Tonic Descending Facilitation from the Rostral Ventromedial Medulla Mediates Opioid-Induced Abnormal Pain and Antinociceptive Tolerance

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The Journal of Neuroscience, January 1, 2001, 21(1):279-286

Tonic Descending Facilitation from the Rostral Ventromedial Medulla Mediates Opioid-Induced Abnormal Pain and Antinociceptive Tolerance
Todd W. Vanderah, Nova M. H. Suenaga, Michael H. Ossipov, T. Philip Malan Jr, Josephine Lai, and Frank Porreca
Departments of Pharmacology and Anesthesiology, University of Arizona, Tucson, Arizona, 85724

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Many clinical case reports have suggested that sustained opioid exposure can elicit unexpected, paradoxical pain. Here, weexplore the possibility that (1) opioid-induced pain results fromtonic activation of descending pain facilitation arising in therostral ventromedial medulla (RVM) and (2) the presence of suchpain manifests behaviorally as antinociceptive tolerance. Ratsimplanted subcutaneously with pellets or osmotic minipumps deliveringmorphine displayed time-related tactile allodynia and thermalhyperalgesia (i.e., opioid-induced "pain"); placebo pellets orsaline minipumps did not change thresholds. Opioid-induced painwas observed while morphine delivery continued and while the ratswere not in withdrawal. RVM lidocaine, or bilateral lesions ofthe dorsolateral funiculus (DLF), did not change response thresholdsin placebo-pelleted rats but blocked opioid-induced pain. Theintrathecal morphine antinociceptive dose-response curve (DRC)in morphine-pelleted rats was displaced to the right of that inplacebo-pelleted rats, indicating antinociceptive "tolerance."RVM lidocaine or bilateral DLF lesion did not alter the intrathecalmorphine DRC in placebo-pelleted rats but blocked the rightwarddisplacement seen in morphine-pelleted animals. The subcutaneousmorphine antinociceptive DRC in morphine-pelleted rats was displacedto the right of that in placebo-pelleted rats; this right shiftwas blocked by RVM lidocaine. The data show that (1) opioids elicitpain through tonic activation of bulbospinal facilitation fromthe RVM, (2) increased pain decreases spinal opioid antinociceptivepotency, and (3) blockade of pain restores antinociceptive potency,revealing no change in antinociceptive signal transduction. Thesestudies offer a mechanism for paradoxical opioid-induced painand allow the development of approaches by which the loss of analgesicactivity of opioids might beinhibited.

Key words: descending facilitation; opioid-induced pain; opioid tolerance; supraspinal/spinal synergy; lidocaine; tactile allodynia; thermal hyperalgesia

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Opioid analgesics, especially morphine, continue as the primary treatment of moderate to severe pain. Numerous clinical casereports indicate that opioids can paradoxically produce abnormalpain, which includes allodynia (pain elicited by normally innocuousstimuli) and hyperalgesia (enhanced responses to noxious stimulation)(for review, see Arner et al., 1988). Typically, opioid-inducedabnormal pain differs in location and quality from the originalcomplaint (Ali, 1986; Stillman et al., 1987; De Conno et al.,1991; Devulder, 1997). Opioids can also elicit paradoxical, abnormalpain in experimental models after acute (Yaksh and Harty, 1988;Larcher et al., 1998; Celerier et al., 1999, 2000) or sustained(Mao et al., 1995) administration. The mechanisms of such opioid-inducedparadoxical pain are unknown but have been linked in animals tothe NMDA receptor (Mao et al., 1995; Larcher et al., 1998; Celerieret al., 1999, 2000).

In both clinical and experimental settings, sustained opioid analgesia is limited by tolerance. NMDA receptor blockade hasbeen repeatedly demonstrated to block opioid tolerance becauseof either repeated or infused opioid administration (Trujilloand Akil, 1991; Tiseo and Inturrisi, 1993; Mao et al., 1994, 1995,1996; Tiseo et al., 1994; Manning et al., 1996). However, themechanism by which opioid tolerance is altered by NMDA receptorblockade also remainsunclear.

Fields et al. (1983), Fields and Heinricher (1985), Fields et al. (1991), and Morgan and Fields (1994) have characterizeddescending pain modulatory systems arising in the rostral ventromedialmedulla (RVM). In these studies, bulbospinal projections mediatingboth descending pain inhibition and facilitation have been noted(for review, see Fields and Basbaum, 1999). Such descending pathwaysare believed to travel in the dorsolateral funiculus (DLF) tothe spinal dorsal horn (Fields and Basbaum, 1999). Whereas theimportance of descending pain facilitation under physiologicalconditions is unclear, the existence of these projections ledus to hypothesize that possible tonic activation of such systemsunder pathological conditions may provide a mechanism for chronicabnormal pain such as that seen in neuropathic states (Kovelowskiet al., 2000; Ossipov et al., 2000; Sun et al., 2000). The presentstudies have extended this hypothesis to examine whether tonicactivation of descending pain facilitation may also provide amechanism for the abnormal pain seen with sustained opioids. Ourdata suggest that the presence of opioid-induced pain resultingfrom sustained opioid delivery manifests behaviorally as antinociceptivetolerance. Blockade of such pain reveals no loss of opioid signaltransduction. These findings open clinical possibilities by whichopioid analgesia might be maintained in the treatment of chronicpainstates.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Male Sprague Dawley rats (Harlan Sprague Dawley, Indianapolis, IN), 200-300 gm at time of testing, were maintained in a climate-controlledroom on a 12 hr light/dark cycle (lights on at 6:00 A.M.) withfood and water available ad libitum. All testing was performedin accordance with the policies and recommendations of the InternationalAssociation for the Study of Pain and the National Institutesof Health guidelines for the handling and use of laboratory animalsand received approval from the Institutional Animal Care and UseCommittee of the University of Arizona. It should be noted thatterm "pain" used in this report reflects measured changes in sensorythresholds (i.e., enhanced nociceptive responses) in animals.Any relationship to human states of pain are necessarily limited,and no claims are made regarding possible cortical or thalamicprojections. Groups of 5-10 rats were used in allexperiments.

