Body Temperature and Analgesic Effects of Selective Mu and Kappa Opioid Receptor Agonists Microdialyzed into Rat Brain

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Vol. 281, Issue 1, 499-507, 1997

Body Temperature and Analgesic Effects of Selective Mu and Kappa Opioid Receptor Agonists Microdialyzed into Rat Brain¹

Li Xin, Ellen B. Geller and Martin W. Adler

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

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Opioids administered by i.c.v. injection produce body temperature (T_b) changes and analgesic responses in rats. The presentstudy was undertaken to investigate the effects on T_b and analgesiaof highly selective mu and kappa opioid receptor agonists andantagonists delivered directly into the preoptic anterior hypothalamus(POAH) and periaqueductal gray (PAG) by the intracerebral microdialysismethod. Microdialyzed into the POAH, the mu receptor agonist Tyr-Pro-N-MePhe-D-Pro-NH₂induced dose-related hyperthermia that could be prevented or antagonizedby the mu receptor antagonist cyclic D-Phe-Cys-Tyr-D-Trp-Arg-Thr-Pen-Thr-NH₂or by naloxone, but not by the kappa receptor antagonist nor-binaltorphimine.The kappa receptor agonist dynorphin A_1-17, microdialyzedinto the POAH, induced dose-related hypothermia that was preventedor antagonized by nor-binaltorphimine but not cyclic D-Phe-Cys-Tyr-D-Trp-Arg-Thr-Pen-Thr-NH₂.Neither Tyr-Pro-N-MePhe-D-Pro-NH₂ nor dynorphin A_1-17 microdialyzedinto the PAG produced significant changes in T_b. However, theseagonists microdialyzed into the PAG produced analgesic responsesthat did not occur after administration into the POAH. These resultssupport the hypothesis that the hyperthermic response to opioidsis mediated by the mu receptor and the hypothermic response ismediated by the kappa receptor in rats. The POAH is a primaryfunctional area in T_b, but not in analgesic, responses to opioids,whereas the PAG is a sensitive area for analgesic, but not forT_b, responses to opioids.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Opioid drugs and opioid peptides alter T_b (Lotti et al., 1966, Clark and Lipton, 1985). The direction and magnitude of T_bresponses caused by opioids vary widely under different test conditions.Although the detailed mechanisms of these variations are stillnot known completely, there is little doubt that opioid receptorsare involved in thermoregulation (Geller et al., 1983; Adler etal., 1988; Burks, 1991; Adler and Geller, 1993).

Highly selective agonists and antagonists can be used to distinguish the specific action on T_b mediated through one type ofopioid receptor from the others in the brain. Previous resultsfrom this and other laboratories demonstrated that i.c.v. administrationof selective mu receptor agonists produced hyperthermia (Adlerand Geller, 1993; Spencer et al., 1988; Handler et al., 1992)that could be blocked or antagonized by selective mu receptorantagonists, whereas kappa receptor agonists produced hypothermia(Spencer et al., 1988; Adler et al., 1983; Adler et al., 1986)that could be blocked or antagonized by selective kappa receptorantagonists (Cavicchini et al., 1988; Handler et al., 1992). Onthe basis of findings such as these, we hypothesized that thehyperthermic response to opioids is mediated by the mu receptorand the hypothermic response is mediated by the kappa receptor(Geller et al., 1982; Geller et al., 1986; Adler et al., 1988).However, it was not known whether the same effects would occurwhen those agonists or antagonists were administered directlyinto the POAH, a vital region in T_b regulation, rather than bythe i.c.v. route, which allows the drugs to diffuse rapidly throughoutthe brain.

The POAH is generally considered to be the primary site for central control of T_b, because a large population of thermosensitiveneurons is located there (Boulant, 1980) and because its destructionor inactivation disrupts thermoregulation. It receives and integratesthe T_b information from both central and peripheral sensors andsends the modulating signal to direct T_b-regulatory effectorsfor maintaining T_b around a given temperature, the set point.It has been suggested that the POAH is the site of action of opioidsthat are given centrally and have effects on T_b (Lotti et al.,1966; Tseng et al., 1980; Stanton et al., 1985). At least threetypes of opioid receptors, mu, kappa and delta, have been discoveredso far within the POAH (Mansour et al., 1987), and opioids alterthe activities of the thermosensitive neurons within this region(Baldino et al., 1980; Lin et al., 1984).

The PAG is known to be one of the most important regions involved in pain modulation (Basbaum and Fields, 1984). It has alsobeen reported to be involved in opioid-induced T_b responses (Tsenget al., 1980). Previous results from this laboratory have demonstratedthe analgesic effects of selective opioid receptor agonists, giveni.c.v., using the cold-water tail-flick test (Pizziketti et al.,1985; Tiseo et al., 1988; Adams et al., 1993), but it was notknown whether these agonists, microdialyzed into the PAG, wouldalso affect T_b.

