Substance P Release in the Rat Periaqueductal Gray and Preoptic Anterior Hypothalamus after Noxious Cold Stimulation: Effect of Selective Mu and Kappa Opioid Agonists

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Vol. 282, Issue 2, 1055-1063, 1997

Substance P Release in the Rat Periaqueductal Gray and Preoptic Anterior Hypothalamus after Noxious Cold Stimulation: Effect of Selective Mu and Kappa Opioid Agonists¹

Li Xin, Ellen B. Geller, Lee-Yuan Liu-Chen, Chongguang Chen and Martin W. Adler

Department of Pharmacology, Temple University School of Medicine, Philadelphia, Pennsylvania

	Abstract

Top Abstract Introduction Methods Results Discussion References

Intracerebral microdialysis was used to measure changes in the extracellular level of substance P (SP) released from the periaqueductalgray (PAG) and the preoptic anterior hypothalamus (POAH) of freelymoving Sprague-Dawley rats after noxious cold stimulation. Artificialcerebrospinal fluid was perfused into the dialysis probe in thePAG or POAH and samples were collected every 30 min for 4 hr.SP-like immunoreactivity in the samples was measured by radioimmunoassay.In the PAG, SP base-line release was 0.43 ± 0.08 fmol/fraction.SP release was increased to 1.3 ± 0.4 fmol/fraction during thefirst collection period after noxious cold. Pretreatment withthe selective mu opioid receptor agonist PL017 (0.8-3.4 nmol)or the kappa opioid receptor agonist dynorphin A1-17 (4.6-9.2nmol), administered into the PAG by microinjection, produced dose-relatedinhibition of the cold-evoked SP release. Naloxone (10 mg/kg s.c.)administration 10 min before these opioid agonists reduced theinhibition of SP release. In the POAH, SP base-line release was0.45 ± 0.06 fmol/fraction and noxious cold did not cause any significantchange in SP release. Microdialysis of SP (271 fmol-271 pmol/µl/min,for 30 min) into the PAG, but not the POAH, induced dose-relatedanalgesia (35-68% MPA) in the cold-water tail-flick test. However,microdialysis of SP into the POAH or PAG failed to induce anysignificant change in body temperature. These data suggest that1) SP released from the PAG acts as a neuromodulator to transmitnociceptive information; 2) opioid receptor agonists can suppressthis information by inhibiting SP release; 3) SP evoked by noxiouscold may have a role in triggering the antinociceptive functionof the PAG; and 4) SP does not appear to act as a neuromodulatorfor thermoregulatory responses in the POAH.

	Introduction

Top Abstract Introduction Methods Results Discussion References

SP is either a neurotransmitter or a neuromodulator in conduction of nociceptive information in the CNS (Marx, 1979). Duringnoxious cold or mechanical stimuli, the SP release level is increasedin the spinal cord (Kuraishi et al., 1985; Tiseo et al., 1990)and this increased SP release can be inhibited by pretreatmentwith opioids (Kuraishi et al., 1983; Tiseo et al., 1990; Yakshet al., 1980). These findings suggest that SP may carry or modulatenoxious signals to the CNS and that opioids produce their analgesiceffects by suppressing SP release. It has been proposed that SPcan be released not only from the spinal cord but also from thebrain regions that are involved in endogenous pain suppression,such as the PAG, to transmit afferent noxious signals and activatethe pain-modulating pathway descending from the PAG (Basbaum andFields, 1984). Indeed, SP-immunoreactive neurons, nerve terminals(Hökfelt et al., 1977; Moss and Basbaum, 1983) and receptors(Quirion et al., 1983) can be observed in the PAG. Some of theascending inputs to the PAG from the spinal cord contain SP (Noguchiand Ruda, 1992). SP can be released from brain tissue slices (Iversenet al., 1976; Calvo et al., 1990) or certain brain regions invivo (Brodin et al., 1983; Lindefors et al., 1986, 1987; Morilaket al., 1988) by stimulation with potassium. The findings thatSP microinjection into the PAG produces naloxone-reversible analgesia(Malick and Goldstein, 1978; Mohrland and Gebhart, 1979) and thatopioids inhibit SP release from the brain (Micevych et al., 1982;Rosen and Brodin, 1989) suggest that SP within the brain may playa neuromodulatory role in transmitting nociceptive informationand interact with either endogenous opioid peptides or exogenousopioid drugs. A previous report from our laboratory has shownthat noxious cold stimulation to the rat's tail induced elevationof SP release from the spinal cord, whereas noxious heat inducedelevation of somatostatin release (Tiseo et al., 1990). The SPincrease could be inhibited by i.c.v. pretreatment with Dyn. Itis not known, however, if noxious cold can also induce an increaseof SP in the brain. SP release from brain regions in vivo is detectableby a combination of intracerebral microdialysis and RIA methods(Brodin et al., 1983; Lindefors et al., 1986, 1987).

In the present study, with use of intracerebral microdialysis and RIA, we investigated SP release from the PAG after noxiouscold-water stimulation with or without pretreatment with the muopioid receptor agonist PL017 or the kappa opioid receptor agonistDyn. We reported previously that both drugs produce analgesiceffects when dialyzed into the PAG in the CWT (Xin et al., 1993).For comparison, we also investigated whether noxious cold couldinduce any change in SP release level from another brain region,i.e., the POAH, which is a primary site for Tb regulation andcontains SP nerve terminals and receptors (Panula et al., 1984).Finally, SP was perfused into the PAG and POAH to examine itseffects on analgesia and Tb.

