GR89,696: A Potent kappa -Opioid Agonist with Subtype Selectivity in Rhesus Monkeys

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Vol. 298, Issue 3, 1049-1059, September 2001

GR89,696: A Potent $kappa$ -Opioid Agonist with Subtype Selectivity in Rhesus Monkeys

Eduardo R. Butelman, M. C. Holden Ko, John R. Traynor, Jeffrey A. Vivian¹ , Mary-Jeanne Kreek and James H. Woods

Laboratory on the Biology of Addictive Diseases, The Rockefeller University, New York, New York (E.R.B., M.J.K.); and Departments of Pharmacology (M.C.H.K., J.T., J.A.V., J.H.W.) and Psychology (J.H.W.), University of Michigan, Ann Arbor, Michigan

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion Summary References

GR89,696 is a synthetic $kappa$ -opioid receptor agonist, recently reported to have an agonist profile consistent with selectivityat the proposed " $kappa$ ₂" subtype. The present studies evaluated theeffects of GR89,696 in vitro {i.e., in radioligand binding and[³⁵S]guanosine-5'-O-(3-thio)triphosphate assays} and in vivo in rhesusmonkeys, in assays used to study $kappa$ -opioid agonists (i.e., thermalantinociception, sedation and muscle relaxation, diuresis, andincreases in serum prolactin levels, as well as ethylketocyclazocineand U69,593 discrimination). Furthermore, the sensitivity of GR89,696to naltrexone and nor-binaltorphimine (nor-BNI) antagonism wascompared with that of U50,488 and U69,593, ligands selective forthe proposed " $kappa$ ₁" subtype. Overall, GR89,696 displayed the profileof a highly potent $kappa$ -opioid agonist, following parenteral administrationin rhesus monkeys. GR89,696 was less sensitive than U50,488 andU69,593 to naltrexone or nor-BNI antagonism, consistent with anaction through the proposed $kappa$ ₂ receptorsubtype.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion Summary References

$kappa$ -Opioid agonists may have pharmacotherapeutic potential in the treatment of pain or hyperalgesia and in the management ofpsychostimulant addiction (Caudle et al., 1998; Mello and Negus,1998; Kreek et al., 1999; Schenk et al., 1999). However, the clinicalapplication of selective nonpeptidic $kappa$ -agonists has been limitedby the occurrence of characteristic undesirable effects (e.g.,sedation and dysphoria). In contrast, the peptidic $kappa$ -agonists(i.e., dynorphin peptides, dynorphin A[1-13], and the dynorphinA[1-8] analog E-2078) have not caused sedation or dysphoria inhumans (Ohnishi et al., 1994; King et al., 1999; Kreek et al.,1999).

Apparent subpopulations of $kappa$ -opioid receptors have been detected in central nervous system tissue of rodents, nonhuman primates,and humans, based on radioligand binding studies (Zukin et al.,1988; Kim et al., 1996; Butelman et al., 1998; Caudle et al.,1998). The molecular nature of these apparent $kappa$ -opioid subtypesis still unclear since only a single $kappa$ -receptor clone has beendetected within each species (Raynor et al., 1994). These apparentsubtypes could therefore represent post-translational modificationsof one gene product, or heterogeneous interactions between differentreceptor systems (e.g., formation of receptor dimers; Jordan andDevi, 1999; Simonin et al., 2001). It has also been suggestedthat these apparent subtypes may represent different affinitystates of the same receptor (Richardson et al., 1992). At an appliedlevel, it is important to investigate whether selectivity fora particular $kappa$ -receptor subpopulation confers a characteristicin vivoprofile.

GR89,696 (4-[(3,4-dichlorophenyl)acetyl]-3-(1-pyrrolidinylmethyl)-1-piperazinecarboxylic acid methyl ester fumarate) is asynthetic $kappa$ -opioid agonist, as determined from in vivo and invitro studies in rodents (Hayes et al., 1990). GR89,696 was developedfrom the structure of the prototypical arylacetamide $kappa$ -agonistU50,488 (Szmuszkovicz, 1999). Recent studies have led to the suggestionthat GR89,696 has agonist selectivity for the proposed " $kappa$ ₂" subpopulation(Ho et al., 1997). GR89,696 displayed a distinctive profile whenadministered intrathecally in rats, in that it blocked hyperalgesiawithout affecting nociception. In contrast, a µ- and a $delta$ -agonistblocked both hyperalgesia and nociception, whereas a $kappa$ ₁ ligand(U69,593) blocked neither (Ho et al., 1997).

The in vivo pharmacological characterization of the proposed $kappa$ ₂ subpopulation has been limited by the lack of agonists orantagonists selective for $kappa$ ₂ sites. The aim of the present studieswas to compare the in vivo profile of GR89,696 with that of proposed $kappa$ ₁ ligands in rhesus monkeys (i.e., U50,488 and U69,593). Thediscriminative stimulus effects of GR89,696 were therefore evaluatedin subjects trained to discriminate either ethylketocyclazocine(EKC; a nonselective $kappa$ -opioid) or U69,593 (a $kappa$ ₁-selective opioid)from vehicle. The profile of GR89,696 was also studied in thermalantinociception and respiratory depression and diuresis assays,in sedation and muscle relaxation scales, and in a neuroendocrineassay (release of a pituitary hormone, prolactin). Particularcombinations of the above-mentioned assays are typically responsiveto either $kappa$ - or µ-agonists (Table 3). The effects of GR89,696were also studied after pretreatment with the opioid antagonistsnaltrexone and nor-binaltorphimine (nor-BNI). Both these antagonistsin rhesus monkeys are selective for $kappa$ ₁ sites versus overall $kappa$ -sites(Table 3; Butelman et al., 1993b, 1998; Ko et al., 1998).

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion Summary References

Subjects

Captive-bred, intact rhesus monkeys of either sex (Macaca mulatta; weight range 4.5-11 kg) were singly housed in rooms maintainedat 20-22°C with controlled humidity, and a 12:12-h light/darkcycle (lights on at 7:00 AM). Monkeys used in serum prolactin(six females) and antinociception studies were fed standard primatechow biscuits (Purina, Richmond, VA) daily, supplemented by fruittwo times per week. Monkeys in the drug discrimination experimentswere fed appropriate amounts to maintain body weight at approximately90% of free-feeding levels. Water was freely available in homecages, via an automatic waterspout. Animals used in these studieswere maintained in accordance with the Institutional Animal Careand Use Committees of Rockefeller University and the Universityof Michigan, and Guidelines of the Committee on the Care and Useof Laboratory Animals of the Institute of Laboratory Animal Resources,National Health Council (Department of Health, Education and Welfare,Publication ISBN 0-309-05377-3, revised1996).