The intracerebral microdialysis method provides a new approach either to delivery of drugs into, or to extracellular collectionof neurochemicals from, a selected brain area (Ungerstedt, 1991).Microdialysis of a substance obviates contact between fluid andtissue and therefore minimizes the local irritation inherent inmost other intracerebral injection procedures. Thus the methodmay mimic closely the release of a substance under physiologicalconditions (Westerink and Justice, 1991). Furthermore, drug deliveryby microdialysis can be conducted in conscious, freely movinganimals without handling the animal, thus avoiding physical restraintand stress that can affect T_b and analgesic responses.

In the present study, we investigated the effects of the activation of mu and kappa opioid receptors on both T_b and analgesiaby using highly selective mu and kappa opioid receptor agonistsand antagonists microdialyzed directly into the POAH or the PAGof rats. All drugs were administered to freely moving animalsto avoid effects of anesthesia or restraint on T_b and analgesia.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Animals

Male Sprague-Dawley rats (Zivic-Miller, Pittsburgh, PA) weighing 250 to 300 g were used in this study. They were housed 3to 4 per cage for at least 1 week before experimental use andwere fed laboratory chow and tap water ad libitum. The temperatureof the animal room was 22 ± 2°C, and a 12-hr light/12-hr darkcycle was used.

Microdialysis Probes

The microdialysis probes used in this study were constructed as follows: Cellulose fibers (Spectrum Medical Industries, LosAngeles, CA; M W cutoff 6 KDa and I.D. = 150 µm) were used asmicrodialysis tubing for the perfusion probe. The probes consistedof two parallel, soldered stainless steel, 25-gauge cannulas witha U-shaped loop of microdialysis tubing 2 mm in effective lengthat their tips. The two parts were joined by epoxy. A fine (0.075-mm)tungsten wire (World Precision Instruments, Inc. Sarasota, FL)was preincorporated into the loop to provide the necessary stiffnessand to prevent the open ends of the loop from closing. The remainingtwo open ends of the cannulas were connected to PE-20 tubing asinput and output cannulas, respectively (fig. 1A).

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Fig. 1. A) Schematic drawing of a microdialysis probe used in these experiments. B) Coronal section of the rat brain, showing thelocation of the microdialysis probe (shaded region: dialysis membrane).

Surgery and Probe Implantation

Eight days before the experiment, each rat was anesthetized with an i.p. injection of a mixture of ketamine hydrochloride(100-150 mg/kg) and acepromazine maleate (0.2 mg/kg), and a 20-mm,17-gauge stainless steel guide cannula with an indwelling styletwas stereotaxically implanted unilaterally into the POAH (AP:7.8, R: 1.0, V: $-$ 1) or PAG (AP: 0.6, R: 0.8, V:1) (Pellegrinoand Cushman, 1967). The guide cannula was fixed with dental cementand self-tapping bone screws. After surgery, the animals werehoused individually to prevent them from destroying the cannulas.One week later, the animals were anesthetized again with ketamine,and the stylet was replaced by a microdialysis probe such thatits dialysis membrane tip protruded exactly 1 mm beyond the guide.It, too, was fixed to the skull with dental cement. The open endsof the probe were protected by two short pieces of PE-20 tubingthat were sealed on their top ends. In order to avoid the influenceon T_b of acute injury produced by insertion of the probe, theanimals were allowed to recover for another 24 hr before the experimentswere begun.

Drugs

The following drugs were tested: the mu receptor agonist PL017; the mu receptor antagonist CTAP; the kappa receptor agonistDyn (Multiple Peptide Systems, San Diego, CA), the kappa receptorantagonist nor-BNI (Research Biochemicals International, Natick,MA) and the general opioid antagonist, naloxone (National Instituteon Drug Abuse, Rockville, MD). Drug doses were chosen on the basisof prior i.c.v. experiments in which a dose-response curve wasobtained. In most cases, aCSF (composition in mM: NaCl, 125; KCl,2.5; NaHCO₃, 27; NaH₂PO₄, 0.5; Na₂HPO₄, 1.2; CaCl₂, 1.2; MgCl₂,1; ascorbic acid, 0.1; glucose, 5; pH 7.4) was the vehicle andcontrol solution. For purposes of comparison, sterile pyrogen-freeisotonic 0.9% saline was also used as a vehicle or control insome cases.

Experimental Protocols

Evaluation of the dialysis probe. Both in vitro and in vivo studies were conducted to assess the efficiency of the dialysis probes in delivering the opioidreceptor agonists and antagonists. During the in vitro studies,probes were tested by perfusing the agonists or antagonists throughthem at a rate of 1 µl/min while their tips were immersed in microtubescontaining 60 µl saline at 37°C. The 10-µl samples were takenfrom the microtubes after 15, 30, 60, 120 and 180 min of perfusion.During the first 60-min period, 5-µl samples were also taken fromthe outflow collections. The concentration of the drugs in eachsample and in perfusion vehicles was measured by HPLC. We calculatedwhat percentage of the drug concentration in the dialysis perfusatewas represented by the percentage (Y) of the drug concentrationin the bathing medium by dividing the concentration per microliterof the medium solution (C_m) by that of the input solution (C_i):

Y=Cm<IT>/C</IT>i<IT>×100</IT>

To determine the amount of drug that may have been lost (or that stuck to the membrane or tubing) during the 60-min perfusionperiod, we calculated the difference (A_lost) between drug amountin the input solution and that in the output solution as follows:

Alost<IT>=</IT>[<IT>C</IT>i<IT>−</IT>(<IT>C</IT>o<IT>+C</IT>m)]<IT>×60 &mgr;</IT>l

where C_o is the output concentration. During in vivo studies, the drugs were perfused through the probes in situ in the POAH.The effluents were collected over intervals of 0 to 0.5, 0.5 to1, 1 to 2 and 2 to 3 hr during perfusions. The rates (Z) of drugsperfused into the dialysis system were estimated by the concentrationdifferences between the output and input solutions:

Z=[1−(Co<IT>/C</IT>i)]<IT>fC</IT>i

where C_i and C_o are the average input and output concentrations of the corresponding collecting intervals, respectively,and f is the flow rate of the perfusion, 1 µl/min; C_o/C_i was estimatedby dividing the drug concentration of the output solution by thatof the input solution. The amount (A) of drug actually deliveredinto the brain during the first 60-min perfusion period was estimatedas follows:

A=[(Z30×30 min) + (<IT>Z</IT>60 ×30 min)]−<IT>A</IT>lost

Microdialysis experiments. Experiments were performed between 8:30 A.M. and 4:00 P.M. On the test day, the rats were placed into individual plastic cagesin an environmental room kept at 21°C ± 0.3°C and 52% ± 2% relativehumidity. At the beginning of the experiment, the sealed tubingon both input and output cannulas of the microdialysis probeswas removed, and the input cannulas were connected by PE-20 tubingto a single-channel swivel (series 375, Instech Laboratories,Inc., Plymouth Meeting, PA) that was then connected to a 1-mltuberculin syringe (Becton Dickinson & Co., Rutherford, NJ) clampedto a perfusion pump (Harvard Apparatus, Inc., South Natick, MA).T_b measurements were made according to standard procedures inour laboratory. After a 1-hr acclimation period, a thermistorprobe (YSI series 400, Yellow Springs Instrument Co., Inc., YellowSprings, OH) was lubricated and inserted approximately 7 cm intothe rectum; T_b measurements were read from a digital thermometer(Model 49 TA, YSI). During the readings, the rat's tail was heldgently between two fingers, and the animal was otherwise freeto move about. The first three measurements were taken at 30-minintervals. To allow for adaptation to the procedure, the firstreading was discarded, and the next two were averaged to establisha base line. In this way, each animal served as its own control.Experimental values were then compared to the predrug base-linevalues obtained for each animal. Immediately after the third measurement,the drug of interest was perfused through the microdialysis probeat the rate of 1 µl/min over a 1-hr period or, in some cases,a 3-hr period. As soon as drug perfusion was ended, sterile pyrogen-freesaline was substituted for the drug and perfused at a rate of8 µl/min for 1 min, or, in some cases, a second drug was perfusedimmediately after the first drug perfusion ended.

Analgesia testing. The cold-water tail-flick test was used to assess the analgesic effects of opioid receptor agonists according to standardprocedures in our laboratory (Pizziketti et al., 1985). A 1:1mix of ethylene glycol/water was maintained at $-$ 3°C with a circulatingwater bath (Model 9500, Fisher Scientific, Pittsburgh, PA). Animalswere held firmly over the opening of the bath, and their tailswere submerged approximately halfway into the solution. The nociceptivethreshold was taken as the latency until the rat removed or flickedits tail. Three predrug latencies were measured: 60, 30 and 0min before drug perfusion. For each animal, the first readingwas discarded to minimize variability, and the remaining two wereaveraged to determine the base-line latency. After 60 min of drugperfusion, latency to tail-flick was tested at 15, 30, 60 and120 min. If an animal did not respond within 60 sec, the trialwas terminated, and a maximum latency of 60 sec was recorded.The analgesic effect of drug treatment was calculated for eachrat as follows:

%MPA<IT>=</IT>[(postdrug latency<IT>−</IT>base-line latency)/

(60<IT>−</IT>base-line latency)]<IT>×</IT>100.

HPLC procedures. The samples taken from both in vitro and in vivo probe evaluation tests were analyzed by reverse-phase HPLC (Model 1050, HewlettPackard, Co., San Fernando, CA). The analysis was performed atroom temperature with a C₄ column (5 µm, 4.6 × 25 mm, Vydac),a 1050 quarternary pump, a 1050 dual-wavelength detector and twointegrators (all from Hewlett Packard). The mobile phase consistsof two solutions: 0.1% trifluroacetic acid in water and 0.1% trifluroaceticacid in 80% acetonitrile. A linear gradient of acetonitrile (0%-50%)at 1 ml/min is used, followed by isocratic elution with acetonitrile(50%). Drug standards or samples were dissolved in a small volumeof 0.1% trifluroacetic acid, filtered through a 0.22-µm filter(Milipore) and injected onto a C₄ column.