Surgical procedures. While under halothane anesthesia, some groups of rats were implanted with intrathecal catheters (PE-10,7.5 cm) as described previously (Yaksh and Rudy, 1976) for drugadministration at the level of the lumbar spinal cord. Animalswere allowed to recover for 4d.

Rats were prepared for bilateral RVM drug administration by placing anesthetized (ketamine-xylazine; 100 mg/kg, i.p.) animalsin a stereotaxic headholder. For intracranial bilateral drug administrations,the skull was exposed, and two 26 gauge guide cannula separatedby 1.2 mm (Plastics One, Roanoke, VA) were directed toward thelateral portions of the RVM (anteroposterior $-$ 11.0 mm from bregma,lateral ±0.6 mm from midline, dorsoventral $-$ 8.5 mm from the cranium);these coordinates were obtained from the atlas of Paxinos andWatson (1986). The guide cannulas were cemented in place and securedto the skull by small stainless steel machine screws. The animalswere allowed to recover 5 d after surgery before any pharmacologicalmanipulations were made. Drug administrations into the RVM wereperformed by slowly expelling 0.5 µl of drug solution or salinethrough a 33 gauge injection cannula inserted through the guidecannula and protruding an additional 1 mm into fresh brain tissueto prevent backflow of drug into the guide cannula. At the terminationof the experiments, Pontamine blue was injected into the siteof the RVM injections, and catheter placement was verified histologically.Data from animals with incorrectly placed cannulas werediscarded.

Spinal DLF lesions. Spinal lesions at the T₈ level were performed in halothane-anesthetized rats. A laminectomy was made atthe T₈ level to expose the spinal cord. Lesions of the DLF wereperformed by crushing the area with fine forceps. Sham spinalsurgery was performed by exposing the vertebrae and performingthe laminectomy, but without cutting any neuronal tissue. Hemostasiswas confirmed, and the wound over the exposed spinal cord waspacked with Gelfoam and closed. All lesions were verified histologicallyat the termination of the experiment by fixing the spinal sectionsobtained from the lesion site in paraffin. Sections (40-µm-thick)were mounted and stained with Luxor fast blue myelin stain tovisualize intact and disrupted white matter. Behavioral resultsobtained only from animals that had appropriately placed DLF lesionswere included inanalysis.

Drug administration. For sustained administration, two 75 mg morphine pellets or two placebo pellets were implanted subcutaneously.Continuous subcutaneous infusions were also performed with osmoticminipumps (Alza, Mountain View, CA). The osmotic pumps deliveredsaline at 1 µl/hr or morphine at 45 µg · µl¹ · hr¹ for 7 d and were implanted in the subcutaneous space. Test compoundswere injected either through the intrathecal catheter in a volumeof 5 µl followed by a 9 µl saline flush or by a subcutaneous administrationat a volume of 1 ml/kg. The intrathecal administration of morphinewas performed 30 min before tail flick in all studies. Each animalwas used only once to avoid possibility of acute tolerance. Lidocaine(4% w/v) was administered bilaterally (0.5 µl) into the RVM. Inthe tail flick, RVM lidocaine time course studies, lidocaine waseither coadministered with morphine or given 10 or 20 min beforeor 10 or 20 min after morphine administration. Saline was injectedinto the RVM as a control for the lidocaine administration. Subcutaneousmorphine or placebo pellets were implanted 2 d after animals underwenteither sham or DLF lesion as describedabove.

Thermal hyperalgesia. The method of Hargreaves et al. (1988) was used to assess paw-withdrawal latency to a thermal nociceptivestimulus. Rats were allowed to acclimate within a Plexiglas enclosureon a clear glass plate maintained at 30°C. A radiant heat source(i.e., high-intensity projector lamp) was activated with a timerand focused onto the plantar surface of the hindpaw. Paw-withdrawallatency was determined by a motion detector that halted both lampand timer when the paw was withdrawn. The latency to withdrawalof the paw from the radiant heat source was determined both beforeand after drug or vehicle administration. Baseline latencies wereestablished at ~20 sec to allow for detection of possible hyperalgesia.A maximal cutoff of 40 sec was used to prevent tissue damage.Comparisons among group means were determined by Student's t testat a significance level of 0.05.