Radioligand Binding Studies

Procedure. Rhesus monkey cortical membranes were prepared in Tris-HCl buffer according to the methods of Emmerson et al. (1994). Membranes(400 µg of protein) were incubated in Tris-HCl buffer (50 mM,pH 7.4) with appropriate radioligand in a total volume of 1 mlfor 60 min at 25°C with increasing concentrations of GR89,696.µ-Opioid receptor sites were labeled with [³H]DAMGO (1.06 nM) and $delta$ -opioid receptor sites were labeled with[³H]DPDPE (1.8 nM). $kappa$ -Opioid sites were labeled by [³H]U69,593 (1 nM) or with [³H]bremazocine (1 nM) in the presence of 1 µM DAMGO and 1 µM DPDPEto prevent binding to µ- and $delta$ -opioid receptor sites, respectively.A standard concentration of 1 to 1.8 nM ligand was used for eachassay as the level of ³H-labeled ligand was taken into account in determining K_i valuesof competing ligands. In binding experiments, nonspecific bindingwas defined with naloxone (10 µM). Bound and free ligands wereseparated by vacuum filtration through glass fiber filters andquantified by liquid scintillationcounting.

Data Analysis. IC₅₀ values were determined with GraphPad Prism (version 2.0; GraphPad, San Diego, CA) and converted to K_i values accordingto the Cheng-Prusoff equation. The K_d values for [³H]U69,593 (0.95 nM) and [³H]DAMGO (0.57 nM) are from Emmerson et al. (1994). The K_d valuefor [³H]bremazocine (0.12 nM) in the presence of DAMGO and DPDPE (1µM each; to mask µ- and $delta$ -receptors, respectively) was determinedfrom saturation binding analysis (data notshown).

[³⁵S]GTP $gamma$ S Assay

GR89,696-induced stimulation of [³⁵S]GTP $gamma$ S binding was studied in a C6 cell line expressing the rat µ-receptor and in CHO cellsexpressing the human $kappa$ -receptor, as described previously (Traynorand Nahorski, 1995; Zhu et al., 1997). Briefly, membranes wereincubated for 1 h with [³⁵S]GTP $gamma$ S (100 pM), in the presence of several concentrations ofGR89,696. Control (unstimulated) binding of [³⁵S]GTP $gamma$ S was studied in the absence of GR89,696. Maximal stimulationof [³⁵S]GTP $gamma$ S binding was determined with 10 µM DAMGO (µ-receptors)or 10 µM U69,593 ( $kappa$ -receptors). The effect of GR89,696 in thisassay was expressed as a percentage of the maximal effect of theabove-mentioned reference compounds, which are high-efficacy agonistsin their respective cell lines. To study the antagonism of µ-receptor-mediatedGTP $gamma$ S binding, DAMGO, at an approximately 80% effective concentration(100 nM), was incubated as described above (100 pM GTP $gamma$ S, 1 h)in the presence of increasing concentrations of GR89,696 (0.001nM-100 µM).

Data Analysis. ED₅₀ values for the stimulation of GTP $gamma$ S were determined using nonlinear regression analysis (GraphPad Prism). The AD₅₀ valueof GR89,696 (concentration of antagonist reversing the effectof DAMGO by 50%) was determined using regression analysis (GraphPadPrism), and data were compared using a Student's ttest.

EKC Discrimination

The procedure has been described in detail previously (Butelman et al., 1999d).

Apparatus. All experiments used similar operant panels consisting of two primate response levers (BRS-LVE model PRL-001; Laurel, MD).The levers required a force of 0.25 N over a distance of 2 mmfor a response to be recorded. A panel of 7.5-W stimulus lightswas located above, and a food receptacle located between, thelevers, and both were mounted to one wall of the testing chamber.Delivery of 300-mg banana-flavored pellets (Noyes formula G/T;Lancaster, NH) was controlled by an externally mounted food dispenser(Gerbrands model G5210; Arlington, MA). A PC-compatible computerconnected to a custom-made interface controlled the schedulingof events and recorded data. A lever press was counted as aresponse.

Procedure. Chair-trained monkeys (n = 3) were trained to respond for pellets under a fixed ratio 30 (FR 30) schedule for food reinforcement.Subsequently, discrimination training was undertaken in whichreinforcer delivery was made contingent upon the selection ofthe lever previously paired with a drug stimulus. For all subjects,EKC (0.0056 mg/kg s.c.) was paired with the right, and salinewith the left, lever. Training sessions consisted of two to fivecycles. Each cycle comprised two periods: an initial 10-min time-outperiod in which light stimuli were extinguished and respondinghad no consequence. This was followed by a 5-min response periodin which light stimuli were illuminated, and monkeys could obtainup to 10 pellets (reinforcers) through completion of the FR 30schedule of reinforcement on the drug-appropriate lever. If 10reinforcers were obtained prior to the end of the response period,the stimulus lights were extinguished and responding had no consequences.Monkeys were trained five days/week and were not tested untilgreater than 80% drug-appropriate responding was attained priorto the first reinforcer delivery and across the session; thiscriterion was maintained across four of five consecutive trainingsessions. In addition, no tests were performed unless responserates were maintained within 20% across four of fivesessions.

Test sessions were performed as described above, with a 15-min cycle (10-min time-out, 5-min response period), and reinforcerdelivery was made contingent upon completion of the fixed ratioschedule regardless of the lever selected. For GR89,696, bothsingle (time course) and cumulative dosing procedures were used.During single-dosing procedures, the first response period commenced5 min after drug administration, and discrete 15-min cycles wereperformed thereafter, continuing for 4 h after drug administration.During cumulative dosing procedures, vehicle or drugs were administeredat the beginning of consecutive 15-mincycles.

Data Analysis. For discrimination data, lever selection was expressed as percentage of EKC responding by dividing the number of responseson the EKC lever by the total number of responses. The percentageof control response rates for individual monkeys was calculatedby dividing the response rates for each cycle by the saline controlresponse rates for that session, and are presented graphically.Generalization was considered to occur if a subject emitted atleast 80% of responses on the EKC-appropriatelever.

U69,593 (U69) Discrimination

Apparatus. Two-lever primate operant boxes were custom built by MED Associates (Georgia, VT), and connected with a MED Associates interfaceto a PC computer. Chaired subjects were placed in the boxes; theyhad within easy reach the two levers and a food hopper. A lightwas lit above each of the levers to signal food availability duringsessions, and a house light was also lit during the period offoodavailability.