Verification of dialysis probe placement. At the conclusion of the experiments, animals were placed into a bucket containing dry ice within a metal mesh basket forat least 10 min. The animals were almost instantaneously anesthetizedby the carbon dioxide, rapidly asphyxiated and cooled. Their brainswere excised and coronally cut, and the visible track of the microdialysisprobe was checked. In some cases, bromophenol blue (0.2%) wasmicrodialyzed into the POAH for 3 hr or into the PAG for 1 hr,and the brain was removed and frozen. A block of tissue containingthe track of the probe and the stain of the dialyzed dye was cutand checked (fig. 2). Data from rats in which the probes werenot located within the POAH or PAG (approximately 10%) were notincluded in the results.

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Fig. 2. Photographs of coronal sections of rat's brain showing spread of bromophenol blue after 1 hr (panel A) or 3 hr (panel B) ofdialysis into the POAH and after 1 hr of dialysis into the PAG(C). Arrows point to edge of dye stain. Horizontal bar = 1 mmin length. ac: anterior commissure; aq: aqueductus; oc: opticchiasm; pag: periaqueductal gray; poah: preoptic anterior hypothalamus.

Statistical Analysis

The results are reported as T_b changes ( $Delta$ T, means ± S.E.) from base line and % MPA (means ± S.E.). These changes were analyzedfor each agonist or agonist/antagonist combination using a one-wayanalysis of variance with a repeated-measure variable of time,followed by a post-hoc Fisher's test. Treatment differences ateach time-point were compared with aCSF controls by using themodified t statistic, in which the significance level is reducedby the Bonferroni procedure (Wallerstein et al., 1980). The 5%level of probability was accepted as statistically significant.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

The range of drug diffusion within the POAH and PAG. The range of drug diffusion within the brain regions is estimated by the stain of the bromophenol blue dialyzed into the POAH(1-hr and 3-hr perfusion) and the PAG (1-hr perfusion). The resultsare illustrated in figure 2. After a 1-hr perfusion, the dye diffusedaround the probe tip and created a spherical stain 1.2 mm in diameterwithin the POAH (fig. 2A) and the PAG (fig. 2C). The spread ofthe dye increased to 1.6 mm in diameter after a 3-hr perfusioninto the POAH, but it still did not extend outside of the POAH(fig. 2B).

The efficiency of the dialysis probes in delivering drugs. The amounts of PL017, Dyn, naloxone, CTAP and nor-BNI that crossed the dialysis membrane and diffused into the medium in vitroare shown in figure 3. There was some absorption of Dyn and CTAPby the dialysis probe or perfusion/collection tubings, because18% and 14% of the input amount for these two drugs, respectively,was lost during the 60-min perfusion (table 1). In vivo, PL017diffused into the dialysis system at a rate of 0.14 ± 0.006 nmol/minduring the first 30-min perfusion period and slowed to a rateof 0.12 ± 0.004 nmol/min during the 120 to 180-min perfusion period(fig. 4, top). Dyn diffused into the system at a rate of 0.074± 0.013 nmol/min during the first 30-min perfusion period andat a rate of 0.065 ± 0.018 nmol/min during the 120 to 180-minperfusion period (fig. 4, top). The diffusion rates of CTAP, nor-BNIand naloxone into the dialysis system are shown in the bottompanel of figure 4. On the basis of the percentage of drug lostas observed in in vitro tests, the amounts of drugs that passedthrough the dialysis membrane and were actually delivered to thebrain during in vivo tests are estimated as shown in table 1.

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Fig. 3. Time course of the diffusion of drugs across the dialysis membrane to surrounding medium in vitro. Y: ratio (expressed aspercentage) of concentration of drug in medium to that in dialysistube.

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TABLE 1
Estimation of the amount of drugs (nmol) perfused into the dialysis system and the amount that actually passed into the brainduring 60 min of in vivo perfusion (n = 6)

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Fig. 4. Top panel) Rates of PL017 (1.69 nmol/µl) and Dyn (0.35 nmol/µl) diffusion into brain tissue in vivo during time intervals0 to 30, 30 to 60, 60 to 120 and 120 to 180 min of dialysis. Bottompanel) Rates of CTAP (0.9 nmol/µl), nor-BNI (1.2 nmol/µl) andnaloxone (1.3 nmol/µl) diffusion into brain tissue in vivo duringtime intervals 0 to 15, 15 to 30 and 30 to 60 min of dialysis.

T_b responses to the mu receptor agonist PL017 microdialyzed into the POAH. A 3-hr perfusion of vehicle (saline or aCSF) into the POAH produced no change in T_b (fig. 5, top). However, 3 hr of perfusionof PL017 induced a dose-related hyperthermia (fig. 5, bottom).The maximum T_b changes, which occurred about 180 min after theperfusions began, were 1.1 ± 0.13°C, 1.72 ± 0.12°C and 2.0 ± 0.18°Cfor doses of 0.32 nmol/µl, 1.69 nmol/µl and 3.38 nmol/µl, respectively.The recovery time course in which T_b returned to base line was180 min for the lowest dose (0.32 nmol/µl), whereas for higherdoses, average changes in T_b ( $Delta$ T) remained at 45% and 65% of themaximum hyperthermic response, respectively, 180 min after theend of the perfusions. A 1-hr perfusion of PL017 in a dose of1.69 nmol/µl produced a 1.7 ± 0.15°C maximum T_b change at 60 minafter the perfusions began, and the recovery time course was 180min (fig. 6, top). A 1-hr perfusion of PL017 (1.69 nmol/µl) followedby a 1-hr perfusion of saline or CSF induced similar T_b changesand recovery time courses (fig. 6, top).