Tactile allodynia. The paw withdrawal thresholds of the hindpaws of the rats were determined in response to probing with eightcalibrated von Frey filaments (Stoelting, Wood Dale, IL) in logarithmicallyspaced increments ranging from 0.41 to 15 gm (4-150 mN). Eachfilament was applied perpendicularly to the plantar surface ofthe ligated paw of rats kept in suspended wire-mesh cages. Measurementswere taken both before and after administration of drug or vehicle.Withdrawal threshold was determined by sequentially increasingand decreasing the stimulus strength ("up and down" method), analyzedusing a Dixon nonparametric test (Chaplan et al., 1994) and expressedas the mean withdrawal threshold. Comparisons among group meanswere determined by Student's t test at a significance level of0.05.

Tail-flick test. Acute nociception was determined by using the nociceptive hot water (52°C) tail-flick reflex. The tail-flicktest was performed by placing the distal third of the tail ofrats in a heated water bath maintained at 52°C. The latency untiltail withdrawal (rapid flick) from the bath was determined andcompared among the treatments. A 10 sec cutoff was used to avoidtissue damage. Tolerance to the antinociceptive effect of opioidswas indicated by a significant reduction in tail-flick latencyafter challenge with an A₉₀ dose. Data were converted to percentageof antinociception by the following formula: (response latency $-$ baseline latency)/(cutoff $-$ baseline latency) × 100 to generatedose-response curves (Tallarida and Murray, 1987). Regressionanalysis of the dose-response curves was used to detect significantshifts in drug potency (Tallarida and Murray, 1987).

Rotarod test. Rats were tested for their ability to balance on a slow rotating rod (diameter 3.5 cm; rate of rotation 10 rpm).Rats were conditioned before the experiment, and rats (naive ratsremaining on the rotarod for 180 sec) were then injected bilaterally(0.5:l) via the RVM route with either lidocaine (4% w/v) or saline.Rats were tested at 30 min after RVM administration, and the latencyto fall off the rod was recorded. Animals falling of the rod beforecutoff of 180 sec were considered as having motorimpairment.

Compounds. Morphine sulfate was purchased from Sigma (St. Louis, MO). Morphine pellets and placebo pellets were a generousgift from the National Institute on Drug Abuse. Lidocaine (4%w/v in sterile saline) was purchased from Roxane Laboratories(Columbus, OH). All compounds were dissolved in normalsaline.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Sustained administration of morphine by subcutaneous implantation of two 75 mg morphine pellets produced tactile allodyniaand thermal hyperalgesia when measured on day 7 after pellet implantation.Paw withdrawal thresholds to probing with von Frey filaments weresignificantly reduced to 2.9 ± 0.5 gm from a baseline of 15 ±0 gm (Fig. 1). Paw withdrawal latencies from radiant heat weresignificantly (p $<=$ 0.05) reduced to 14.3 ± 0.7 sec from a baselineof 22.2 ± 1.6 sec (Fig. 1). Similar results were achieved withsubcutaneous infusion of morphine through an osmotic pump (45µg · µl¹ · hr¹) for 7 d. Paw withdrawal thresholds were significantly (p $<=$ 0.05)reduced from 15 ± 0 gm to 7.4 ± 1.6 gm 7 d after the start ofmorphine infusion. Similarly, paw withdrawal latencies were significantly(p $<=$ 0.05) reduced from a preinfusion baseline of 22.0 ± 0.6 secto 16.6 ± 0.3 sec. The onset of tactile allodynia and thermalhyperalgesia elicited by subcutaneous morphine pellets were time-relatedand could be detected as early as day 2 (Fig. 2). As expected,antinociception was evident during the first few hours after subcutaneousmorphine pellet implantation and could readily be detected inthe foot-flick assay (Fig. 2). Placebo pellets did not elicitantinociceptive effects, and no changes in response thresholdsto a non-noxious stimulus were observed in placebo-pelleted animals(Fig. 2). Similarly, subcutaneous minipumps delivering salinedid not elicit changes in sensory threshold to either non-noxiousor noxious stimulation.

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Figure 1. Male Sprague Dawley rats were implanted subcutaneously with either two placebo or two morphine (75 mg each) pellets. The 7 d of constant exposure to morphine pellets resulted in tactile allodynia indicated by a significant (*p $<=$ 0.05; Student's t test; n = 10) decrease in paw withdrawal thresholds to probing with von Frey filaments (A). The bilateral microinjection of lidocaine (0.5 µl; 4% w/v) into the RVM on day 7 blocked tactile allodynia when given 30 min before testing in morphine-pelleted rats (n = 10) (A). Rats with placebo pellets demonstrated no significant (p > 0.05) difference in paw withdrawal thresholds to probing with von Frey filaments on day 7. The bilateral microinjection of lidocaine (0.5 µl; 4% w/v) into the RVM on day 7 produced no changes in paw withdrawal thresholds in placebo-pelleted rats (A). The exposure to subcutaneous morphine pellets also resulted in thermal hyperalgesia indicated by a significant (*p $<=$ 0.05; Student's t test; n = 10) decrease in paw withdrawal latencies to radiant heat applied to the plantar aspect of the hindpaw (B). The bilateral microinjection of lidocaine (0.5 µl; 4% w/v) on day 7 blocked thermal hyperalgesia when given 30 min before testing in morphine-pelleted rats (n = 10) (B). Placebo-pelleted animals demonstrated no significant (p > 0.05) difference in paw withdrawal latencies to radiant heat on day 7, nor were there any significant changes after the bilateral RVM administration of lidocaine (0.5 µl; 4% w/v) (B).