Procedure. A separate group of three subjects was trained to discriminate s.c. injections of U69,593 from vehicle, in a food-reinforcedFR 20 operant procedure (sessions were carried out 5 days/week).U69,593 training doses were 0.0056 mg/kg for one subject and 0.013mg/kg for the two other subjects. Subjects were trained essentiallyas described above, with some modifications. Each cycle commencedwith a s.c. injection of drug or vehicle and was followed by a15-min time-out, during which responses had no consequence. Thistime-out was followed by a 5-min response period. Ten reinforcerswere available during each response period, and these occurredafter 20 responses on the injection-appropriate lever (FR 20).Before the onset of testing, subjects had to satisfy the followingperformance criteria: five consecutive sessions had to reach atleast 90% injection-appropriate responding, with response ratesabove 1 response/s. After the initial training criteria were met,subjects were tested after a minimum of two consecutive sessionsmeeting the above-mentioned criteria. Test sessions were identicalto that described above, except that 20 responses resulted ina food presentation, irrespective of theinjection.

Design and Data Analysis. Subjects were tested in time course sessions; one injection was therefore followed by response periods starting at differentintervals (e.g., 5, 15, 30, 60 min after injection). A vehiclecontrol experiment was completed in each subject. Different dosesof U69,593 (0.0032, 0.01 mg/kg; 1-2 determinations at each dose)and GR89,696 (0.00001-0.00032 mg/kg; 2-3 determinations at eachdose) were studied for each compound. Mean ± S.E.M. data are presentedfor %U69-appropriate responding and rate of responding (responses/s).Generalization was considered to occur if a subject emitted atleast 90% of responses on the U69-appropriatelever.

Warm Water Tail Withdrawal Assay (Antinociception)

Apparatus and Procedure. The procedure has been described in detail previously (Dykstra et al., 1987a). Monkeys were seated in primate restraint chairs,and the lower portion of the shaved tail (approximately 15 cm)was immersed in a polycarbonate flask containing water at either40, 50, or 55°C. Monkeys were tested at the three water temperaturesin varying order, with tests in the same monkey separated fromeach other by approximately 2 min. Tail withdrawal latencies weretimed on a stopwatch in 0.1-s increments. To prevent tissue damage,tails were removed from the water if they remained immersed for20 s (cutoff latency). Sessions began with control determinationsat each water temperature, presented in a varied order among themonkeys.

Experimental sessions were carried out no more frequently than once per week. The antinociceptive effects of GR89,696 weredetermined using a cumulative dosing procedure with a 1-h interinjectioninterval (testing occurred 50 min after each injection). The testingparameters were based on initial pilot studies on the time courseof the effects of GR89,696.

Antagonist studies of GR89,696 were conducted using three opioid antagonists. First, the antagonist effects of naltrexonewere studied with various pretreatment doses (0.032-0.56 mg/kgs.c.). The antinociceptive effects of GR89,696 were redetermined15 min after pretreatment of a single dose of naltrexone. Second,a single dose (0.1 mg/kg s.c.) of clocinnamox was administered24 h prior to determination of GR89,696-induced antinociception.Clocinnamox is a functionally irreversible µ-opioid receptor antagonist(Zernig et al., 1994

). The present dose of clocinnamox was selectedbased on a previous study, in which clocinnamox produced an approximately1-week-long period of µ-opioid receptor antagonism in rhesus monkeys(Zernig et al., 1994

). Finally, pretreatment with a single doseof nor-BNI (3.2 mg/kg s.c.) was used to compare the " $kappa$ ₁" receptorantagonism between U50,488 and GR89,696. The antinociceptive effectsof U50,488 and GR89,696 were redetermined 1 day and 3 days afternor-BNI pretreatment, respectively. This dose of nor-BNI (3.2mg/kg) produces a long-lasting antagonism of U50,488 in rhesusmonkeys (Butelman et al., 1993b

Data Analysis. Individual data were converted to %maximum possible effect (%MPE) by the following calculation: %MPE = [(test latency $-$ controllatency)/(cutoff latency $-$ control latency)] × 100%. IndividualED₅₀ values were calculated from individual %MPE values by linearregression, and a mean ED₅₀ (±95% confidence limits) were presented.For in vivo apparent pA₂ analysis, dose ratios produced by naltrexonewere analyzed in a Schild plot and individual pA₂ values wereobtained (PHARM/PCS program; Microcomputer Specialists, Philadelphia,PA). The same group of four subjects was used for all the pharmacologicalcomparisons in thisassay.

Respiration

Apparatus and Procedure. The apparatus was similar to that described previously (Howell et al., 1988; Butelman et al., 1993a). Briefly, unanesthetizedmonkeys were seated in restraint chairs enclosed in sound-attenuatingchambers. Gas, either air or a mixture of 5% CO₂ in air (hereafterreferred to as CO₂), was pumped through the helmet and removedat a rate of 8 l/min. Changes in gas flow inside the helmet weremeasured with a pressure transducer connected to a polygraph (model7E; Grass Instrument Co., Quincy, MA). The data were recordedon a polygraph trace and in a microprocessor via an analog todigital converter. Minute volume (V_E) was determined by integrationof changes in flow through the plethysmograph. Frequency (f) wasdirectly determined and tidal volume (V_T) was calculated as V_T= V_E/f.

Experimental sessions contained several consecutive cycles, with each cycle including a 53-min exposure to air followed bya 7-min exposure to 5% CO₂. An experiment was started after measurementof control respiratory values in air and CO₂. The compound wasthen administered (i.m. in the thigh) at the beginning of eachcycle using a cumulative dosing procedure with a 1-h interinjectioninterval. The doses of both GR89,696 and morphine were chosenfrom the same range used in the warm water tail withdrawal procedure.Comparison of both compounds was made in the same monkeys acrossconditions.

In separate experiments (n = 4), the potential µ-antagonist effects of GR89,696 were studied by administering single pretreatmentdoses of GR89,696 (0.000032, 0.00032, and 0.001 mg/kg) 30 minbefore redetermination of the morphine dose-effect curve (0.32-10mg/kg) in thisassay.

Data Analysis. Data from the last 3 min of exposure to air and the second 3 min of exposure to CO₂ in each cycle were used for analysis ofdrug effects on respiratory measures. Values obtained in eachcycle are expressed as percentage of the respective control parameterscollected before drugadministration.

Sedation/Muscle Relaxation Observational Rating

Procedure. Monkeys (n = 5) were rated while in their home cages on two observational rating scales described previously (Butelman etal., 1999b). Rating was carried out by a nonblinded observer,familiar with the individual subjects' baseline behavior. At eachsampling point, subjects were rated initially on a muscle relaxationscale (scores 0-5; based on a subject's spontaneous posture) followedby a sedation scale (scores 0-6; based operationally on the environmentalstimulus that is required to elicit a behavioralresponse).

Design and Data Analysis. Cumulative dose effect curves for GR89,696 (0.000032-0.001 mg/kg) and U69,593 (0.001-0.032 mg/kg) were studied with a 60-mininterinjection interval. Rating occurred before the onset of dosing(preinjection control) and 50 min or 20 min after each injectionfor GR89,696 and U69,593, respectively. A similar design was institutedfor repeated vehicle administration (four consecutive sterilewater injections at 60-min interinjection intervals, with rating50 min after each injection). The same five subjects were usedfor all the observational rating studies. Dose effects curvesfor GR89,696 and U69,593 were analyzed with Friedman's repeatedmeasures ANOVAs ( $alpha$ level was set at the 0.05level).