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Fig. 5. Top panel) T_b changes ( $Delta$ T) of rats in response to a 3-hr intraPOAH microdialysis of pyrogen-free saline or CSF. Base-lineT_b values were 37.6 ± 0.16°C in saline group and 37.9 ± 0.1°Cin aCSF group. Bottom panel) Dose-related T_b changes ( $Delta$ T) inducedby the selective mu opioid receptor agonist PL017 microdialyzedfor 3 hr into the POAH of rats. Base-line T_b values were 37.8± 0.2°C in the 0.32 nmol/µl group, 37.9 ± 0.15°C in the 1.69 nmol/µlgroup and 37.8 ± 0.18°C in the 3.38 nmol/µl group.

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Fig. 6. Top panel) T_b changes ( $Delta$ T) of rats in response to a 1-hr intraPOAH microdialysis of PL017 (1.69 nmol/µl) alone or a 1-hr perfusionof the same dose of PL017 followed by a 1-hr vehicle (aCSF) orsaline perfusion. Base-line T_b values were 37.8 ± 0.18°C in thePL017 alone group, 37.6 ± 0.16°C in the PL017 + saline group and37.8 ± 0.15°C in the PL017 + aCSF group. Bottom panel) T_b responses( $Delta$ T) of rats to a 1-hr intraPOAH microdialysis of antagonistsalone. Base-line T_b values were 37.9 ± 0.14°C in the CTAP group,37.8 ± 0.2°C in the nor-BNI group and 37.9 ± 0.17°C in the naloxonegroup.

T_b responses to reversal or blockade of PL017 with mu or kappa receptor antagonists microdialyzed into the POAH. Perfusion for 1 hr of the mu receptor antagonist CTAP (0.9 nmol/µl), the kappa receptor antagonist nor-BNI (1.2 nmol/µl) orthe general opioid receptor antagonist naloxone (1.3 nmol/µl)did not affect T_b (fig. 6, bottom). However, a 1-hr perfusionof CTAP or naloxone after a 1-hr perfusion of PL017 (1.69 nmol/µl)significantly shortened the recovery time courses to 60 min or90 min, respectively (fig. 7, top), compared with 180 min in thevehicle perfusion after the same dose of PL017 (fig. 6, top).Nor-BNI did not change the recovery time course of PL017 (fig.7, top). Microdialysis of CTAP or naloxone 1 hr before PL017 perfusionprevented the hyperthermic response caused by PL017, whereas a1-hr perfusion of nor-BNI did not block the hyperthermia but delayedthe maximum response to 90 min after the onset of PL017 infusion(fig. 7, bottom).

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Fig. 7. Top panel) T_b changes ( $Delta$ T) of rats in response to a 1-hr intraPOAH microdialysis of PL017 (1.69 nmol/µl) followed by a 1-hrperfusion of the mu receptor antagonist CTAP, the kappa receptorantagonist nor-BNI or the general opioid receptor antagonist naloxone.Base-line T_b values were 37.9 ± 0.14°C in the PL017 + CTAP group,37.8 ± 0.2°C in the PL017 + nor-BNI group and 37.8 ± 0.17°C inthe PL017 + naloxone group. * P < .05. Bottom panel) T_b changes( $Delta$ T) of rats in response to a 1-hr intraPOAH microdialysis ofCTAP, nor-BNI or naloxone, followed by a 1-hr perfusion of PL017.Base-line T_b values were 37.7 ± 0.2°C in the CTAP group, 37.8± 0.17°C in the nor-BNI group and 37.8 ± 0.16°C in the naloxonegroup. * P < .05.

T_b responses to the kappa receptor agonist Dyn microdialyzed into the POAH. Perfusion of Dyn for 3 hr produced a dose-related hypothermia (fig. 8). The maximum T_b changes were $-$ 0.71 ± 0.18°C, $-$ 1.28± 0.08°C and $-$ 1.48 ± 0.09°C for doses of 0.07 nmol/µl, 0.35 nmol/µland 1.05 nmol/µl, respectively, and they occurred 180 min afterperfusions began. The recovery time courses in the responses tothe three different doses were 180 min, 210 min and 240 min afterthe end of the perfusions, respectively. A 1-hr perfusion of Dyn(0.35 nmol/µl) followed by a 1-hr perfusion of saline or aCSFstill induced hypothermia, with a maximum T_b change of $-$ 0.99 ±0.07°C and a recovery time course of 210 min (fig. 9, top).

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Fig. 8. Dose-related T_b changes ( $Delta$ T) of rats in response to a 3-hr intraPOAH microdialysis of Dyn in different doses. Base-line T_bvalues were 37.8 ± 0.18°C in the 0.07 nmol/µl group, 38 ± 0.2°Cin the 0.35 nmol/µl group and 37.9 ± 0.16°C in the 1.05 nmol/µlgroup.