	Methods

Top Abstract Introduction Methods Results Discussion References

Animals. Male Sprague-Dawley rats (Zivic-Miller, Pittsburgh, PA) weighing 250-300 g were used in this study. They were housed threeper cage for at least 1 week before surgery and were fed laboratorychow and tap water ad libitum. The temperature of the room was22 ± 2°C and a 12-hr light/12-hr dark cycle was used.

Microdialysis probe preparation. The microdialysis probes used in this study were constructed in a concentric shape consisting of a 1.5-mm length of hollowtubular dialysis membrane (acrylonitrile-sodium methallyl sulfonate,40-kdalton molecular weight cutoff, 230 µm internal diameter,300 µm outside diameter, Hospal, Uden, The Netherlands) with thetip sealed by epoxy resin and the other end mounted to a 26-gaugethin-wall stainless steel cannula (15-mm length, Small Parts,Inc., Miami Lakes, FL). A 22-mm length of thin polyimide-coatedfused silica tubing (75 µm internal diameter, 140 µm outside diameter,Polymicro Technologies, Phoenix, AZ) as an inlet was threadedthrough the stainless steel cannula into the dialysis membrane,leaving approximately 0.4 mm free between the end of the silicatubing and the epoxy at the tip of the dialysis membrane. Another22-mm length of fused silica tubing as an outlet was also threadedthrough the stainless steel cannula into the upper end of thedialysis membrane. The upper end of the stainless steel cannulawas sealed by epoxy after both inlet and outlet silica tubingwere inserted. For administration of opioid agonists, a 30-mmlength of fused silica tubing was attached to the outside of thestainless steel cannula to form a side catheter, with its tipnear the tip of the dialysis membrane. The upper ends of inlet,outlet and side catheter were each connected with a length ofPE-10 tubing. A schematic drawing of the probe with attached cathetheris shown in figure 1.

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Fig. 1. Schematic drawing of the probe with attached catheter used in the experiments. (A) inside view of the probe; (B) outside viewof the probe.

Surgery and probe implantation. Rats were anesthetized with an i.m. injection of a mixture of ketamine hydrochloride (100-150 mg/kg) and acepromazine maleate(0.2 mg/kg) and stereotaxically (Pellegrino and Cushman, 1967)implanted unilaterally with a guide cannula (21-gauge stainlesssteel tubing, 14 mm long, Small Parts, Inc., Miami Lakes, FL)into the location above the PAG (AP, 0.6; R, 0.8; V, 1.0) or POAH(AP, 7.8; R, 1.0; V, $-$ 1.0). A stylet was inserted into the guidecannula, which was fixed with dental cement and self-tapping bonescrews. A slotted hex head screw (Instech Laboratories, Inc.,Plymouth Meeting, PA) was inversely fixed on the skull behindthe cannula with dental cement for attachment of a tether. Aftersurgery, animals were housed individually to prevent them fromdestroying the cannula and were allowed to recover from the surgeryat least 7 days. One day before the experiment, the rat was anesthetizedagain with ketamine and the stylet was replaced by a microdialysisprobe, so that its dialysis membrane tip protruded exactly 1.5mm beyond the guide and was located within the PAG or POAH. aCSF(see "Materials") was injected into the side catheter (0.2 µl)from its inlet to avoid the injection of air into the brain duringthe experiment, after which the inlet was sealed.

Materials. The following drugs were tested: mu opioid receptor agonist PL017 (Tyr-Pro-N-MePhe-D-Pro-NH₂); kappa opioid receptor agonistDyn (both from Multiple Peptide Systems, San Diego, CA); naloxone(Nal, DuPont Merck Pharmaceutical Co., Wilmington, DE), and SP(Peninsula Laboratories, Inc., Belmont, CA). aCSF (compositionin mM: NaCl, 125; KCl, 2.5; NaH₂PO₄, 0.5; Na₂HPO₄, 5; CaCl₂, 1.2;MgCl₂, 1; ascorbic acid, 0.1; and bovine serum albumen, 0.025%,pH 7.4) was the vehicle and control solution. SP antiserum wasprepared in rabbits and was generously provided by Dr. Susan E.Leeman of Boston University. The final dilution of the antiserumused was 1:180,000. Half-maximal displacement was 2 fmol/250 µl.Cross-reactivities of this antiserum were such that no measurabledisplacement was observed at 100 pM with substance K, met-enkephalin,somatostatin or physalaemin. Isotope [¹²⁵I]Tyr⁸-SP was purchased from Dupont New England Nuclear Research Products(Boston, MA). The second antiserum (goat anti-rabbit $gamma$ -globulin),used for separation of anti-SP-bound tracer from free tracer,was purchased from Calbiochem Corporation (La Jolla, CA).

Microdialysis in vivo experiments. On the test day, the rat was placed into an individual plastic cage where it could move freely in an environmental room keptat 21 ± 0.3°C and 52 ± 2% relative humidity. A light-weight stainlesssteel spring tether (30.5 cm, M105, Instech Laboratories, Inc.,Plymouth Meeting, PA) was connected to the screw captured in thehead block by inserting the tether blade into the slot of thescrew. A small tubular nut locked the tether in place. The upperend of the tether was attached to the clamp of a single-channelswivel (series 375, Instech Laboratories, Inc., Plymouth Meeting,PA) which was held on a lever arm. A length of PE-10 tubing wasthreaded through the tether and connected with the output of theswivel and the input cannula of the dialysis probe. The inputof the swivel was then connected to a 1-ml tuberculin syringe(Becton Dickinson & Co., Rutherford, NJ) clamped to a perfusionpump (Harvard Apparatus, Inc., South Natick, MA). The output ofthe probe was connected with a length of PE-10 tubing fed intoa 1.5-ml polyethylene collection tube which was mounted in a tubeholder clipped on the tether just over the rat's head. aCSF wascontinually perfused into the dialysis probe at a rate of 4 µl/min.After at least a 1-hr perfusion for equilibrium, dialysate sampleswere collected every 30 min for 240 min. Samples were frozen immediatelyafter collection and stored at $-$ 70°C until assayed. The firstthree samples were collected as base-line release for SP. Thenoxious cold stimulus was performed by placing the rat's tailinto a circulating cold water bath (model 9500, Fisher Scientific,Pittsburgh, PA) until the animal flicked its tail or reached cutofftime (20 sec/min), in a 1:1 mix of ethylene glycol/water maintainedat $-$ 10°C. The cold stimulus was given five times during a 5-mintest period. In some cases, a water bath of 25°C was also usedas a control. The mu opioid receptor agonist PL017 (0.8-3.4 nmol),the kappa opioid receptor agonist Dyn (2.3-9.2 nmol) or aCSF wasmicroinjected in a volume of 0.5 µl into the brain region throughthe side catheter attached to the dialysis probe 5 min beforethe noxious cold stimulus. In two groups, Nal (10 mg/kg) was administereds.c. 10 min before microinjection of PL017 or Dyn into the PAG.

