(S)-(-)-HA-966, a gamma -Hydroxybutyrate-Like Agent, Prevents Enhanced Mesocorticolimbic Dopamine Metabolism and Behavioral Correlates of Restraint Stress, Conditioned Fear and Cocaine Sensitization

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Vol. 283, Issue 2, 712-721, 1997

(S)-( $-$ )-HA-966, a $gamma$ -Hydroxybutyrate-Like Agent, Prevents Enhanced Mesocorticolimbic Dopamine Metabolism and Behavioral Correlates of Restraint Stress, Conditioned Fear and Cocaine Sensitization¹

Bret A. Morrow, Edward J. K. Lee, Jane R. Taylor, John D. Elsworth, Heather E. Nye and Robert H. Roth

Laboratory of Neuropsychopharmacology, Departments of Pharmacology (E.J.K.L., R.H.R.) and Psychiatry (B.A.M., J.R.T., J.D.E., H.E.N., R.H.R.), Yale University School of Medicine, New Haven, Connecticut 06520-8066

	Abstract

Top Abstract Introduction Methods Results Discussion References

This report investigates the effect of the negative enantiomer of 1-hydroxy-3-aminopyrrolidone-2 (HA-966) on behavioral andbiochemical changes elicited by pharmacological or experimentalparadigms which activate mesocorticolimbic dopaminergic neurotransmission.Several paradigms were used, including cocaine sensitization andtwo stressors: restraint for 30 min and an aversive conditioningmodel. (S)-( $-$ )-HA-966 (3 and 5 mg/kg i.p.) prevented restraintstress-induced dopamine utilization in both the medial prefrontalcortex and nucleus accumbens, in contrast to the positive enantiomer.Conditioned fear increased dopamine metabolism in both the coreand shell subdivisions of the nucleus accumbens, an effect blockedby (S)-( $-$ )-HA-966. The conditioned stress-induced increase indopamine metabolism in the medial prefrontal cortex was also blockedby (S)-( $-$ )-HA-966. In addition, (S)-( $-$ )-HA-966 suppressed fear-inducedbehaviors: immobility and defecation. In other studies, (S)-( $-$ )-HA-966(3 mg/kg i.p.) prevented locomotor sensitization without alteringthe acute motoric response elicited by cocaine. The highest doseof (S)-( $-$ )-HA-966 (5 mg/kg i.p.) blocked acute cocaine-inducedlocomotion but resulted in sedation. In addition, the highestdose of (S)-( $-$ )-HA-966 tested suppressed weight gain in controlrats, unlike its enantiomer, (R)-(+)-HA-966. Because (S)-( $-$ )-HA-966has been proposed to act at the $gamma$ -aminobutyric acid (GABA)_B receptor,we examined the ability of (S)-( $-$ ) and (R)-(+)-HA-966 to displace[³H]-( $-$ )-baclofen from cortical membranes to assess GABA_B receptorbinding. Neither enantiomer significantly altered [³H]-( $-$ )-baclofen binding at relevant concentrations, indicatingthe actions of (S)-( $-$ )-HA-966 reported here are the results ofa mechanism apparently independent of the baclofen binding siteon the GABA_B receptor.

	Introduction

Top Abstract Introduction Methods Results Discussion References

The pharmacological, physiological and behavioral properties of (±)-HA-966 have been widely documented in the past. As a heterocyclicimido five-member ring, (±)-HA-966 appears to be structurallysimilar to a cyclic form of GABA. Bonta et al. (1971) observedthat racemic HA-966 had sedative qualities that mimicked the behavioralproperties of $gamma$ HB. Furthermore, it was found that after the administrationof (±)-HA-966, DA levels were increased in the striatum of therat brain (Bonta et al., 1971) and the spontaneous firing rateof substantia nigra dopaminergic neurons was reduced in a dose-dependentfashion (Nowycky and Roth, 1977; Shepard and Lehmann, 1992), actionssimilar to those noted with $gamma$ HB (Roth et al., 1977). In contrastto these findings, Davies and Watkins (1972) discovered that (±)-HA-966was an excitatory amino acid antagonist, later discovered to actthrough the glycine modulatory site of the NMDA receptor (Fosterand Kemp, 1989).