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Fig. 9. Top panel) T_b changes ( $Delta$ T) of rats in response to a 1-hr intraPOAH microdialysis of Dyn (0.35 nmol/µl) followed by a 1-hrperfusion of vehicle (saline or aCSF), CTAP or nor-BNI. Base-lineT_b values were 37.9 ± 0.17°C in the Dyn + saline group, 37.8 ±0.2°C in the Dyn + aCSF group, 37.9 ± 0.16°C in the Dyn + CTAPgroup and 38 ± 0.17°C in the Dyn + nor-BNI group. Bottom panel)T_b changes ( $Delta$ T) of rats in response to a 1-hr intraPOAH microdialysisof CTAP or nor-BNI followed by a 1-hr perfusion of Dyn. Base-lineT_b values were 38 ± 0.16°C in CTAP + Dyn group and 37.9 ± 0.2°Cin nor-BNI + Dyn group. * P < .05.

T_b responses to Dyn before and after CTAP or nor-BNI microdialyzed into the POAH. A 1-hr microdialysis of nor-BNI into the POAH after a 1-hr microdialysis of Dyn shortened the recovery time course to 90 min,compared with 210 min in the case of vehicle perfusion after Dyn,but a 1-hr dialysis of CTAP did not shorten the recovery time(fig. 9, top). A 1-hr perfusion of nor-BNI before Dyn preventedhypothermia; however, the hypothermia still occurred with Dynafter 1-hr perfusion of CTAP (fig. 9, bottom).

T_b responses to PL017 or Dyn microdialyzed into the PAG. Compared with the vehicle control (fig. 10, top), a 1-hr microdialysis of Dyn into PAG, in the same doses that induced hypothermiain the POAH, did not produce a significant change in T_b (fig.10, bottom). After a 1-hr perfusion of PL017, in the same dosethat caused hyperthermia in the POAH, only one dose (2.5 nmol/µl)produced a slight increase (0.5°C ± 0.13°C), which was not significant(fig. 10, bottom).

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Fig. 10. Top panel) T_b responses of rats to a 1-hr intraPAG microdialysis of vehicle (aCSF). Base-line T_b value was 38.1 ± 0.15°C.Bottom panel) T_b responses ( $Delta$ T) of rats to a 1-hr intraPAG microdialysisof PL017 or Dyn. Base-line T_b values were 37.9 ± 0.18°C in thePL017 1.69 nmol/µl group, 38 ± 0.2°C in the PL017 2.5 nmol/µlgroup, 37.8 ± 0.2°C in the Dyn 0.35 nmol/µl group and 38 ± 0.16°Cin the Dyn 1.05 nmol/µl group.

Analgesic responses to PL017 or Dyn microdialyzed into the PAG. A 1-hr microdialysis of PL017 in doses of 1.69 nmol/µl and 2.5 nmol/µl into the PAG produced 47% and 59% of maximum analgesia,respectively, on the cold-water tail-flick test, with 30% and40% of MPA, respectively, still remaining 90 min after the endof PL017 perfusion (fig. 11, top). A 1-hr perfusion of Dyn in dosesof 0.35 nmol/µl, 0.74 nmol/µl and 1.87 nmol/µl into PAG induced30%, 39% and 51% of maximum analgesia, respectively, with 15%,24% and 30% of MPA observed 90 min after the end of the perfusion(fig. 11, top).

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Fig. 11. Top panel) Time course of analgesic responses of rats after a 1-hr microdialysis of aCSF, PL017 or Dyn into the PAG. The pointsabove that caused by the Dyn 0.35 nmol/µl group at 120 min weresignificant, compared with the points of aCSF group at the correspondingtime (P < .05). %MPA: percent maximum possible analgesia. Bottompanel) Time course of analgesic responses of rats after a 1-hrmicrodialysis of aCSF, PL017 or Dyn into the POAH. No points ofthe PL017 and Dyn groups were significant, compared with the pointsof aCSF group at the corresponding time (P > .05).