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Figure 2. Male Sprague Dawley rats received subcutaneous implantation of placebo or morphine pellets (two 75 mg pellets or 150 mg/animal). Paw withdrawal thresholds to probing with von Frey filaments (A) and paw withdrawal latencies to radiant heat (B) applied to the plantar aspect of the hindpaw were determined 2 and 6 hr after implantation and once daily afterward for 7 d. Morphine pellets initially produced antinociception (at 2 and 6 hr) in the radiant heat paw-flick test (B). Subsequently, tactile allodynia and thermal hyperalgesia, as indicated by a decrease in paw withdrawal thresholds and latencies were observed. Allodynia and hyperalgesia were significant (*p $<=$ 0.05; Student's t test; n = 6) by the second day after morphine pellet implantation.

During measurement periods, both placebo- and morphine-pelleted animals, and animals with osmotic minipumps delivering morphineor saline were carefully monitored for behavioral signs of opioidabstinence using a previously established scoring system. Theseincluded the presence of "wet-dog" shakes, excessive grooming,diarrhea, chromodacryorrhea, and jumping (Wei, 1973). In no caseswere signs of opioid withdrawal observed over the 7 d period whilemorphine was being delivered; the behavioral scores for thesewithdrawal signs were essentially zero and showed no differencesbetween placebo versus morphine-pelleted groups or saline- versusmorphine-infusion groups (data notshown).

The administration of lidocaine (0.5 µl, 4% w/v) into the RVM did not alter response thresholds to von Frey filaments or noxiousthermal stimulation in placebo-pelleted or saline-infused rats.However, RVM lidocaine blocked both tactile allodynia and thermalhyperalgesia seen in morphine-pelleted or morphine-infused rats.Paw withdrawal thresholds to probing with von Frey filaments wereincreased to 15 ± 0 gm in both the morphine pellet-implanted (Fig.1) and morphine-infused groups of rats. Similarly, paw withdrawallatencies from a radiant heat source were increased by the microinjectionof lidocaine into the RVM. The postlidocaine withdrawal latencieswere 23.2 ± 3.6 and 21.1 ± 1.3 sec for the morphine pellet-implanted(Fig. 1) and infused groups, respectively. These data indicatethat RVM lidocaine returned sensory thresholds to, but not above,baseline levels. No behavioral abnormalities (ataxia, catatonia,loss of righting, or placement response) were noted in animalsreceiving RVM lidocaine. The microinjection of lidocaine intosites dorsal to the RVM, performed as a site control experiment(n = 4), produced motor hyperactivity including circling and barrel-rollingbehavior. No such signs were observed in rats with microinjectionsmade into the RVM. The administration of saline in the RVM producedno changes in sensory thresholds or motor function. Neither lidocaine(4% w/v) nor saline administered bilaterally (0.5:l) into theRVM impaired motor function. All animals remained on the rotaroduntil cutoff (data notshown).

In sham DLF-lesioned rats, subcutaneous morphine pellets elicited tactile allodynia and thermal hyperalgesia (measured onday 7 after morphine), as indicated by paw withdrawal thresholdsto von Frey filaments of 4.2 ± 0.7 gm and paw withdrawal latenciesto radiant heat of 13.9 ± 0.7 sec (Fig. 3). These values weresignificantly (p $<=$ 0.05) less than those of sham-DLF rats implantedwith placebo pellets. The corresponding values were 15 ± 0 gmand 20.6 ± 1.2 sec, respectively (Fig. 3). In rats with DLF lesions,subcutaneous morphine pellet-induced allodynia and hyperalgesiawere not observed. In these DLF-lesioned rats receiving subcutaneousmorphine pellets, the paw withdrawal thresholds (measured on day7 after morphine pellet) to von Frey filaments were 13.2 ± 1.8gm, and the paw withdrawal latencies to radiant heat were 21.2± 0.7 sec (Fig. 3). Lesions of the DLF did not change the behavioralresponses of the placebo-implanted rats (Fig. 3).