RIA. In each RIA, standard curves were constructed for SP by use of known amounts of synthetic standards ranging from 0.1 to 24fmol. The assay was carried out directly in the tubes used forcollection of the dialysate fractions during microdialysis. Thedialysate fractions (120 µl) and the SP standards in aCSF (120µl) were preincubated with rabbit antiserum against SP (80 µl)for 24 hr at 4°C. After addition of [¹²⁵I]Tyr⁸-SP (2500-3500 cpm in 80 µl; approximate specific activity 81TBq/mmol = 1480 µCi/µg), all samples were further incubated for24 hr at 4°C. To separate bound from free tracer, the second antiserumwas added to each assay tube at the end of incubation as recommendedby the manufacturer. All assay tubes were vortexed briefly andcentrifuged for 20 min at 760 × g by a refrigerated SUREspin centrifugeat 4°C. The supernatant was carefully decanted and the precipitatecontaining antibody-bound [¹²⁵I]Tyr⁸-SP was counted in a gamma counter (NE-1600, Nuclear Enterprises,Scotland, UK). Levels of SP were then calculated by linear regressionanalysis derived from logarithmic transformation of data determinedfor known amounts of synthetic SP. Separate samples without standardsand additional samples also without antibodies were incubatedsimultaneously to measure maximal tracer binding and unspecificbinding, respectively. The detection limit of this assay was 0.2fmol/250 µl.

Microdialysis in vitro. In vitro recovery of SP through the acrylonitrile membrane was determined by placing microdialysis probes in aCSF solution(200 µl, at 37°C bath) containing 1 nM synthetic SP. The probeswere continuously perfused at a flow rate of 4 µl/min. After equilibrium,three 120-µl samples of perfusate were collected and assayed forSP by RIA as described above. The SP-containing aCSF solutionwas also assayed. The recovery of the probe membrane was determinedby calculating the percentage of the SP concentration in the perfusateversus that in the medium solution. The in vitro recovery of thisdialysis membrane for SP was 1.9 ± 0.6% (mean ± S.E.M., n = 6).The percentage of the amount of SP that may bind to the probematerial or tubing was 0.2 ± 0.12% (mean ± S.E.M., n = 5). Thiswas estimated by the difference between the SP amount in the inputsolution and the sum of SP amount in the both perfusate and mediumsolutions.

Analgesia testing. Separate experiments were conducted to investigate the analgesic effect of SP microdialyzed into the PAG or POAH of the rat.The microdialysis system used to deliver SP into the PAG or POAHwas similar to that described above (see "Microdialysis in VivoExperiments") without the sample collecting and microinjectingprocedures. At the beginning, aCSF was continuously perfused intothe brain regions at 4 µl/min. The CWT was used to assess theanalgesic effects of SP according to standard procedures in ourlaboratory (Tiseo et al., 1988). Animals were held firmly overthe water bath ( $-$ 10°C) and their tails submerged approximatelyhalf-way into the solution. The nociceptive threshold was takenas the latency until the rat removed or flicked its tail. Threelatencies were measured: 60, 30 and 0 min before drug perfusion.For each animal, the first reading was discarded to minimize variability,and the remaining two were averaged to determine the base-linelatency. After the predrug latency measurements, the input solutionwas switched to the SP-containing aCSF (27.1 fmol-271 pmol/µl)and was continuously perfused at 4 µl/min for 30 min. The latencyto tail-flick was tested at the end of SP perfusion and 15, 30,60 and 120 min after that. If an animal did not respond within60 sec, the trial was terminated and a maximum latency of 60 secwas recorded. The analgesic effect of SP treatment was calculatedfor each rat as follows: percent maximum possible analgesia (%MPA) = [(postdrug latency $-$ base-line latency)/(60-base-line latency)]× 100. In some cases, Nal in a dose of 10 mg/kg was injected s.c.10 min before the CWT to investigate the effect of Nal injectionalone on the tail-flick response. Testing was also carried outafter pretreatment with Nal (10 mg/kg s.c.) 10 min before thelow dose (27.1 fmol/µl) or high dose (271 pmol/µl) of SP perfusion.

Tb response testing. Effects on Tb of SP microdialyzed into the PAG or POAH were also investigated in separate experiments. The microdialysis procedurewas the same as that used in the analgesia testing. Tb measurementswere made according to standard procedures in our laboratory (Gelleret al., 1986). After a 1-hr acclimation period, a thermistor probe(YSI series 400, Yellow Springs Instrument Co., Inc., Yellow Springs,OH) was lubricated and inserted approximately 7 cm into the rectum.The rat was lightly hand-held by the tail, but was otherwise freeto move. Tb measurements were read from a digital thermometer(model 49 TA, YSI). The first three measurements were taken at30-min intervals. To allow for adaptation to the procedure, thefirst reading was discarded and the subsequent two averaged toestablish a base line. After the third measurement, the inputsolution was switched to SP-containing aCSF and perfused at 4µl/min for 30 min. Tb was measured at the end of SP perfusionand 15, 30, 45, 60, 90 and 120 min later.