Analgesic responses to PL017 or Dyn microdialyzed into the POAH. When either PL017 or Dyn, in the same doses that induced T_b changes in POAH (1.69 nmol/µl and 0.74 nmol/µl, respectively),was microdialyzed into POAH, neither of them produced significantanalgesic responses in the cold-water tail-flick test. Higherdoses of PL017 (2.5 nmol/µl) and Dyn (1.87 nmol/µl) caused maximumresponses of only 20% ± 4% and 14% ± 3% of MPA, respectively,which were not significant (P > .05) compared with those in aCSFcontrols (10% ± 3% MPA) (fig. 11, bottom).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Intracerebral microdialysis, the method used in the present study, is a way to discriminate the sites in the brain where opioidsact. The drugs microdialyzed into the PAG and POAH are limitedwithin the desired brain regions even after a 3-hr perfusion (fig.2). Therefore, the T_b and analgesic effects can be consideredthe result of drugs acting directly within these regions ratherthan by diffusion to other brain areas. This method minimizesstress to the animals during drug administration. Although animalhandling during testing may be considered a stressor, there areno significant changes in T_b or tail-flick latency from the firstto the last of the measurements, as shown by the data from theaCSF control groups. Because substances pass the microdialysisprobe membrane by diffusion, and there is no direct contact betweenthe liquid flowing inside the membrane and the cells of the tissue,the acute tissue injury is less than that seen with the microinjectionmethod, where the injector is inserted immediately before drugdelivery. Also, the addition of extra volume and pressure seenwith other methods of drug delivery is avoided. In the presentstudy, after the probe was inserted into the POAH or PAG, 24 hrelapsed before the experiment was begun. This interval is important,because hyperthermia caused by an extensive mechanical lesionof the POAH fully subsides 18 hr after the lesion (Rudy et al.,1977; Rudy, 1980), and local tissue perturbations that occur immediatelyafter implantation of a probe abate in 24 hr (Benveniste et al.,1987), whereas gliosis becomes maximal in 4 days (Hamberger etal., 1983). Another advantage in using intracerebral microdialysisto deliver drugs is that it is possible to maintain sterilityduring drug delivery because the membrane excludes large molecules,such as bacterial lipopolysaccharides, from diffusing into thebrain, thereby preventing bacteria from getting to the deliverysite. A disadvantage in using microdialysis to deliver high-molecular-weightpeptide drugs is that they may be absorbed in the dialysis membraneor perfusion/collection tubing instead of diffusing into the targettissue, as seen with Dyn and CTAP dialyzed into the brain in thepresent study. However, the amount of drug delivered into thebrain was still effective, because it produced T_b or analgesicresponses similar to those obtained by i.c.v. drug administrationin our laboratory (Adams et al., 1993; Handler et al., 1992; Tiseoet al., 1988).

Previous results from this and other laboratories demonstrated that mu receptor agonists caused hyperthermia (Spencer et al.,1988; Handler et al., 1992; Adler and Geller, 1993) and kappareceptor agonists produced hypothermia in rats (Adler et al.,1983; Adler et al., 1986; Spencer et al., 1988; Handler et al.,1992) after i.c.v. administration, which indicates that the thermicactions of opioids occurred in the brain. In the present study,microdialysis was used as the method of administration to facilitatedrug delivery to the POAH and to restrict the administered drugto the relevant thermoregulatory site and minimize ancillary actionsat other sites not directly involved in regulation of T_b. TheT_b responses produced by the opioid agonists and antagonists microdialyzedinto the POAH are similar to those seen in the experiments usingi.c.v. administration, which demonstrates that the POAH is thecrucial locus. It is not possible to determine from this study,however, whether the full effects of drugs on heat loss and heatgain are mediated solely by the receptors in the POAH.

No previous reports appear to have involved the use of highly selective opioid receptor agonists or antagonists delivereddirectly into the POAH. Although some showed the T_b responsesby intraPOAH microinjections of morphine (Lotti et al., 1966;Cox et al., 1976; Trzcinka et al., 1977), $beta$ -endorphin (Martinand Bacino, 1979; Tseng et al., 1980; Thornhill and Saunders,1984), the leu-enkephalin analog DADL-enkephalin (Tepperman andHirst, 1983) and the met-enkephalin analog met-enkephalinamide(Stanton et al., 1985), these drugs are not highly selective forone type of receptor. For example, although morphine is a mu-preferringopioid receptor agonist, in vitro binding (Magnan et al., 1982)and functional (Takemori and Portoghese, 1987) assays have shownthat it has low affinity for delta and kappa opioid receptors,and therefore, high concentrations of morphine can activate allopioid receptors. In terms of T_b effects, a low dose of morphineacts at mu receptors and induces hyperthermia, whereas a highdose of morphine produces hypothermia (Lotti et al., 1966) thatis mediated by kappa receptors (Adler et al., 1988). $beta$ -endorphinhas almost the same affinity for both mu and delta receptors (Leslie,1987), and both enkephalins can act on mu and delta receptors(Akil et al., 1984). In the present study, highly selective opioidreceptor ligands, such as PL017 and CTAP for the mu receptor (Changet al., 1983; Pelton et al., 1986) and Dyn and nor-BNI for thekappa receptor (Chavkin and Goldstein, 1981; Takemori et al.,1988), were employed to distinguish among the actions of differentopioid receptors within the POAH and PAG. That highly selectiveopioid agonists produce opposite T_b changes that can be inhibitedonly by their corresponding antagonists proves the hypothesisthat mu and kappa opioid receptors mediate the hyper- and hypothermiceffect of opioids, respectively, and that the actions of thoseagonists given i.c.v. in our previous experiments occur mainlywithin the brain, rather than outside the brain as a result ofdiffusion of the drugs across the blood-brain barrier. That PL017or Dyn microdialyzed into the POAH, but not into the PAG, inducedopposite T_b changes adds to the evidence that the POAH is a primarysite of opioid action on T_b and that the opioid system is involvedin thermoregulation.