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Figure 3. Male Sprague Dawley rats received either bilateral lesions of the DLF or sham lesions. In addition, 2 d after surgery, animals received either subcutaneous implantation of placebo pellets or morphine (75 mg) pellets. No significant differences were observed in paw withdrawal thresholds to probing with von Frey filaments or to paw withdrawal latencies to radiant heat between animals receiving sham surgery and placebo pellets or DLF ablation and placebo pellets (A). Morphine pellet implantation resulted in tactile allodynia, as indicated by a significant (*p $<=$ 0.05; Student's t test; n = 10) decrease in paw withdrawal thresholds to probing with von Frey filaments (A), and thermal hyperalgesia, indicated by decreased paw withdrawal latencies to radiant heat (B), in the rats with sham DLF lesions. However, morphine-induced tactile allodynia (A) and thermal hyperalgesia (B) both were completely blocked in animals with bilateral DLF lesions. The paw withdrawal thresholds to probing with von Frey filaments and paw and the withdrawal latencies to radiant heat were significantly ( $dagger$ p $<=$ 0.05; Student's t test; n = 10) greater than those of morphine-pelleted, sham-lesioned rats. C, A schematic of the cross-sectional view of the thoracic spinal cord. The shaded area depicts the area of bilateral DLF lesions.

Baseline tail-flick latencies were 3.9 ± 0.14 sec and 4.02 ± 0.23 sec in placebo and morphine-pelleted groups (measured onday 7 after pellet implantation), respectively, values that werenot significantly different. The failure to detect hyperalgesiain the tail-flick response may reflect the rapid response latencyin this endpoint. RVM lidocaine did not alter baseline tail-flicklatencies in either placebo-pelleted or morphine-pelleted rats(data not shown). The subcutaneous implantation of morphine pelletsfor 7 d produced antinociceptive tolerance to intrathecal morphine.The antinociceptive dose-response for intrathecal morphine inrats with placebo pellets and bilateral administration of salineinto the RVM in the 52°C tail flick test had an A₅₀ value of 1.4µg [0.8-2.3; 95% confidence level (CL)]. The antinociceptive dose-responsefor intrathecal morphine in morphine pellet-implanted rats andbilateral administration of saline into the RVM was significantly(p $<=$ 0.05) shifted to the right, as indicated by an A₅₀ valueof 35.0 µg (26.3-46.8; 95% CL) (Fig. 4). The concurrent microinjectionof lidocaine (0.5 µl; 4% w/v) bilaterally into the RVM with intrathecalmorphine restored the antinociceptive potency of morphine to thatof the placebo-implanted rats (Fig. 4), as demonstrated by theA₅₀ value of 1.6 µg (0.9-2.7; 95% CL). The microinjection of lidocaineinto the RVM of the placebo pellet-implanted rats did not alterthe antinociceptive potency of intrathecal morphine. The intrathecalmorphine A₅₀ value was 1.7 µg (0.8-2.1; 95% CL) in the placebopellet-implanted group in the presence of lidocaine; this valuewas not significantly different (p > 0.05) from that of placebopellet alone (Fig. 4). The microinjection of saline into the RVMdid not alter the antinociceptive effects of spinal morphine.

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Figure 4. Male Sprague Dawley rats were implanted subcutaneous with either two placebo or two morphine (75 mg each) pellets. Antinociceptive dose-response curves for intrathecal morphine were generated in the 52°C water tail flick test at the time of peak effect of morphine (30 min as determined by pilot experiments). One group each of rats with placebo pellets and with morphine pellets received morphine intrathecally concurrently with bilateral RVM lidocaine (0.5 µl; 4% w/v). The following groups were used: placebo-pelleted rats with bilateral RVM saline and challenged with intrathecal morphine ( $open circle$ ), placebo-pelleted rats with bilateral RVM lidocaine and challenged with intrathecal morphine (), morphine-pelleted rats with bilateral RVM saline and challenged with intrathecal morphine (), and morphine-pelleted rats with bilateral RVM lidocaine and challenged with intrathecal morphine ( $black-square$ ). The dose-effect curve for intrathecal morphine in the morphine-pelleted group was shifted significantly to the right of that for the placebo-pelleted group. This dose-effect curve was restored that of the placebo-pelleted groups by RVM lidocaine.

The effect of lidocaine in the RVM was short-acting and reversible. The greatest reduction in A₅₀ value in morphine-tolerantrats occurred when lidocaine was microinjected concurrently withintrathecal morphine (Fig. 5). The microinjection of lidocaineeither 20 min before or after intrathecal morphine yielded A₅₀values of 29.0 µg (20.6-40.9; 95% CL) and 31.2 µg (17.5-55.8;95% CL), respectively. Likewise, the microinjection of lidocaineeither 10 min before or after intrathecal morphine yielded A₅₀values of 2.8 µg (1.5-5.0; 95% CL) and 8.9 µg (5.6-14.3; 95% CL),respectively.

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Figure 5. Male Sprague Dawley rats were implanted subcutaneously with either two placebo or two morphine (75 mg each) pellets. Antinociceptive dose-response functions for intrathecal morphine were generated in the 52°C water tail flick test at the time of peak effect of morphine (30 min). Lidocaine (0.5 µl; 4% w/v) was microinjected into the RVM at 0, 10, and 20 min before and after intrathecal morphine. The A₅₀ values were lowest, and similar to placebo-implanted values, when lidocaine was given concurrently with morphine. The largest A₅₀ values occurred when lidocaine was given 20 min before or after intrathecal morphine. These results demonstrate the reversibility of the effect of RVM lidocaine and suggest a direct causal relationship between inhibition of RVM activity and loss of morphine antinociceptive tolerance.