Verification of dialysis probe placement. At the end of the experiments, rats were placed for at least 10 min into a bucket containing dry ice within a metal mesh basket.The animals were almost instantaneously anesthetized by the carbondioxide, rapidly asphyxiated and cooled. Their brains were excisedand coronally cut; the visible track of the microdialysis probewas checked. In some cases, bromophenol blue (0.2%) was microdialyzedinto the PAG or POAH for 30 min after the experiment ended. Thebrains were removed, rapidly frozen and stored at $-$ 70°C. A blockof tissue containing the track of the probe and the stain of thedialyzed dye was cut and checked (fig. 2). Data from rats in whichthe probes were not located within the PAG or POAH were not includedin the results.

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Fig. 2. Photographs of coronal sections of rat's brain showing spread of bromophenol blue after 30 min dialysis into the PAG (A) andPOAH (B). Arrows point to the edge of the dye stain. Horizontalbar = 1 mm in length. Ac, anterior commissure; aq, aqueductus;oc, optic chiasm; pag, periaqueductal gray; poah, preoptic anteriorhypothalamus.

Data presentation and statistical analysis. The results for SP are reported as mean ± S.E.M. values of the measured dialysate concentrations. The results for the analgesiceffect of SP are reported as % MPA (mean ± S.E.M.). The resultsfor the Tb effect of SP are expressed as Tb changes ( $Delta$ T, mean± S.E.M.) from base line. The changes of cold-evoked SP releasein the groups pretreated with opioid agonists and Nal are expressedas the percentage of cold-evoked SP in the group without pretreatment.In the experiment that examined the effects of pretreatment withopioid agonists and Nal on cold-evoked SP release, data were evaluatedby a one-way analysis of variance followed by a post hoc Fisher'stest. Other experimental data were analyzed by a repeated-measuresanalysis of variance model, in which factor 1 was treatment andfactor 2 was time. The 5% level of probability was accepted asstatistically significant.

	Results

Top Abstract Introduction Methods Results Discussion References

SP base-line release from the PAG and POAH. The average basal release of SP from the PAG was 0.43 ± 0.08 fmol/fraction during the 3-hr collection period (table 1). Inthe POAH, SP base-line release was 0.45 ± 0.06 fmol/fraction duringthe 3-hr collection period.

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TABLE 1
SP base-line release (fmol/fraction, means ± S.E.M.) from the PAG and the POAH of freely moving rats

SP release from the PAG after noxious cold stimulation. SP release level was significantly increased to 1.3 ± 0.4 fmol/fraction during the collection period of 30 min after noxiouscold stimulation and then returned to base-line level during thenext collection period (fig. 3, top). In contrast, 25°C waterdid not produce any significant change in SP released from thePAG.

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Fig. 3. (Top panel) Changes of SP release level (mean ± S.E.M.) in the PAG after noxious cold ( $-$ 10°C, solid column, n = 6) or 25°Cwater (open column, n = 5) stimulation to the rat's tail. (Bottompanel) Changes of SP release level (mean ± S.E.M.) in the POAHafter noxious cold (solid column, n = 5) or 25°C water (open column,n = 4) stimulation to the rat's tail. Arrow represents the timewhen the stimulation starts. *P < .05, compared with 25°C waterstimulation group.

SP release from the POAH after noxious cold stimulation. Neither noxious cold nor 25°C water stimuli evoked any significant change in the level of SP released from the POAH (fig.3, bottom).

Effects of pretreatment with PL017 in the PAG on SP release evoked by noxious cold. Although aCSF microinjection into the PAG did not affect the SP increase evoked by cold, PL017 microinjected into the PAGsignificantly reduced the SP release evoked by noxious cold ina dose-dependent manner (fig. 4, top). PL017, in a dose of 0.8nmol, reduced the cold-evoked SP increase level to an average0.48 fmol/fraction increase over base-line, a 42% reduction comparedwith that in the aCSF-pretreatment group (0.84 fmol/fraction equals100%). PL017, in dose of 1.7 nmol, reduced that SP increase 66%and 3.4 nmol, 89%, compared with that in the aCSF-pretreatmentgroup. These doses of PL017 were capable of producing analgesia(40% MPA-85% MPA) in the CWT in earlier studies (Adams et al.,1993; Xin et al., 1993).

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Fig. 4. (Top panel) Effects of pretreatment with aCSF, different doses of PL017 (0.8, 1.7 and 3.4 nmol) and Nal (10 mg/kg) plus PL017(3.4 nmol) on the cold-evoked SP increase in the PAG. (Bottompanel) Effects of pretreatments with aCSF, different doses ofDyn (2.3, 4.6 and 9.2 nmol) and Nal (10 mg/kg) plus Dyn (9.2 nmol)on the cold-evoked SP increase in the PAG. The average increasedSP level (0.84 fmol/fraction) evoked by the cold over base-linerelease (0.43 fmol/fraction) in the non-pretreatment group istaken as 100%. The average increased SP level in each pretreatmentgroup is compared with that in the non-pretreatment group. n =4 in each group. *P < .05.