Diuresis

Procedure. The procedure has been described previously (Butelman et al., 1999d). Urine volumes were collected at hourly intervals over3-h subsequent to the administration of the test drugs (GR89,696,U69,593, and fentanyl). Tests were performed in the home cageof each monkey (n = 3), with a clean cage pan placed under thegrid floor, for urine collection. Water was available via automaticspouts throughout the session. Sessions were carried out twiceperweek.

Data Analysis. Mean urine volumes were analyzed with a one-factor (dose) repeated measures ANOVA. When significant, post hoc Dunnett's comparisonswere performed. In tests involving antagonists, paired t testswere performed. $alpha$ was 0.05, two-tailed.

Serum Prolactin Levels

Procedure. The procedure has been described previously (Butelman et al., 1999c). Chair-trained monkeys were tested after habituationto the experimental situation. Monkeys were chaired and broughtinto the experimental room between 9:30 and 10:00 AM on each testday. An indwelling catheter (24 gauge, Angiocath; Becton Dickinson,Sandy, UT) was placed in a superficial leg vein and secured withtape. An injection port (Terumo, Elkton, MD) was attached to thehub of the catheter; the port and catheter were flushed (0.3 mlof 50 U/ml heparinized saline) before use, and after each bloodsampling. Approximately 15 min following catheter placement, twopreinjection baseline blood samples were collected, 5 min apart(defined as $-$ 10 and $-$ 5 min relative to the onset of dosing). Ateach sampling point, an initial 0.5-ml blood aliquot was obtained;this aliquot was not used in the present assay due to the presenceof the heparin "lock" solution. This was followed by a separate1.5-ml blood aliquot, which was placed in a plain vacutainer,and kept at room temperature until the time of spinning (5 minat 3000 rpm; 4°C) and serum separation. Serum samples were keptat $-$ 40°C until the time ofanalysis.

The samples were analyzed in duplicate with a standard human prolactin radioimmunoassay kit (44 samples/kit; Nichols DiagnosticsInstitute, San Juan Capistrano, CA). Standard calibration curveswere determined for each kit with human prolactin (3-150 ng/ml).The reported cross-reactivity of this assay was of largest magnitudefor human growth hormone (0.07% cross-reactivity).

Monkeys were tested either in a time course or cumulative dosing design. Time course studies were carried out by administeringa single s.c. injection (after baseline sample collection). Bloodsamples were then obtained at intervals (5-120 min) after injection.Cumulative s.c. dose-effect curve studies were carried out witha 60-min interinjection interval, with doses increasing by 0.5log units in each cycle. Sample collection occurred 50 min afterinjection (for GR89,696) and 20 min after each injection (forU69,593). These sampling times were adjusted based on the approximatepeak effect times determined from time course studies for theseagonists.

Design and Data Presentation. Each experiment was carried out in four to five females in the follicular phase (days 2-12 of each cycle of 28 days, as definedby the onset of visible bleeding). Consecutive experiments inthe same subject were separated by at least 48 h (72 h followingnaltrexone administration). Time course studies were determinedfor GR89,696 (0.0001 or 0.00032 mg/kg) and U69,593 (0.032 mg/kg).Based on these time course studies, cumulative dose-effect curveswere designed for GR89,696 (0.000032-0.00032 mg/kg) and U69,593(0.001-0.01 mg/kg). For control purposes, a vehicle experimentwas studied with an identical design to the GR89,696 dose-effectcurve experiment described above. The GR89,696 and U69,593 dose-effectcurves were redetermined after 5-min pretreatment with naltrexone(0.1 or 0.32 mg/kg). Naltrexone apparent pK_B values were calculatedfor GR89,696 and U69,593, from individual dose ratios. ApparentpK_B values were calculated according to a modified formula (Neguset al., 1993): pK_B = $-$ log[B/DR $-$ 1], where B was the dose of naltrexonein moles per kilogram and DR was the dose ratio. The same poolof subjects (n = 4-5/experiment) was used for the pharmacologicalcomparisons in this assay; the 0.05 $alpha$ level was adopted for allthe studies presentedherein.

Chemicals and Drugs. GR89,696 (Sigma/RBI, Natick, MA), naltrexone HCl (National Institute on Drug Abuse, Research Triangle Park, NC), and nor-binaltorphimine(provided by Dr. H. I. Mosberg, Division of Medicinal Chemistry,University of Michigan, Ann Arbor, MI) were dissolved in sterilewater. U50,488 and U69,593 (Pharmacia & Upjohn, Kalamazoo, MI)were dissolved in sterile water with 1 to 2 drops of lactic acid(if necessary). Compounds were injected in volumes of 0.05 to0.1 ml/kg. All doses are expressed as the above-mentioned formsof the compounds. DAMGO and DPDPE were purchased from Sigma (St.Louis, MO). The following radioligands were used: [³H]DAMGO (40.7 Ci/mmol; Amersham Pharmacia Biotech, Arlington Heights,IL), [³H]DPDPE (30 Ci/mmol; PerkinElmer Life Science Products, Boston,MA), [³H]bremazocine (30 Ci/mmol; PerkinElmer Life Science Products),and [³H]U69,593 (47.9 Ci/mmol; PerkinElmer Life Science Products). [³⁵S]GTP $gamma$ S was purchased from PerkinElmer Life ScienceProducts.

	Results

Top Abstract Introduction Materials and Methods Results Discussion Summary References

Radioligand Binding. In the presence of DAMGO and DPDPE masking agents, GR89,696 displaced the specific binding of [³H]U69,593 with a 5-fold lower K_i than for [³H]bremazocine sites [K_i (±S.E.M.): 0.22 ± 0.05 and 1.15 ± 0.47nM, respectively]. GR89,696 also displaced binding of [³H]DAMGO (µ-sites) and [³H]DPDPE ( $delta$ -sites) [K_i (±S.E.M.) were 0.65 ± 0.15 and 30.61 ± 11.8nM, respectively].

[³⁵S]GTP $gamma$ S Assay. GR89,696 was a potent, high-efficacy "full" agonist on cloned $kappa$ -receptors expressed in CHO cells, as measured by its abilityto stimulate [³⁵S]GTP $gamma$ S binding, relative to U69,593 (Table 1). GR89,696 wasapproximately 100-fold less potent at µ-receptors in C6 cells,and also displayed a lower maximal stimulatory effect on [³⁵S]GTP $gamma$ S binding, compared with DAMGO. U69,593 and DAMGO are high-efficacy"full" agonists at cloned $kappa$ - and µ-receptors, respectively, inthis assay (Alt et al., 1998; Remmers et al., 1999).