To further explore the possible bulbospinal contribution to behavioral manifestation of opioid antinociception, intrathecalmorphine dose-response curves were constructed using the 52°Ctail-flick test in animals with either bilateral DLF or sham lesionsin the presence of either morphine or placebo pellets. The antinociceptiveA₅₀ values for intrathecal morphine in animals with placebo pelletsand either DLF or sham lesions did not differ significantly (p $<=$ 0.05); the A₅₀ values were 3.0 µg (2.1-4.4; 95% CL) and 2.9µg (2.1-3.9; 95% CL), respectively. These values were also notsignificantly different from the A₅₀ value seen in unoperatedgroup which was 3.38 µg (2.0-3.7 µg; 95% CL). The antinociceptivedose-response for intrathecal morphine in animals with sham-DLFlesion on day 7 of morphine pellet implantation was significantly(p $<=$ 0.05) shifted to the right, as indicated by an A₅₀ valueof 19.8 µg (16.0-24.4; 95% CL) (Fig. 6). This value did not differsignificantly from that seen in unoperated rats implanted withmorphine pellets in which the A₅₀ value was 21.6 µg (17.7-26.4µg; 95% CL). However, the intrathecal morphine dose-response inanimals with DLF lesion and morphine pellets resulted in an A₅₀value of 2.8 µg (2.0-4.0; 95% CL) 7 d after pellet implantation(Fig. 6). This dose-response curve was similar to those of theunoperated or the placebo-pelleted control groups.

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Figure 6. Male Sprague Dawley rats received either bilateral lesions of the DLF or sham lesions. In addition, 2 d after surgery, animals received either subcutaneous implantation of placebo pellets or morphine (75 mg) pellets. After 7 d of pellet exposure, antinociceptive dose-response functions for intrathecal morphine were generated in the 52°C water tail flick test at the time of peak effect of morphine (30 min). The following groups were used: placebo-pelleted rats with sham DLF lesions ( $open circle$ ), placebo-pelleted rats with DLF lesions (), morphine-pelleted rats with sham DLF lesions (), and morphine-pelleted rats with DLF lesions ( $black-square$ ). The dose-effect curve for intrathecal morphine in the morphine-pelleted group was shifted significantly to the right of that for the placebo-pelleted group. This dose-effect curve of the morphine-pelleted group with DLF lesions was not different from that of the placebo-pelleted groups.

Lidocaine in the RVM in the absence of subcutaneous morphine did not significantly change tail-flick baseline latencies ineither placebo or morphine-pelleted rats (data not shown). Thesubcutaneous implantation of morphine pellets for 7 d also producedantinociceptive tolerance to subcutaneous morphine. The antinociceptiveA₅₀ value for subcutaneous morphine in rats with placebo pelletsin the 52°C tail flick test was 3.1 mg/kg (2.5-4.8; 95% CL). Theantinociceptive dose-response for subcutaneous morphine in themorphine pellet-implanted rats was significantly (p $<=$ 0.05) displacedto the right, as indicated by an A₅₀ value of 21.6 mg/kg (15.7-29.6;95% CL) (Fig. 7). The microinjection of lidocaine (0.5 µl; 4%w/v) bilaterally into the RVM concurrently with subcutaneous morphinerestored the antinociceptive potency of morphine to that of theplacebo-implanted rats (Fig. 7), as demonstrated by the A₅₀ valueof 4.2 mg/kg (3.6-5.1; 95% CL). The microinjection of lidocaineinto the RVM of the placebo pellet-implanted rats did not alterthe antinociceptive potency of subcutaneous morphine. The subcutaneousmorphine A₅₀ value of the placebo pellet-implanted group in thepresence of lidocaine was 2.8 mg/kg (2.2-3.5; 95% CL), and itwas not significantly (p > 0.05) different from that of placebopellet alone (Fig. 7). Saline injected in the RVM did not alterthe potency of subcutaneous morphine.