Effects of pretreatment with Dyn in the PAG on SP release evoked by noxious cold. Pretreatment with Dyn administered into the PAG also produced an inhibition in SP release evoked by noxious cold (fig. 4,bottom). Dyn, in doses of 4.6 and 9.2 nmol, reduced the elevationin SP release evoked by noxious cold to an average 0.54 and 0.11fmol/fraction increase over base line, respectively, a 36 to 87%reduction compared with that in the aCSF-pretreatment group (0.84fmol/fraction equals 100%). These doses of Dyn were capable ofproducing analgesia (28% MPA-70% MPA) in the CWT, as reportedpreviously (Tiseo et al., 1988; Xin et al., 1993). Dyn, in a doseof 2.3 nmol, did not induce significant changes in cold-evokedSP increase.

Effect of Nal on the inhibition of cold-evoked SP release caused by PL017 and Dyn. Nal (10 mg/kg) administered s.c. 10 min before PL017 or Dyn microinjection reduced the inhibition of cold-evoked SP increaseby these opioid agonists. The 89% reduction of SP increase causedby PL017 (3.4 nmol) was decreased to a 7% reduction when Nal wasgiven before PL017 (fig. 4, top). The 87% reduction of SP increasecaused by Dyn (9.2 nmol) was decreased to only 6% when Nal wasgiven before Dyn (fig. 4, bottom).

Effects of SP microdialyzed into the PAG and POAH on the latency to tail-flick. The lowest dose (27.1 fmol/µl) of SP microdialyzed into the PAG produced a slight but not significant increase in latencyto tail-flick in the CWT (fig. 5). After a 30-min perfusion atthis dose, the amount of SP delivered into the PAG can be estimatedat as much as 65 fmol, which is the mean amount of extracellularSP evoked by cold, according to the in vitro recovery rate ofthe probe for SP. However, higher doses of SP microdialyzed intothe PAG produced a dose-related analgesia. SP in a dose of 271fmol/µl, which is 10 times higher than the lowest dose, induced30% MPA at 30 min after the end of SP perfusion; and SP, in adose of 27.1 pmol/µl, induced 41% MPA at 15 min. SP, in dosesof 271 pmol/µl, produced 35% MPA at the end of the perfusion and65% MPA 15 min later. The analgesic effect lasted until 30 minafter the end of perfusion (38% MPA). However, SP, in doses whichcould produce analgesia when given into the PAG, did not induceany significant change in the tail-flick latency when it was microdialyzedinto the POAH (fig. 6).

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Fig. 5. Effects of different doses of SP microdialyzed into the PAG on antinociception in the CWT. SP was perfused at 4 µl/min for30 min. Horizontal bar represents the perfusion period. n = 4-6in each group. *P < .05, compared with aCSF group. Base-line latencyvalues for each group (sec, mean ± S.E.M.): 10 ± 3 in aCSF group;13 ± 2 in SP 27.1 fmol/µl group; 11 ± 3 in SP 271 fmol/µl group;12 ± 2 in SP 27.1 pmol/µl group; 11 ± 2 in SP 271 pmol/µl group.

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Fig. 6. Effects of SP microdialyzed into the POAH on antinociception of the rat in the CWT. SP was perfused at 4 µl/min for 30 min.Horizontal bar represents the perfusion period. n = 4-6 in eachgroup. SP was perfused at 4 µl/min for 30 min. Horizontal barrepresents the perfusion period. n = 4-6 in each group. Base-linelatency values for each group (sec, mean ± S.E.M.): 10 ± 3 inaCSF group; 11 ± 2 in SP 27.1 pmol/µl group; 10 ± 2 in SP 271pmol/µl group.

Effects on tail-flick latency of SP microdialyzed into the PAG after pretreatment with Nal. Nal (10 mg/kg s.c.) alone induced a small decrease in tail-flick latency ( $-$ 7% MPA at 30 min, $-$ 5.2% MPA at 45 min, $-$ 2.5% MPAat 60 min) (fig. 7), which was not functionally significant (basedon the standard used in our laboratory, at least ± 20% changein MPA is considered a significant response in the CWT). Pretreatmentwith Nal (10 mg/kg, s.c.) 10 min before microdialysis of a lowdose of SP (27.1 fmol/µl, by which no significant change in tail-flicklatency was produced) into the PAG induced a similar response( $-$ 7.5% MPA at 30 min) to that seen with Nal given alone. Pretreatmentwith s.c. Nal 10 min before microdialysis of a high dose of SP(271 pmol/µl) into the PAG significantly blocked the analgesiceffect of this dose of SP.

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Fig. 7. Effects of Nal (10 mg/kg s.c.) alone or 10 min before SP perfusion on antinociception of the rat in the CWT. SP was perfusedat 4 µl/min for 30 min. Horizontal bar represents the perfusionperiod. n = 4-6 in each group. Base-line latency values for eachgroup (sec, mean ± S.E.M.): 12 ± 2 in Nal alone group; 10 ± 3in SP 27.1 fmol/µl group; 11 ± 3 in SP 271 pmol/µl group.

Effects of SP microinjected into the PAG and POAH on Tb. The same doses of SP (27.1-271 pmol/µl) that produced analgesia in the PAG failed to produce any significant change in Tbwhen microdialyzed into the PAG and POAH (fig. 8).

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Fig. 8. Tb responses of the rats to SP microdialyzed into the POAH or PAG. SP was perfused at 4 µl/min for 30 min. Horizontal barrepresents the perfusion period. $Delta$ T, Tb changes compared withthe Tb base line before SP perfusion. The Tb base lines (mean± S.E.M.) were 37.9 ± 0.18°C to 38.2 ± 0.14°C. n = 4-6 in eachgroup.