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TABLE 1
Comparison of the efficacy of GR89,696 measured by stimulation of [³⁵S]GTP $gamma$ S binding

A single concentration of DAMGO (100 nM) caused 77 ± 2.5% stimulation of GTP $gamma$ S binding. This was reduced to a 20.7 ± 2.1%stimulation (p < 0.0001) in a concentration-dependent manner byGR89,696, affording an AD₅₀ for GR89,696 of 212 ± 40 nM. In thepresent experiment, GR89,696 had to compete for µ-receptors withDAMGO; thus, the AD₅₀ value depended on the amount of DAMGO used.Therefore, the GR89,696 AD₅₀ value is not directly comparableto the ED₅₀ value for GR89,696 alone in the presentassay.

EKC Discrimination. Single doses of GR89,696 (0.00001-0.0001 mg/kg s.c.) dose and time dependently increased EKC lever selection (Figs. 1 and2). At the highest dose tested (0.0001 mg/kg), greater than 80%EKC lever selection was observed 30 to 120 min after administration.Similarly, cumulative dosing with GR89,696 dose dependently engenderedEKC responding, with greater than 80% EKC lever selection observedat 0.0001 mg/kg. U69,593 (0.0001-0.0032 mg/kg s.c.), but not fentanyl(0.0001-0.0032 mg/kg s.c.), was generalized in EKC-trained monkeys.

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Fig. 1. Time course of the effects of GR89,696 in monkeys trained to discriminate EKC from vehicle. Abscissae: time (min) from injection. ordinates: percentage of drug-appropriate responding (top), rate of responding (responses/s; bottom).

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Fig. 2. Cumulative dose-effect curves for GR89,696, U69,593, and fentanyl in monkeys trained to discriminate EKC from vehicle. Abscissae: log drug dose (mg/kg). Other details as in Fig. 1 legend.

U69,593 Discrimination. Vehicle administration (s.c. bolus, 0.1 ml/kg) produced less than 5% mean U69-appropriate responding when tested between 5and 60 min after injection (n = 3; one or two determinations).Time course studies with single U69,593 doses (0.0032 and 0.01mg/kg) resulted in dose-dependent generalization (Fig. 3). The0.01 mg/kg U69,593 dose resulted in generalization in all threesubjects 15 min after administration. Vehicle-appropriate respondingwas observed in all three subjects by 120 min after 0.01 mg/kgof U69,593 (Fig. 3). GR89,696 (0.00001-0.0001 mg/kg) also occasioneddose-dependent generalization in all three subjects (Fig. 3).Two of the subjects generalized at the 0.0001-mg/kg dose, between30 and 120 min after administration (Fig. 3). The third subjectdid not generalize at this dose, therefore a larger dose (0.00032mg/kg) was probed in this subject alone (two determinations).In both these determinations, the subject generalized GR89,696(0.00032 mg/kg) to the training drug (at 30 and 60 min).

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Fig. 3. Time course of the effects of vehicle and U69,593 (left) or GR89,696 (right) in monkeys trained to discriminate U69,593. See Fig. 1 legend for other details.

Antinociception. The subjects (n = 4) used in this study had a consistent profile of tail-withdrawal responses. In the absence of drug treatment,they kept their tails in 40°C water for 20 s (cutoff latency)and removed their tails from 50 and 55°C water rapidly (within1-3 s). GR89,696 (0.0001-0.0018 mg/kg) dose dependently producedantinociception against the 50^o and 55°C water stimuli (Fig. 4). ED₅₀ (95% CL) values for eithertemperature were 0.00052 mg/kg (0.00046-0.00058) and 0.0013 mg/kg(0.0012-0.0013), respectively. Pretreatment with naltrexone (0.032-0.56mg/kg) dose dependently produced rightward shifts of the dose-effectcurve of GR89,696-induced antinociception (Fig. 4). The naltrexoneapparent pA₂ value (95% CL) for GR89,696 in 50°C water was 7.0(6.9-7.1), the obtained slope from a Schild plot was $-$ 1.1 (1.3-1.0).The naltrexone apparent pA₂ value (95% CL) for GR89,696 in 55°Cwater was 6.9 (6.7-7.1) and with a Schild slope of $-$ 1.1 (1.4-0.8).

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Fig. 4. Cumulative dose-effect curves for GR89,696 alone and after naltrexone pretreatment in the warm water tail withdrawal assay of thermal antinociception (50°C, top; 55°C bottom). Abscissae: GR89,696 dose (mg/kg). Ordinates: percentage of maximum possible effect. Naltrexone (NTX) pretreatment doses are in milligrams per kilogram.

Pretreatment with the µ-selective antagonist clocinnamox (0.1 mg/kg; 24 h PT did not significantly antagonize GR89,696-inducedthermal antinociception (data not shown). This clocinnamox treatmentis sufficient to cause profound antagonism of µ-receptor mediatedeffects in this assay (Zernig et al., 1994

In separate experiments, 3-day pretreatment with the $kappa$ ₁-selective antagonist nor-BNI (3.2 mg/kg) also did not antagonize theantinociceptive effects of GR89,696 in either 50 or 55°C water(Fig. 5). In a control study, 1-day pretreatment with nor-BNI(3.2 mg/kg) produced 3.3- and 3.6-fold rightward shifts of U50,488-inducedantinociception against 50 and 55°C water, respectively (Fig.5; Butelman et al., 1993b

). Nor-BNI's inactivity against GR89,696was not due to a difference in the time of testing; the presentlyused nor-BNI dose was active against U50,488 for more than 10days after administration (Butelman et al., 1993b

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Fig. 5. Cumulative dose-effect curves for U50,488 (right) and GR89,696 (left) alone and after pretreatment with nor-BNI (3.2 mg/kg) in the warm water tail withdrawal assay of thermal antinociception. See Fig. 5 legend for other details.

Respiration. Untreated monkeys (n = 4) exhibited a consistent pattern of respiration in the head plethysmograph apparatus. A stable baselinerate of respiration was recorded in monkeys breathing air. Themean control values (± S.E.M.) for monkeys breathing air wereas follows: f = 28 ± 3 (frequency; breaths/min), V_T = 102 ± 15(tidal volume; ml/breath), and V_E = 2882 ± 407 (minute volume;ml/min). When 5% CO₂ was introduced, a prompt increase in allrespiratory parameters was observed, with individual monkeys displayingstable patterns of CO₂-induced increases across sessions. Themean control values (± S.E.M.) for monkeys breathing 5% CO₂ inair were as follows: f = 37 ± 3 (breaths/min), V_T = 167 ± 12 (ml/breath),and V_E = 5992 ± 486 (ml/min). Cumulative administration of morphine(1-18 mg/kg) dose dependently produced suppression of f, V_T, andV_E in both air and 5% CO₂. Figure 6 portrays the effects of morphineand GR89,696 in monkeys breathing 5% CO₂ (the profile of theseeffects is the same for monkeys breathing air; data not shown).Following the largest dose administered, morphine suppressed V_Eto 25% ± 3 (S.E.M.) of control levels. In contrast, the largestdose of GR89,696 (0.0018 mg/kg) only suppressed V_E to 69% ± 8(S.E.M.) of control levels. This difference between morphine andGR89,696 at the largest doses was also observed with V_T and fparameters (V_T: morphine (41 ± 3%) versus GR89,696 (81 ± 4%);f: morphine (60 ± 7%) versus GR89,696 (84 ± 7%).