Only after the enantiomers of (±)-HA-966 were resolved, however, was it possible to attribute the unique characteristics ofthe racemic compound to its components. Radioligand binding andelectrophysiological studies demonstrated that the antagonisticeffects of (±)-HA-966 on the glycine/NMDA receptor mainly residedin the (R)-(+) enantiomer, whereas behavioral studies indicatedthat the sedative/ataxic properties of (±)-HA-966 were primarilydue to the (S)-( $-$ ) enantiomer. The effects of the racemic compoundon nigrostriatal DA neurons seem to reside with the (S)-( $-$ ) enantiomer,including increased striatal DA levels (Singh et al., 1990) andinhibition of nigrostriatal DA neuron firing (Shepard and Lehmann,1992). The simultaneous blockade in spontaneous firing with diminishedrelease and continued synthesis of DA in striatal dopaminergicneurons has been used to explain the increases in striatal DAlevels attributed to ( $-$ )-HA-966 (Singh et al., 1990).

Increased striatal DA levels, as well as the sedative behavioral properties, were noted to mirror those seen with $gamma$ HB and $gamma$ -butyrolactone (Roth et al., 1977), both of which are structurallysimilar to (±)-HA-966 (Bonta et al., 1971; Singh et al., 1990).It was postulated that ( $-$ )-HA-966 exerted its effects throughthe GABA_B receptor based on the resemblance of HA-966 to the cyclicform of GABA and because $gamma$ HB has been proposed to elicit its actionsthrough the GABA_B receptor (Engberg and Nissbrandt, 1993). Insupport of this, the GABA_B antagonist CGP 35348 was found to attenuatethe increase in DA synthesis by $gamma$ -butyrolactone, HA-966 and theGABA_B agonist ( $-$ )-baclofen (Waldmeier, 1991). The binding siteby which $gamma$ HB affects GABA_B receptors is not clear, although ahighly specific membrane $gamma$ HB binding site, without affinity forGABA or GABAergic agonists, has been identified (Benavisea etal., 1982; Maitre et al., 1983). These data suggest that (S)-( $-$ )-HA-966may act by affecting GABA_B-ergic neurotransmission.

Shepard et al. (1995) proposed that both enantiomers of HA-966 may normalize DA firing pattern through a common mechanismrelated to GABA_B. Both enantiomers are able to dose-dependentlyinhibit nigral DA neuronal firing, and in each case, this inhibitioncan be reversed by a GABA_B antagonist, CGP-35348. However, (R)-(+)-HA-966was found to be ~10-fold less potent than the negative enantiomer.In addition, both enantiomers, at different doses, display a normalizationof firing pattern of midbrain DA neurons, resulting in an increasein the regularity of cell firing without changing the overallfiring rate in chloral hydrate anesthetized rats (Shepard et al.,1995). Again, a 10-fold difference in potency was noted betweenthe enantiomers. The normalization of firing pattern was not mimickedby the administration of a competitive NMDA receptor antagonist,NPC-12626, indicating that this effect is probably not due toblockade of the NMDA receptor complex (McMillen et al., 1992).Previously, we proposed that the normalization in firing patternseen by Shepard et al. may be the mechanism by which (R)-(+)-HA-966prevents stress-induced changes in DA metabolism without disruptingbasal DA turnover (Morrow et al., 1993). In addition, it seemedfeasible that this hypothesis could be extended to explain theability of (R)-(+)-HA-966 to prevent cocaine-induced locomotorsensitization (Morrow et al., 1995a, 1995b). If the normalizationof DA neuron firing is necessary for these actions, the negativeenantiomer of HA may provide efficacy in these models but at lowerdoses.

	Methods

Top Abstract Introduction Methods Results Discussion References

Restraint stress protocol. Male Sprague-Dawley rats initially weighing ~250 g were used in these experiments. For restraint stress experiments, ratswere injected with saline or (S)-( $-$ )-HA-966 (1, 3 or 5 mg/kg i.p.;Research Biochemicals, Natick, MA), returned to the home cagefor 20 min, moved to a separate room and placed into a wire restraintapparatus for 30 min. The apparatus restrained without immobilizingthe rat. In addition, special care was taken to avoid pinchingor crushing the animal during the restraint period. Control ratsremained in the home cages in a separate room. At the end of theexperiment, rats were rapidly decapitated, the brains were removedand the following regions dissected as previously described: mPFC,NAS and striatum (Horger et al., 1995).