	Discussion

Top Abstract Introduction Methods Results Discussion References

It has been reported by our laboratory and others that SP release could be evoked from the spinal cord by noxious cold (Tiseoet al., 1990) or noxious mechanical (Kuraishi et al., 1983, 1985)stimuli. The increased SP level is selective for noxious coldand mechanical stimuli as there is no such increase during noxiousheat (Kuraishi et al., 1985; Tiseo et al., 1990). The PAG is oneof the brain regions that receives a major projection arisingfrom the spinal cord lamina I pain-responsive neurons (Hyldenet al., 1986). One study with retrograde labeling and in situhybridization histochemistry demonstrated that 61% of the spinomesencephalicprojection neurons (part of which distribute to the PAG) in laminaI of the spinal cord express preprotachykinin mRNA (which encodestachykinin peptides, including SP), and this expression is significantlyincreased (80%) after peripheral inflammation, which indicatesthat SP plays an important role in nociception in ascending CNSpathways (Noguchi and Ruda, 1992). Other studies showed that thePAG also contains extensive SP-positive nerve terminals as wellas cell bodies (Hökfelt et al., 1977; Moss and Basbaum 1983)and moderate-to-high concentrations of SP receptors (Quirion etal., 1983). In addition, reports indicated that tissue levelsof SP in the PAG can be changed after administration of drugs(Brodin et al.,1987; Rosen and Brodin, 1989). Increased SP releasewithin the PAG during cold stimulation may represent a nociceptivesignal arising from the spinal cord to this region. This ideais supported by the present observation that there is an immediateincrease of SP release (the first 30-min collection) from thePAG after noxious cold water, but not 25°C water, stimulation.On the basis of the present results, however, we could not determinewhether the increased SP in the PAG was released by the nerveterminals projecting directly from the spinal cord or by the localSP-containing cells within the PAG which were secondarily excitedby the spinal cord ascending projection.

Our observations that pretreatment with an analgesic dose of PL017 (fig. 4, top) or Dyn (fig. 4, bottom) inhibits the cold-evokedSP increase in this region and that this inhibition can be reversedby the opioid receptor antagonist Nal support the hypothesis thatincreased SP within the PAG carries noxious input. It has beenproposed that the PAG is one of several brain regions involvedin the modulation of nociceptive input through descending inhibitoryneuronal processes that project to the spinal cord (Basbaum andFields, 1984). Administration of opioids into the PAG (Jensenand Yaksh, 1986; Smith et al, 1992) or electrical stimulationof the PAG (Basbaum et al., 1977) produces antinociception andreduces the firing of nociresponsive dorsal horn neurons (Bennettand Mayer, 1979; Gebhart and Jones, 1988). Both mu and kappa opioidreceptors exist within the PAG (Mansour et al., 1995). Our previousreports have shown that activation of the mu and kappa opioidreceptors in the PAG by administration of PL017 and Dyn, respectively,into this region produces dose-related analgesia in the CWT (Xinet al., 1993). These findings suggest that opioid administrationsuppresses the neuronal activities and the neurotransmitters whichtransmit pain input. A reasonable explanation for the inhibitionof SP increase after pretreatment with PL017 and Dyn would bethat increased SP release within the PAG represents the noxiousinformation during the cold-water stimulation. Similar resultshave been reported in studies by Tiseo et al. (1988, 1990) inwhich i.c.v. injection of Dyn induced analgesia in the CWT andprevented the increase of SP released from the spinal cord duringnoxious cold. Also, Yaksh et al. (1980) reported a 4.9-fold increasein SP release from the spinal cord by activating the sciatic nerveand a naloxone-reversible inhibition of the SP release by morphineat concentrations known to elicit analgesia. Additional evidencefor opioid action on SP levels in the PAG was reported by Rosenand Brodin (1989). They found that morphine, given systemicallyin doses that are known to produce increasing degrees of analgesia(3 or 10 mg/kg s.c.), dose-dependently elevates the tissue levelof SP in the PAG of rats. The authors explained that one possiblemechanism for the increased tissue level of SP in the PAG aftermorphine is an accumulation of the peptide caused by inhibitionof its release. Our present results support this suggestion inthat opioids inhibited the increased SP release evoked by noxiouscold.

We further investigated the direct effect of SP within the PAG on pain threshold by microdialyzing different doses of SP intothis region. SP, in a dose of 27.1 fmol/µl over a 30-min perfusion(which delivers a total of 65 fmol), induced a slight but nonsignificantincrease in MPA (fig. 5). However, higher doses of SP (271 fmol/µlto 271 pmol/µl) produced a significant increase of MPA in a dose-relatedmanner. The latter result is consistent with the reports fromother laboratories (Stewart et al., 1976; Malick and Goldstein,1978; Mohrland and Gebhart, 1979; Li et al., 1991), which suggeststhat these doses of SP within the brain have analgesic effects.An analgesic effect was also seen in an experiment conducted inmice with i.c.v. injection of 1.25 to 5 ng SP (Frederickson etal., 1978). Malick and Goldstein (1978) reported that the analgesiceffect of SP microinjected into the PAG in rats was five timesas potent as morphine on a weight basis (25 times as potent ona molar basis). Our present results show that SP microdialyzedinto the rat's PAG in a dose of 271 fmol/µl (cumulative dose,650 fmol or 0.9 ng in the PAG, on the basis of the recovery rate)can induce analgesia. The lowest dose of SP (27.1 fmol/µl or 65fmol total) was in the range of the estimated peak extracellularSP level in the PAG evoked by noxious cold (1.3 fmol/120 µl indialysis samples or 65 fmol in the PAG, on the basis of the recoveryrate). The failure of this dose to produce a significant analgesiceffect could be explained in two ways. First, SP evoked by thecold may only present the noxious signal but not affect the painthreshold, so that the analgesic effect of higher doses of SPmay be a pharmacological action. Second, the real amount of SPin the synapses evoked by noxious cold may be higher than thatof estimated extracellular SP, because the latter was calculatedbased on the amount of SP that escaped from the synapses and wascaptured by the probe. Therefore, the lowest dose of SP microdialyzedinto the PAG may not be high enough to mimic the real action ofendogenous SP in the synapses. If this were true, SP in a dose10 times higher than the lowest dose may be close to the physiologicalrange of SP acting in the synapses during noxious cold. Becausethis dose of SP produced analgesia, the SP evoked by noxious coldnot only signals noxious information to the PAG but also appearsto further trigger the antinociceptive function of the PAG.