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Fig. 6. Cumulative dose-effect curves for GR89,696 and morphine in the head plethysmograph assay of respiratory function. Abscissae: dose in milligrams per kilogram. Ordinates: percentage of control values for respiratory frequency (f; left), tidal volume (V_T; middle), and minute volume (V_E; right). Presented data were collected while subjects were breathing 5% CO₂ (see text for other details).

Pretreatment with GR89,696 (0.000032, 0.00032, or 0.001 mg/kg; n = 4 each) did not affect the respiratory depressant effectsof morphine (0.32-10 mg/kg) under the present conditions. In thesedeterminations, the morphine baseline ED₅₀ value for CO₂ V_E (themost sensitive parameter) was 2.7 mg/kg (95% CL = 1.0-7.6). Inthe presence of GR89,696, the CO₂ V_E values were 2.9 mg/kg (95%CL = 1.1-7.4; 0.000032-mg/kg GR89,696 PT dose), 2.5 mg/kg (95%CL = 0.7-9.3; 0.00032-mg/kg PT dose), and 1.5 mg/kg (95% CL =1.1-2.2; 0.001-mg/kg PTdose).

Sedation/Muscle Relaxation Rating. Monkeys rated in the absence of pharmacological treatment (preinjection controls; n = 5) displayed no signs of sedation ormuscle relaxation (i.e., scores = 0), as defined in the presentrating scales. Likewise, four consecutive vehicle injections (60-mininterinjection interval, with rating 50 min after each injection)produced scores of 0 for all subjects in the present scales. BothGR89,696 (0.000032-0.001 mg/kg) and U69,593 (0.001-0.032 mg/kg)caused dose-dependent elevations in sedation and muscle relaxationscores (Fig. 7). Up to the largest doses presently tested, bothcompounds produced similar maximal effects on either rating scale.GR89,696 was approximately 30-fold more potent than U69,593, asestimated from the plotted dose-effect curves. Significant Friedman'sANOVAs were obtained for GR89,696's effects on sedation and musclerelaxation (X²_F [5] = 18.23 and 17.27, respectively). Posthoc Dunn's tests revealed that for both scales, the largest GR89,696dose (0.001 mg/kg) produced higher scores than preinjection control.Significant Friedman's ANOVAs were also obtained for U69,593'seffects on sedation and muscle relaxation scales (X²_F [5] = 17.44 and 18.02, respectively). Dunn'stests also revealed that the largest U69,593 dose (0.032 mg/kg)caused a significant increase in sedation and muscle relaxationscores from preinjection control.

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Fig. 7. Cumulative dose-effect curves for GR89,696 and U69,593 on sedation and muscle relaxation scores (top and bottom, respectively), using observational rating scales. Abscissae: dose in milligrams per kilogram. Ordinates: median rating score (n = 5), where 0 is the absence of sedation or muscle relaxation signs.

Diuresis. Saline-injected monkeys produced approximately 30 ml of urine during the 3-h observation period. GR89,696 (0.00001-0.00032mg/kg i.m.) dose dependently increased urine output [F(4,8) =7.14, p = 0.01] (Fig. 8), reaching significance beginning at 0.0001mg/kg. At the highest dose tested (0.00032 mg/kg), urine volumewas increased to approximately 230%. Pretreatment with quadazocine(1 mg/kg) prevented the diuretic effects of GR89,696 [0.00032mg/kg; t(2) = 5.03, p = 0.04], returning urine volumes to vehiclecontrol [t(2) = 1.22, N.S.], while producing no effects on itsown [t(2) = 0.77, N.S.] (Fig. 9).

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Fig. 8. Diuretic effect of GR89,696 and U69,593 (left and right, respectively). Abscissae: drug or control ("C") condition. Ordinates: total urine volume after drug or control injection.

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Fig. 9. Diuretic effects of peak doses of GR89,696 or U69,593 (0.00032 and 0.1 mg/kg, respectively) alone and after pretreatment with quadazocine (1 mg/kg). Data above "Q" represent the diuretic effects of quadazocine alone. See Fig. 9 legend for other details.

The $kappa$ -agonist U69,593 (0.01-0.32 mg/kg i.m.) also increased urine output at all doses tested [F(4,8) = 29.97, p < 0.01]. U69,593(0.1 mg/kg) produced a 283% increase in urine volume (Fig. 8).Pretreatment with quadazocine reversed the diuretic effects ofU69,593 [0.1 mg/kg; t(2) = 6.96, p = 0.02] (Fig. 9). In contrast,the µ-agonist fentanyl (0.001-0.01 mg/kg) dose dependently decreasedurine output [F(3,6) = 4.62, p = 0.05] (data notshown).

Serum Prolactin Levels. Preinjection prolactin levels were typically 3 ng/ml or less in these female subjects. Three consecutive vehicle injections(60-min interinjection intervals, with blood sampling occurring20 min after each injection) did not result in an elevation ofprolactin levels compared with preinjection levels (n = 3; datanot shown). The time course of single GR89,696 (0.0001 and 0.00032mg/kg) and U69,593 (0.032 mg/kg) doses was studied between 5 and120 min after s.c. administration. GR89,696 peak effects on prolactinwere observed 30 to 60 min after administration, whereas U69,593caused a peak increase in prolactin levels 15 to 30 min afteradministration (Fig. 10).

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Fig. 10. Time course of single doses of GR89,696 and U69,593 on serum prolactin levels. Abscissa: time after injection (min); point above BL represents the mean of two preinjection baseline samples. Ordinate: prolactin levels (ng/ml).

Both GR89,696 (0.000032-0.00032 mg/kg) and U69,593 (0.001-0.01 mg/kg) caused dose-dependent increases in prolactin levels,when tested in a cumulative dosing design (Fig. 11). GR89,696 was23-fold more potent than U69,593 in this neuroendocrine end point(Table 2). Naltrexone (0.1-0.32 mg/kg) was administered 5 minbefore the redetermination of GR89,696 and U69,593 dose-effectcurves (Fig. 11). The smaller naltrexone pretreatment dose (0.1mg/kg) did not affect the GR89,696 dose-effect curve, whereasthe larger naltrexone dose (0.32 mg/kg) caused a 2.6-fold rightwardsurmountable shift. In contrast, the smaller naltrexone pretreatmentdose (0.1 mg/kg) caused an 8.6-fold rightward surmountable shiftin the U69,593 dose-effect curve. Naltrexone alone (0.01-0.32mg/kg; studied in a cumulative dose-effect curve) did not causean elevation in serum prolactin levels (n = 4; data not shown).Apparent pK_B analysis (Table 2) confirmed that naltrexone wasa significantly more potent antagonist of U69,593 than of GR89,696in this neuroendocrine end point.

