 2: 1-4.
Nathan C and Xie Q,-W (1994) Nitricoxide synthase: Roles, tolls and controls. Cell 78: 915-918[Medline].
Przewlocki R, Machelska H and Przewlocki B (1993) Inhibitionof nitric oxide synthase enhances morphine antinociception inthe rat spinal cord. LifeSci 53: PL1-5[Medline].
Puttfarcken PS, Werling LL and Cox BM (1988) Effectsof chronic morphine exposure on opioid inhibition of adenylylcyclase in 7315c cell membranes: A useful model for the studyof tolerance at µ opioid receptors. MolPharmacol 33: 520-527[Abstract].
Roerig SC and Fujimoto JM (1989) Multiplicativeinteraction between intrathecally and intracerebroventricularlyadministered mu opioid agonists but limited interactions betweendelta and kappa agonists for antinociception in mice. JPharmacol Exp Ther 249: 762-768[Abstract/Free Full Text].
Salter M, Duffy C, Garthwaite J and Strijbos PJ (1995) Substantialregional and hemispheric differences in brain nitric oxide synthase(NOS) inhibition following intracerebroventricular administrationof N-nitro-L-arginine (L-NA) and its methyl ester (L-NAME). Neuropharmacology 34: 639-649[Medline].
Salter M, Duffy C, Garthwaite J and Strijbos PJ (1996) Exvivo measurement of brain tissue nitrite and nitrate accuratelyreflects nitric oxide synthase activity in vivo. JNeurochem 66: 1683-1690[Medline].
Satoh M, Zieglgansberger W and Herz A (1976) Supersensitivityof cortical neurons of the rats to acetylcholine and l-glutamatefollowing chronic morphine treatment. Naunyn-Schmiedeberg'sArch Pharmacol 293: 101-103[Medline].
Schulz R and Herz A (1977) Naloxone-precipitatedwithdrawal reveals sensitization to neurotransmitters in morphinetolerant/dependent rats. Naunyn-Schmiedeberg'sArch Pharmacol 299: 95-99[Medline].
Sharma SK, Klee WA and Nirenberg M (1975) Dualregulation of adenylate cyclase accounts for narcotic dependenceand tolerance. Proc Natl AcadSci USA 72: 3092-3096[Abstract/Free Full Text].
Stevens CW and Yaksh TL (1989) Potencyof infused spinal antinociceptive agents is inversely relatedto magnitude of tolerance after continuous infusion. JPharmacol Exp Ther 250: 1-8[Abstract/Free Full Text].
Tallarida RJ and Murray RB (1986) Manualof Pharmacologic Calculations with Computer Programs., 2nded, Springer-Verlag, NewYork.
Tiseo P and Inturrisi CE (1993) Attenuationand reversal of morphine tolerance by the competitive N-methyl-D-aspartatereceptor antagonist, LY274614. JPharmacol Exp Ther 264: 1090-1096[Abstract/Free Full Text].
Trujillo KA and Akil H (1991) Inhibitionof morphine tolerance and dependence by the NMDA receptor antagonistMK-801. Science 251: 85-87[Abstract/Free Full Text].
Vaught JL and Takemori AE (1979) Differentialeffects of leucine and methionine enkephalin on morphine-inducedanalgesia, acute tolerance and dependence. JPharmacol Exp Ther 208: 86-90[Abstract/Free Full Text].
Xu JY and Tseng LF (1995) Nitricoxide/cyclic GMP system in the spinal cord differentially modulatesintracerebroventricularly administered morphine- and $beta$ -endorphin-inducedantinociception in the mouse. JPharmacol Exp Ther 274: 8-16[Abstract/Free Full Text].

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via Google Scholar

Google Scholar

	Articles by Xu, J. Y.
	Articles by Bidlack, J. M.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Xu, J. Y.
	Articles by Bidlack, J. M.

The Nitric Oxide/Cyclic GMP System at the Supraspinal Site Is Involved in the Development of Acute Morphine Antinociceptive Tolerance1,2

The Nitric Oxide/Cyclic GMP System at the Supraspinal Site Is Involved in the Development of Acute Morphine Antinociceptive Tolerance¹^,²