Reports showed that some types of noxious stimuli can inhibit neuronal and behavioral responses to noxious stimulation byactivation of an opioid-mediated mechanism which involves thePAG network (Watkins and Mayer, 1986; Bodnar, 1986). These resultsled to a suggestion that the endogenous pain-suppression system,which includes the descending modulatory control pathways, canbe activated by stimuli such as stress and pain (Fields and Basbaum,1994). In the present experimental procedure, we attempted tominimize the influence of stress, such as allowing the rat toacclimate to the experimental environment, to move freely duringthe experiment and by administering SP by microdialysis withoutdisturbing the animal and injecting opioids by microinjectionat a slow speed and without animal restraint. Although handlingof the animal during the test might be stressful, we comparedthe post-treatment data with the animal's own pretreatment base-linedata. In this way, any significant difference between the pre-and post-treatment data is more likely caused by the effects oftreatments, i.e., noxious cold stimulation and the drugs. In addition,the result that no significant change in SP release before andafter the 25°C water test (in which the animal handling procedurewas the same as that used in the $-$ 10°C water test) indicates thatthe significant increase of SP release during the $-$ 10°C watertest is evoked by noxious cold itself rather than handling stress.Our present findings that noxious cold evokes SP release in thePAG and that SP given into the PAG induces analgesia provide furtherevidence for the hypothesis (Basbaum and Fields, 1984) that "paininhibits pain," i.e., pain itself is a critical factor that activatesthese pathways. SP-induced analgesia is related to the endogenousopioid system in the brain because it can be blocked by naloxone(Stewart et al., 1976; Malick and Goldstein, 1978; Stewart etal., 1982). Our preliminary data also showed that the selectivemu opioid receptor antagonist CTAP (cyclic d-phe-Cys-Tyr-d-Trp-Arg-Thr-Pen-Thr-NH₂)and the delta opioid receptor antagonist naltrindole can blockor attenuate the analgesic effect of SP administered into thePAG (Xin et al., 1996). Because SP itself does not bind to theopioid receptor (Terenius, 1975), it is generally believed thatit may be affecting opioid receptors indirectly through mediationof the release of endogenous opioid peptides. Malick and Goldstein(1978) suggested that the most likely candidates among the opioidpeptides would be $beta$ -endorphin (because it has been shown to exhibita potent long-lasting analgesic response and a rapid onset) andenkephalins (because antibodies to met-enkephalin also antagonizeSP analgesia). Cell bodies and terminals containing these opioidpeptides exist within the PAG (Watson and Barchas, 1979; Fallonand Leslie, 1986; Mansour et al., 1995). Indeed, we observed anincrease of $beta$ -endorphin release from the PAG after both SP administrationinto this region and noxious cold stimulation, and this increasewas attenuated by pretreatment with a SP receptor antagonist,which indicates involvement of this opioid peptide in SP analgesia(Xin et al., 1994). A possible mechanism for SP within the PAGinteracting with opioid peptides and inducing analgesia has beenproposed by Basbaum and Fields (1984). Their hypothesis is thatSP, released either from local PAG neurons activated by ascendingnociceptive pathways or directly from the terminals of those pathways,acts upon local opioid peptide neurons to cause release of opioidpeptides. They, in turn, activate PAG output neurons by inhibitingan inhibitory interneuron. It should be mentioned that althoughSP evoked by noxious cold could trigger the antinociceptive functionof the PAG, this function was still not strong enough to totallysuppress the tail-flick response of the rat to cold water. Hence,the weak analgesic action of endogenous SP seems to be one ofseveral feedback procedures involved in the response to noxiouscold.

There are reports demonstrating that various SP metabolites can influence nociceptive responses (Larson and Sun, 1994; Stewartet al., 1982). For example, the major metabolite of SP, amino-terminalSP 1-7, is able to inhibit nociceptive behavior (Hall and Stewart,1983; Larson and Sun, 1994) and this effect can be blocked byeither Nal (Stewart et al., 1982) or mu and delta opioid receptorantagonists (Larson and Sun, 1993). On the other hand, the carboxylterminal of SP, SP 7-11, exerts an opposite effect (Hall and Stewart,1983). An in vitro study also shows that N-terminal SP 1-7 playsa role in modifying guanine nucleotide-modulated mu opioid receptorbinding, whereas the C-terminal SP 5-11 is without effect (Kruminset al., 1993). These results suggest that, unlike peripheral effectsof SP, which are mediated by receptors that recognize the C-terminalpart of the SP molecule, certain central actions of SP are mediatedby the receptors which recognize the N-terminal part of the SPmolecule. It is possible that SP may be metabolized to this activefragment before its action at these receptors, which then producethe analgesic effect observed in our present results. However,on the basis of our experimental procedure, we cannot determinewhich fragment of SP is involved.