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Figure 7. Male Sprague Dawley rats were implanted subcutaneously with either two placebo or two morphine (75 mg each) pellets. Antinociceptive dose-response functions for subcutaneous morphine were generated in the 52°C water tail flick test at the time of peak effect of morphine (30 min). One group each of rats with placebo pellets and with morphine pellets received morphine subcutaneously concurrently with bilateral RVM lidocaine (0.5 µl; 4% w/v). The following groups were used: placebo-pelleted rats with bilateral RVM saline and challenged with subcutaneous morphine ( $open circle$ ), placebo-pelleted rats with bilateral RVM lidocaine and challenged with subcutaneous morphine (), morphine-pelleted rats with bilateral RVM saline and challenged with subcutaneous morphine (), and morphine-pelleted rats with bilateral RVM lidocaine and challenged with subcutaneous morphine ( $black-square$ ). The dose-effect curve for subcutaneous morphine in the morphine-pelleted group was shifted significantly to the right of that for the placebo-pelleted group. This dose-effect curve was restored to that of the placebo-pelleted groups by RVM lidocaine.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present results suggest that sustained morphine exposure elicits neuroplasticity resulting in tonic activation of descendingfacilitation. The importance of the RVM to the neuroplastic changesresulting in pain caused by tonic facilitation is demonstratedby (1) the time-related onset of opioid-induced pain and (2) thereversible blockade of opioid-induced pain by RVM lidocaine. Disruptionof the DLF, a principal neural conduit of spinopetal tracts fromthe RVM, including those mediating facilitation of pain, blockedopioid-induced pain without altering normal sensory thresholdsor motor activity. Importantly, opioid-induced pain was evidentduring the course of morphine delivery by continuous infusionwith osmotic minipumps, as well as by morphine pellets, minimizingpossible pharmacokinetic concerns about sustained opioid delivery.No signs of the opioid withdrawal syndrome were detected in spiteof careful monitoring, suggesting that opioid-induced pain observedwas not the result of abstinence or states of "mini-withdrawal"(Gutstein,1996). This conclusion is reinforced by the time-related onsetof opioid-induced pain, which was clearly detectable by day 3of morphine administration. The consequence of opioid-inducedpain was significant in determining subsequent opioid antinociceptivepotency. Our studies show that manipulations that block opioid-inducedpain, such as RVM lidocaine or DLF lesions, also restore morphineantinociceptive potency. These manipulations revealed no apparentalteration of antinociceptive signal transduction in morphine-pelletedrats. Based on such observations, the central hypothesis of thisinvestigation is that tonic activation of descending facilitationarising in the RVM represents a mechanism of chronic pain, includingthat induced by opioids, and that such opioid-induced pain manifestsbehaviorally as antinociceptivetolerance.

Some studies have reported opioid-induced hyperalgesia (Colpaert, 1996; Laulin et al., 1999) although others did not findthis effect (Kayser and Guilbaud, 1985; Gutstein et al., 1995).Reported "opioid-induced" hyperalgesia has been suggested to resultfrom the unmasking of compensatory neuronal hyperactivity occurringafter the opioid is removed or intermittently between injections(Gutstein, 1996). Whereas the nature of such neuronal hyperactivityremains to be elucidated, the resulting hyperalgesia could beinterpreted as the result of episodes of opioid "miniwithdrawals"(Gutstein, 1996). This possibility may apply to studies of opioidhyperalgesia conducted either after termination of opioid administrationor with repeated injections (Trujillo and Akil, 1991; Mao et al.,1994, 1995; Larcher et al., 1998; Laulin et al., 1998; Celerieret al., 2000).

The present studies with sustained morphine differ from these previous investigations in several important ways. First, ourdata show that sustained opioid administration elicits not onlythermal hyperalgesia but tactile allodynia as well. The latteris a manifestation of an abnormal pain state, in which sustainedopioid exposure resulted in normally non-noxious light touch producingapparent pain. Clinical reports exist of patients developing abnormalpain including both allodynia and hyperalgesia developed whilepatients were receiving opioids (Arner et al., 1988) and may bedifferent in location and quality than the original complaint(Ali, 1986; Stillman et al., 1987; Devulder, 1997). Second, thesebehavioral signs of abnormal pain were not immediate, but developedover a period of days, suggesting the need for neuronal plasticity.Third, allodynia and hyperalgesia developed and were maintainedduring continuous morphine delivery caused by either pellets orosmotic minipump. These similar results in spite of differencesin delivery systems minimize pharmacokinetic concerns and suggestthat the possibility that observed hyperesthesias might be attributableto opioid withdrawal is unlikely. Indeed, no signs of withdrawalwere observed despite carefulmonitoring.

Descending pain modulatory influences, including facilitation, have been identified in the RVM (Zhuo and Gebhart, 1992; Urbanet al., 1996; Urban and Gebhart, 1997; Fields and Basbaum, 1999).RVM neuronal populations include "OFF" cells that comprise a descendinginhibitory system and "ON" cells that facilitate nociceptive processingthrough spinopetal fibers (Fields et al., 1983, 1991; Fields andHeinricher, 1985). The existence of descending facilitation issupported by observations that prolonged stimulation with noxiousheat increased ON-cell and decreased OFF-cell activity and enhancednociceptive responses (Morgan and Fields, 1994). ON-cell activityhas been found to increase along with heightened nociception duringnaloxone-precipitated withdrawal (Bederson et al., 1990; Kim etal., 1990), which were blocked by lidocaine in the RVM (Kaplanand Fields, 1991). However, the state of ON-cell or OFF-cell firingduring sustained morphine administration, in the absence of withdrawal,has not been studied. The presence of such descending pain facilitationsystems in the RVM led us to hypothesize that opioid-induced painmight be the consequence of inappropriate tonic descending facilitation,possibly because of increased ON-cell discharge. Our data supportthis possibility. Tonic neuronal discharge in the RVM is supportedby our findings of blockade of opioid-induced pain by microinjectionof lidocaine into this site. This hypothesis is further strengthenedby the fact that spinopetal projections are known to descend throughthe DLF (Fields and Basbaum, 1999) and our observations in thepresent studies that DLF lesions also blocked opioid-inducedpain.