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Fig. 11. Cumulative dose-effect curves for GR89,696 and U69,593 (top and bottom, respectively) alone and after pretreatment with naltrexone (NTX). Abscissae: dose (mg/kg). Ordinate: prolactin levels (ng/ml). Naltrexone pretreatment dose is expressed in milligram per kilogram.

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TABLE 2
Effects of GR89,696 and U69,593 on serum prolactin levels

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion Summary References

GR89,696 produced agonist effects in assays used to characterize $kappa$ -opioids in rhesus monkeys, consistent with its high affinityfor $kappa$ -opioid receptors in monkey brain, and its high efficacyat cloned $kappa$ -receptors. As indicated by a potency comparison withseveral benzomorphan or arylacetamide compounds, GR89,696 is oneof the most potent $kappa$ -agonists to be characterized in vivo in rhesusmonkeys to date (Dykstra et al., 1987a; France et al., 1994; Butelmanet al., 1999a).

Radioligand Binding and Stimulation of [³⁵S]GTP $gamma$ S Binding. GR89,696 displayed low nanomolar affinity for $kappa$ -opioid sites in monkey brain. GR89,696 had approximately 5-fold selectivityfor $kappa$ -sites sites labeled by [³H]U69,593 over $kappa$ -sites labeled by [³H]bremazocine (in the presence of masking agents for µ- and $delta$ -opioidsites). This is consistent with studies in rodents, suggestingthat GR89,696 does not possess a high degree of binding selectivityfor either of the proposed $kappa$ -subtypes. Based on ex vivo studiesin rats, it has been suggested that GR89,696 is an antagonistat the $kappa$ ₁ receptor subtype, whereas it is an agonist at the $kappa$ ₂receptor subtype (Caudle et al., 1997). GR89,696 had moderateaffinity for sites labeled by [³H]DAMGO (µ-receptors) and lower affinity for sites labeled by[³H]DPDPE ( $delta$ -receptors) in monkeybrain.

GR89,696 was a potent high efficacy "full" agonist in CHO cells transfected with $kappa$ -opioid receptors, as measured by the stimulationof [³⁵S]GTP $gamma$ S binding. However, GR89,696 had approximately 100-foldlower agonist potency on µ-receptors, and was a low efficacy (i.e.,partial) agonist in this µ-receptor preparation. This was confirmedby the ability of GR89,696 to antagonize the effect of the highefficacy µ-agonist DAMGO in thispreparation.

The above-mentioned in vitro findings are consistent with the profile of GR89,696 as a potent high-efficacy $kappa$ -agonist in vivo.The finding that GR89,696 is a high-efficacy $kappa$ -agonist (similarlyto the $kappa$ ₁ ligand U69,593) suggests that this in vitro preparationmay not parallel the characteristics that generate differentialpharmacological effects for proposed $kappa$ ₁ and $kappa$ ₂ agonists, as encounteredin vivo or ex vivo (Zukin et al., 1988

; Caudle et al., 1997

; Schoffelmeeret al., 1997

). A similar situation has been encountered previouslywith regard to the in vitro versus in vivo effects of several $kappa$ -opioids (France et al., 1994

; Remmers et al., 1999

). The lowefficacy (or antagonist effects) of GR89,696 at µ-receptors couldbe detected in vitro in the GTP $gamma$ S assay, but not in vivo in anassay of respiratory depression (seebelow).

EKC and U69,593 Discrimination. GR89,696 (0.000032-0.0001 mg/kg) was generalized by all monkeys trained to discriminate EKC from vehicle. EKC is not a selectiveligand with respect to $kappa$ - versus µ-opioid sites, or with respectto $kappa$ ₁ versus all $kappa$ -receptors (Zukin et al., 1988; Emmerson etal., 1994; Butelman et al., 1998). However, rhesus monkeys trainedto discriminate EKC from vehicle generalize to $kappa$ - but not µ-agonists(Dykstra et al., 1987b; France et al., 1994). Therefore, generalizationobserved in EKC-trained monkeys with GR89,696 indicates that thiscompound shares the discriminative stimulus effects of $kappa$ -opioidagonists (see Carey and Bergman, 2001).

U69,593 is considered a prototypical " $kappa$ ₁"-selective ligand (Zukin et al., 1988

). In the present studies, GR89,696 was generalizedby all subjects trained to discriminate U69,593 from vehicle.Under the present conditions, GR89,696 exhibited a relativelyslow onset, and was approximately 30 to 100 times more potentthan U69,593. Therefore GR89,696, a proposed " $kappa$ ₂" agonist, sharesdiscriminative stimulus effects (interoceptive effects) with U69,593,a ligand selective for the $kappa$ ₁site.

Thermal Antinociception. GR89,696 dose dependently elevated tail withdrawal latencies in 50 and 55°C water. The antinociceptive effect of GR89,696was insensitive to pretreatment with clocinnamox (0.1 mg/kg; 24h PT). This indicates that the effects of GR89,696 were not mediatedby µ-opioid receptors in this assay (Zernig et al., 1994). Theeffects of GR89,696 in this assay were dose dependently antagonizedby naltrexone. The potency of naltrexone (as determined with apparentpA₂ values) was similar to that previously reported for non- $kappa$ ₁-selectiveagonists (such as bremazocine), and is lower than for agonistsselective for the $kappa$ ₁ site (e.g., U50,488 and U69,593; Ko et al.,1998) (Table 3). Consistent with this conclusion, the antinociceptiveeffects of GR89,696 were also insensitive to pretreatment withnor-BNI (3.2 mg/kg). This pretreatment dose of nor-BNI is sufficientto antagonize the antinociceptive effects of selective $kappa$ ₁ ligandssuch as U50,488 and U69,593, but not those of bremazocine (presentstudy; Butelman et al., 1993b; Table 3). Overall, the presentantagonism experiments are consistent with the notion that GR89,696produces its antinociceptive effects under these conditions atleast partially through $kappa$ ₂ receptors.

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TABLE 3
Comparison of the pharmacological profile of GR89,696, U69,593, bremazocine, and fentanyl in vivo in rhesus monkeys
N.D., not determined. Data are from the present studies and the references indicated in footnotes.