The result that pretreatment with Nal blocks the analgesic effect of a high dose of SP (fig. 7) is in agreement with earlierfindings from other laboratories (Stewart et al., 1976; Malickand Goldstein, 1978) and provides evidence that exogenous SP inducesanalgesia through the action of the endogenous opioid system.Because opioids generally produce an inhibitory effect on neuronswhereas SP generally produces an excitatory effect, we furtherinvestigated whether endogenous SP itself could act differentlyto induce hyperalgesia when opioid receptors were blocked by Nal.The result showed that, at least in the PAG, endogenous SP evokedby noxious cold or SP microdialyzed into the PAG in a low doseclose to the evoked-SP level did not cause hyperalgesia in Nal-pretreatedrats (fig. 7). Indeed, SP given intrathecally produces hyperalgesia(Lembeck et al., 1981; Akerman et al., 1982; Yasphal et al., 1982;Dirig and Yaksh, 1996) and SP excites those neurons in the spinalcord responsive to noxious stimuli (Henry, 1976). Thus it appearsthat SP may play a role in sensory transmission within the spinalcord and that this role may be related specifically to pain. SPalso produces excitation of neurons in the PAG (Ogawa et al.,1992) when given into this region. However, the functional consequenceof the excitation produced by SP in the PAG and in the spinalcord seems to be different because reports show that excitationof the PAG by SP or by electrical stimulation (Basbaum et al.,1977) induces analgesia, whereas excitation of the spinal cordby SP causes hyperalgesia (Lembeck et al., 1981; Akerman et al.,1982; Yasphal et al., 1982; Dirig and Yaksh, 1996). One explanationfor this difference may be the distinct neuronal networks in thePAG and the spinal cord, because the descending pain control systemoriginates in the PAG and excitation of the PAG output neuronresults in the initiation of the descending control. In addition,as mentioned above, a different distribution of SP receptors,which recognize the N or C terminals of SP distinctively in thePAG and the spinal cord may contribute to the different resultsof SP in the two regions. Therefore, it appears that SP at thePAG level does not cause pain but activates the descending controlsystem through endogenous opioids to regulate pain.

SP release in the POAH did not change significantly during noxious cold stimulation (fig. 3), although SP and its receptorshave been demonstrated in the POAH of rats (Panula et al., 1984;Quirion et al., 1983). Because microdialysis of SP into the POAHdoes not induce analgesia (fig. 6) and there is no change of SPlevel after noxious cold, it indicates that this region is lessimportant than the PAG in the integrity of pain input and antinociception.The POAH is generally believed to be a primary site for centralcontrol of Tb and a region which contains the highest populationof thermosensitive neurons (Boulant et al., 1989). Opioids canaffect these neurons by either increasing or decreasing theirfiring rate to alter the set point and integrate correspondingTb responses (Baldino et al., 1980; Lin et al., 1984). Opioidpeptides and all three opioid receptors exist in the POAH (Watsonand Barchas, 1979; Fallon and Leslie, 1986; Mansour et al., 1995).Previous results from our laboratory have shown that microdialysisof PL017 and Dyn into the POAH, but not the PAG, produce hyperthermiaand hypothermia, respectively (Xin et al., 1993). These resultsconfirm the hypothesis that mu and kappa opioid receptors in thisregion mediate hyperthermic and hypothermic responses to opioids,respectively (Adler et al., 1988). It is not known whether SPwithin the POAH can interact with those opioid receptors. Thepresent results demonstrate that SP microdialyzed into the POAH,in the same doses that induce analgesia in the PAG, does not affectthe Tb of freely moving rats (fig. 8), which suggests that SPin this region is not involved in Tb regulation and does not interactwith opioid receptors. This suggestion is supported by the reportsthat central application of SP in several doses revealed no oronly small and inconsistent changes in Tb of various mammals (Clarkand Lipton, 1991) and that SP reduced the temperature sensitivityof POAH thermosensitive neurons (Schmid et al., 1993).

In summary, our present results demonstrate that SP release within the PAG, but not the POAH, can be increased after noxiouscold stimulation to the rat's tail and that pretreatment withthe mu opioid receptor agonist PL017 and the kappa opioid receptoragonist Dyn in the PAG can prevent the SP increase. These findingssuggest that SP may transmit noxious cold information to thisregion and that activation of both mu and kappa opioid receptorswithin this region may produce analgesia by suppressing noxiousinput from ascending afferents as well as SP increase in the PAG.The results extend our previous finding that noxious cold caninduce SP increase in the spinal cord and i.c.v. injection ofDyn can prevent the SP increase (Tiseo et al., 1990). In addition,SP, microdialyzed into the PAG in amounts 10 times more than thatof extracellular SP evoked by noxious cold, produced dose-relatedanalgesia, which indicates that SP may not only carry noxioussignals to the PAG but also trigger the antinociceptive functionof the descending pain-suppression system. Finally, our resultsalso demonstrate that SP does not affect Tb when it is microdialyzedinto the POAH or PAG.

	Acknowledgments

We thank Dr. Nigel T. Maidment at Department of Psychiatry, UCLA Medical Center for his generous gift of dialysis membrane.

	Footnotes

Accepted for publication April 7, 1997.

Received for publication September 18, 1996.

¹ This work was supported by Grant DA 00376 from the National Institute on Drug Abuse.

Send reprint requests to: Dr. Li Xin, Department of Pharmacology, Temple University School of Medicine, 3420 North Broad Street, Philadelphia, PA 19140.

	Abbreviations

aCSF, artificial cerebrospinal fluid; CNS, central nervous system; CWT, cold water tail-flick test; Dyn, dynorphin A1-17; i.c.v., intracerebroventricular; MPA, maximum possible analgesia; Nal, naloxone; PAG, periaqueductal gray; PL017, Tyr-Pro-N-MePhe-D-Pro-NH₂; POAH, preoptic anterior hypothalamus; RIA, radioimmunoassay; SP, substance P; Tb, body temperature.

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