The neuronal characteristics of the POAH may be the basis for its important role in T_b response to opioids. The POAH containsopioid receptors (Mansour et al., 1987) and the largest populationof thermosensitive neurons among brain areas (Boulant et al.,1989). The cold-sensitive neurons (mediating heat-gain responses)and the warm-sensitive neurons (mediating heat dissipation) withinthe POAH can respond to morphine by either increasing or decreasingtheir firing rate (Baldino et al., 1980; Lin et al., 1984). Accordingto some models, the changes in firing rate alter the set pointand initiate corresponding T_b responses. There is a hypothesisthat two populations of thermosensitive neurons exist in the POAH,one involved in opioid-induced hyperthermia and another in hypothermia(Adler et al., 1988). Previous reports from this laboratory indicatedthat opioid agonists could indeed alter the set point by changingthe rate of metabolic heat production and by adjustments in heatexchange (Zwil et al., 1988; Lynch et al., 1987; Handler et al.,1992). These experiments, conducted by calorimetric methods, showedthat PL017 given by i.c.v. administration caused an immediateincrease in metabolic heat production (oxygen consumption), resultingin increased T_b. Dyn induced hypothermia through reduction inmetabolic rate.

In a result consistent with our earlier experiments using i.c.v. administration (Tiseo et al., 1988; Tiseo et al., 1990; Adamset al., 1993), both PL017 and Dyn, microdialyzed into PAG, hadanalgesic effects in this study, which shows that mu and kappareceptors mediated the cold-water tail-flick response to opioidsin this brain area. The PAG was the first region to be implicatedin endogenous pain suppression (Reynolds, 1969) and is also believedto be a main target for morphine or other opioids to enhance descendingsupraspinally mediated inhibition (Basbaum and Fields, 1984).There are mu and kappa receptors within this area (Mansour etal., 1987). Both enkephalin- and dynorphin-positive cells andterminals are found in the PAG (Basbaum et al., 1983). The factthat microinjection of opiates into the PAG induces analgesiaand inhibits the firing of the neurons within the nociceptivemodulatory network, such as the dorsal horn of spinal cord androstral ventromedial medulla (Gray and Dostrovsky, 1983; Jensenand Yaksh, 1986; Fang et al., 1989; Morgan et al., 1992), supportsthe hypothesis that opioids activate PAG output neurons by inhibitingan inhibitory interneuron (Basbaum and Fields, 1984).

The same doses of opioids administered into the PAG failed to induce significant analgesia when microdialyzed into the POAH.This result differs from a previous report (Tseng et al., 1980)in which microinjection of $beta$ -endorphin into both POAH and PAGproduced analgesic and T_b responses. It is possible that the differencebetween these findings is due to the different methods and opioidsused, because $beta$ -endorphin has almost equal affinity for mu anddelta receptors (Leslie, 1987). Central administration of deltareceptor agonists by i.c.v. (Adler and Geller 1993; Handler etal. 1992) or microdialysis into the PAG and POAH (Xin et al. 1994)does not induce any significant changes in T_b or in the metabolicparameters, which indicates that the delta receptor is not involvedin the T_b responses to opioids under normal ambient conditions.The delta receptor agonist DPDPE, however, can produce analgesiain the cold-water test (Adams et al., 1993).

In summary, this study has demonstrated that selective mu and kappa receptor agonists, microdialyzed into the POAH of rats,produced hyperthermia and hypothermia, respectively, and thatthe effects could be blocked by their corresponding antagonistsgiven before the agonist and could be reversed if the antagonistwas administered after the agonist. This is the first report ofthe anatomical specificity of the effects on T_b and analgesiaof selective opioid receptor agonists or antagonists administeredinto the POAH or PAG by the intracerebral microdialysis method.It supports the hypothesis that the hyperthermic response to opioidsis mediated by the mu receptor and the hypothermic response bythe kappa receptor in rats. Our results also demonstrate thatthe POAH is a primary functional area in T_b responses to opioidsand that the PAG is a sensitive area in analgesic responses toopioids. The intracerebral microdialysis method appears to bea valuable tool for investigating the effects of drugs and theinteractions between drugs and endogenous chemicals in the brain.

	Acknowledgments

We thank Dr. Lee-Yuan Liu-Chen and Mr. Chongguang Chen for their assistance with the HPLC measurements, Dr. Jill U. Adamsand Mr. Tom Piliero for assistance in the cold-water tail-flickmethod and Dr. Cynthia M. Handler for assistance with the statisticaltreatment of the data.

	Footnotes

Accepted for publication December 5, 1996.

Received for publication September 19, 1995.

¹ This work was supported by grant DA 00376 from NIDA. Preliminary reports of these results were presented at the 22nd AnnualMeeting of the Society for Neuroscience (Anaheim, California,October 1992), the International Symposium on Microdialysis andAllied Analytical Techniques (Indianapolis, Indiana, May 1993)and the 54th Annual Scientific Meeting of the College on Problemsof Drug Dependence (Toronto, Canada, June 1993).

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; CTAP, cyclic D-Phe-Cys-Tyr-D-Trp-Arg-Thr-Pen-Thr-NH₂; Dyn, dynorphin A_1-17; MPA, maximum possible analgesia; nor-BNI, nor-binaltorphimine; PAG, periaqueductal gray; PL017, Tyr-Pro-N-MePhe-D-Pro-NH₂; POAH, preoptic anterior hypothalamus; T_b, body temperature.

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