Respiratory Depression. Up to the largest dose studied presently, GR89,696 only caused moderate respiratory depression. The largest GR89,696 dosestudied in the respiratory depression assay was fully effectivein the assay of thermal antinociception, and produced prominentbehavioral (e.g., sedative) effects in the present studies. Thelimited respiratory depressant effects of GR89,696 are similarto those previously reported for selective $kappa$ -agonists in rhesusmonkeys (e.g., U69,593 or U50,488; Howell et al., 1988; Franceet al., 1994). By comparison, doses of the µ-agonist morphine,which produce antinociceptive effects (Zernig et al., 1994), causedmore profound respiratory depression in the present studies. Thus,at antinociceptive doses, GR89,696 has only a limited capacityto cause respiratorydepression.

Given the low-efficacy/antagonist actions of GR89,696 at µ-receptors in the GTP $gamma$ S assay (see above), the potential µ-antagonisteffects of GR89,696 were studied in this in vivo assay. A broadrange of GR89,696 PT doses (up to doses that produced robust $kappa$ -receptor-mediatedeffects) did not significantly affect the respiratory depressanteffects of morphine under the present conditions. Larger GR89,696doses were not assessed to avoid possible untowardeffects.

Sedation and Muscle Relaxation. GR89,696 produced sedative and muscle relaxant effects qualitatively similar to those U69,593 in the same group of rhesusmonkeys. GR89,696 was approximately 30-fold more potent than U69,593on both these behavioral end points. Therefore, GR89,696 sharedthe overt behavioral effects caused by an agonist selective forthe $kappa$ ₁ site, U69,593.

Diuresis. GR89,696 produced dose-dependent diuresis in rhesus monkeys, similarly to previously reported studies with $kappa$ -opioid ligands(Dykstra et al., 1987a). The diuretic effect of GR89,696 was ofsimilar magnitude to that of U69,593, although GR89,696 was approximately100-fold more potent than U69,593. The diuretic effects of bothGR89,696 and U69,593 were sensitive to pretreatment with the opioidantagonist quadazocine. Quadazocine has been used previously toantagonize the diuretic effects of structurally diverse $kappa$ -opioidsin rhesus monkeys (Dykstra et al., 1987a; Butelman et al., 1999d).The ability of GR89,696 to cause diuresis in rhesus monkeys isconsistent with previous studies in human and nonhuman primates,since both $kappa$ ₁-selective and non- $kappa$ ₁-selective agonists producediuresis (Tang and Collins, 1985; Dykstra et al., 1987a; Rimoyet al., 1991; Butelman et al., 1999d).

Serum Prolactin Levels. In common with synthetic or peptidic $kappa$ -agonists, as well as µ-agonists, GR89,696 produced a dose-dependent increase in prolactinlevels in intact, follicular phase, female rhesus monkeys (Butelmanet al., 1999c). GR89,696 displayed a slower onset than U69,593in this assay, and was 23-fold more potent than U69,593 in dose-effectcurve determinations. Naltrexone has higher affinity for bindingsites labeled by U69,593 (a $kappa$ ₁-selective ligand) than by bremazocine(a nonselective $kappa$ -ligand) in rhesus monkey brain (Ko et al., 1998).It has been suggested that the agonist effects of GR89,696 aremediated by $kappa$ ₂ sites (Ho et al., 1997). Consistent with this suggestion,the prolactin-releasing effects of GR89,696 were less sensitiveto naltrexone antagonism than those of U69,593, in the presentstudies. These neuroendocrine findings are, to our knowledge,the first to show an in vivo differentiation of a proposed $kappa$ ₁versus $kappa$ ₂ effect in a non-behavioral endpoint.

The prolactin-releasing effects of opioid agonists are thought to be mediated by a decrease in tone in the dopaminergic hypothalamicsystems (Moore and Lookingland, 1995

). The potency and durationof action of GR89,696 in releasing prolactin therefore suggestthat this $kappa$ -agonist could produce a long-lasting decrease in hypothalamicdopaminergic tone in vivo, following systemic administration inprimates (Butelman and Kreek, 2001

	Summary

Top Abstract Introduction Materials and Methods Results Discussion Summary References

GR89,696 was a high-efficacy and high-potency agonist at $kappa$ -opioid receptors, but only a low-efficacy agonist at µ-opioid receptors,in the GTP $gamma$ S assay in vitro. In rhesus monkeys in vivo, GR89,696had the profile of a potent and long-lasting $kappa$ -agonist, in thatit produced thermal antinociception, sedation and $kappa$ -agonist-likediscriminative stimulus effects, as well as prolactin release.Naltrexone and nor-BNI antagonism studies in antinociceptive andneuroendocrine assays are consistent with mediation of these effectsof GR89,696 by non- $kappa$ ₁ (i.e., possibly $kappa$ ₂) receptors. Overall,the present studies demonstrate that GR89,696 shares the in vivoeffects of a $kappa$ ₁ ligand (U69,593; see Table 3 for a summary comparison).However, pretreatment studies with naltrexone and nor-BNI suggestthat the effects of GR89,696 may be mediated by a subset of $kappa$ -opioidreceptors with a distinct profile of antagonistsensitivity.

	Acknowledgments

We thank Todd Harris for excellent technicalhelp.

	Footnotes

Accepted for publication May 22, 2001.

Received for publication January 5, 2001.

¹ Current Address: Department of Pharmacological and Physiological Sciences, Bowman-Gray School of Medicine, Winston-Salem,NC27157.

This study was supported by U.S. Public Health Service Grants DA 01113 (to E.R.B.), DA 05130 (to M.J.K.), DA 00049 (to M.J.K.),and DA 00254 (to J.H.W.).

Address correspondence to: Dr. E. R. Butelman, The Rockefeller University (Box 171), 1230 York Ave., New York, NY 10021. E-mail: butelme{at}mail.rockefeller.edu

	Abbreviations

EKC, ethylketocyclazocine; nor-BNI, nor-binaltorphimine; DAMGO, D-Ala²,N-Me-Phe⁴,Gly⁵-ol]-enkephalin; DPDPE, [D-Pen²-D-Pen⁵]-enkephalin; GTP $gamma$ S, guanosine-5'-O-(3-thio)triphosphate; CHO, Chinese hamster ovary; AD₅₀, concentration of antagonist reversing the effect of DAMGO by 50%; FR, fixed ratio; U69, U69,593 [(+)-(5 $alpha$ ,7 $alpha$ ,8 $beta$ )-N-methyl-N-[7-(1-pyrrolidinyl)-1-oxaspiro[4,5]dec-8-yl]-benzeneacetamide]; %MPE, percent maximum possible effect; ANOVA, analysis of variance; CL, confidence limit; U50,488, trans-(+/ $-$ )-3,4-dichloro-N-methyl-N-[2-(1-pyrrolidinyl)-cyclohexyl]-benzeneacetamide; PT, pretreatment.

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