Our studies also show an intimate relationship between the presence of opioid-induced pain and the antinociceptive potencyof morphine. Manipulations that blocked opioid-induced enhancedpain, such as RVM microinjection of lidocaine or DLF lesion, alsorestored the spinal morphine antinociceptive potency. The specificityof the observed effects is reinforced by (1) the time-relatedrestoration of spinal morphine potency by RVM lidocaine and (2)the site-specificity of lidocaine administration. Additionally,neither RVM lidocaine or DLF lesion altered baseline sensory thresholds,motor activity, or the spinal morphine dose-effect curve in placebo-implantedrats, indicating no tonic activity of RVM systems under normalconditions and support the view of time-related RVM plasticityto initiate descending facilitation, opioid-induced abnormal pain,and subsequent decreased spinal antinociceptive potency of morphine.These data reasonably suggest that spinal morphine antinociceptivepotency depends on the intrinsic baseline nociceptive state andthat the observed spinal potency of morphine reflects this painstate in animals as it does clinically (Cherney and Portenoy,1999).

Systemic morphine antinociceptive potency is known to depend on antinociceptive synergy between spinal and supraspinal actions(Yeung and Rudy, 1980; Roerig and Fujimoto, 1989). This site-sitesynergy may be an important factor in the clinical potency andultimate utility of this molecule. An important feature of opioidtolerance is the loss of antinociceptive spinal/supraspinal synergy(Roerig et al., 1984; Roerig and Fujimoto, 1988). It seems reasonableto suggest that the observed decreased antinociceptive potencyof systemic morphine in morphine pellet-implanted rats resultsfrom a loss of supraspinal-spinal antinociceptive synergy andthat an important contributor to such lost synergy is the decreasedspinal morphine potency in these rats. Our finding that RVM lidocainerestored systemic morphine antinociceptive potency might be interpretedas resulting from the restoring supraspinal-spinal synergy subsequentto normalizing spinal morphine activity caused by blockade ofdescending facilitation. Isobolographic analysis will be requiredto confirm thisidea.

It has been determined that disinhibition of OFF cells is the principal mechanism of opioid-mediated antinociception in theRVM (Heinricher et al., 1994). In the present study, systemicmorphine was active in both the morphine- or placebo-pelletedgroups after RVM lidocaine. Because lidocaine would be expectedto inhibit essentially all RVM neuronal activity, it seems likelythat the disinhibition of RVM OFF cells may not be solely responsiblefor supraspinal opioid-mediated antinociception. Many supraspinalsites that mediate antinociception bypass the RVM either partlyor completely (for review, see Fields and Basbaum, 1999). Forexample, the periaqueductal gray (PAG), a major source of projectionsto the RVM and of opioid-mediate antinociception, also sends someprojections directly to the spinal cord (Castiglioni et al., 1978;Willis and Westlund, 1997). Furthermore, the PAG has neuronalcommunications with noradrenergic nuclei, including the locuscoeruleus, A5, and A7, and these regions also have direct spinopetalprojections (for review, see Fields and Basbaum, 1999). Such projectionsmay be sufficient to reinstate hypothesized supraspinal-spinalopioid synergy subsequent to restoration of spinal morphine antinociceptivepotency in morphine-pelleted rats after RVM lidocaine. Furtherexperimental data will be required to substantiate thisconcept.

The results of the present investigation support the hypothesis that tonic descending facilitation may be an important mechanismof chronic pain and may underlie not only pain from sustainedopioids but other conditions as well. In this regard, the abnormalpain elicited by experimental spinal nerve injury is also blockedby RVM lidocaine (Kovelowski et al., 2000). Additionally, experimentalneuropathic pain is associated with decreased spinal morphineantinociceptive potency (Bian et al., 1999), which is restoredby RVM lidocaine (Kovelowski et al., 2000). Additionally, DLFlesions also blocked nerve injury-induced pain (Ossipov et al.,2000). Taken together, these data support the view that abnormalpain caused by tonic descending facilitation from the RVM decreasesthe antinociceptive potency of spinal (and systemic) morphine.Blockade of the pain restores spinal morphine potency and mayreinstate supraspinal-spinal opioid antinociceptive synergy aftersustained opioid exposure or resulting from nerve injury (Bianet al., 1999). The decrease in spinal opioid antinociceptive potencyseen under conditions of sustained opioids or nerve injury maytherefore underlie the apparent loss of opioid analgesia (i.e.,tolerance) seen clinically with opioid use for chronic pain orthe limited opioid activity seen in neuropathic pain patients.Our data show no apparent change in antinociceptive signal transductionafter blockade of opioid-induced pain. It seems likely that approachesthat may block the RVM plasticity associated with sustained opioidexposure (or nerve injury) may allow sustained analgesic efficacyof opioids and their use in treatment of chronicpain.

  FOOTNOTES

Received Sept. 1, 2000; revised Oct. 11, 2000; accepted Oct. 13, 2000.

Correspondence should be addressed to Dr. Frank Porreca, Department of Pharmacology, College of Medicine, University of ArizonaHealth Sciences Center, Tucson, AZ 85724. E-mail: frankp{at}u.arizona.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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