Fear conditioning. Aversive conditioning was performed in test cages as previously described (Morrow et al., 1995b). The test cages were Plexiglasand stainless steel (24 × 30 × 27 cm) with a grid floor wiredfor footshock. To minimize external interference, the test cageswere located within a sound-attenuated chamber illuminated bya red light. A white noise generator provided a constant backgroundnoise, and the cages were cleaned and dried before each sessionwith 70% ethanol to minimize olfactory cues. A PC controlled the2.8-kHz tone along with triggering the shock generators (BRS/LVE)that delivered the foot shock. This tone did not startle naiverats.² The intensity of the foot shock was calibrated to 0.4 mA (Morrowet al., 1995b).

Habituation, aversive conditioning and test sessions were given on 3 consecutive days. On day 1, the habituation day, ratswere placed into the test cages and left for 30 min. No tonesor foot shocks were given on day 1. On day 2, the aversive conditioningday, rats were treated with (S)-( $-$ )-HA-966, 5 mg/kg or saline;returned to the home cage for 20 min and then placed into thetest cages and given 10 tones with or without a paired footshockover 30 min. The intervals between tones were randomly selectedby the computer to be between 1 and 4 min. The tones were 5 seclong and paired with the 0.5-sec-long foot shocks so that thetone and foot shock terminated together. Thus, conditioned ratsreceived a total of 10 × 0.5 sec of mild foot shock. The responseof the rats to the foot shock itself was typical of that to mildfoot shock: initial startle and eventual immobility. No rat attemptedescape during the administration of foot shock, and no vocalizationwas noted. On day 3, the test day, rats were returned to the testcages and given 10 computer-controlled, random tones without footshock over 30 min. Immediately after the completion of the testsession, rats were killed by decapitation, and the following brainregions were rapidly dissected on a 1°C stage: mPFC, NAS core,NAS shell, striatum and VTA (Horger et al., 1995

). Care was takento avoid the anterior portion of the NAS, which is predominatelythe shell subdivision. The tissue was stored at $-$ 70°C until assayedfor monoamines. Rats were in one of four groups: saline/nonstress,(S)-( $-$ )-HA-966/nonstressed, saline/conditioned and (S)-( $-$ )-HA-966/conditionedgroups.

The videotape of the rat's behavior on the test day was evaluated for the duration of immobility associated with the presentationof the tone. A 1-min interval that included the 5-sec tone and55 sec after the tone was selected for analysis and scored byan experimenter blinded to each subject's treatment. Immobilitywas defined as no visible movement except those necessary forrespiration. Occasionally, nonstressed, control rats would fallasleep during the last three tones; those data were excluded fromanalysis. Sleeping was noted only in nonstressed rats and wasnot associated with the tone but was usually preceded by groomingand other preparatory behaviors. The number of fecal boli leftafter each session was also counted.

Behavioral sensitization to cocaine. Thirty-two naive, male Sprague-Dawley rats (~250 g) were tested for locomotor sensitization to repeated cocaine administration,as previously described (Morrow et al., 1995a). Locomotor testingwas performed in cages identical to the housing cages that werecontained within a sound-attenuated chamber illuminated by a redlight and equipped with a white noise generator. Locomotor activitywas monitored by an automated 16-photocell array (Omnitech DigiscanMicro-monitor, Columbus, OH) set to count photocell beam interruptionsper 10-min interval. The cages were cleaned with 70% ethanol beforeeach testing session, and fresh bedding was used for each rat.On the first day of the experiment, rats were injected with (S)-( $-$ )-HA-966(3 or 5 mg/kg i.p.; Research Biochemicals) or saline and placedinto the test cages. After 30 min of monitoring locomotion, therats were injected with cocaine HCl (15 mg/kg i.p.; Sigma Chemical,St. Louis, MO) or saline, immediately returned to the test cageand monitored for an additional 60 min. Locomotion during this60-min period after the administration of cocaine was used foranalysis. This procedure was repeated for 5 consecutive days,with the sole exception that on the second and fourth days, therats were treated in the home cage. Seven days after the end ofthe chronic treatment, rats were placed into the test cages; after30 min, all rats were injected with cocaine (15 mg/kg i.p.), andlocomotor activity was monitored for 60 min.

GABA_B binding assay. The ability of either (S)-( $-$ ) or (R)-(+)-HA-966 to displace [³H]-( $-$ )-baclofen from a rat tissue preparation was tested in aprotocol based on Hill and Bowery (1981) and Motohashi et al.(1989) with minor modifications. The cerebral cortex from normalrats was dissected, weighed and stored at $-$ 70°C. These frozentissue samples were homogenized in 10 volumes of 0.32 M ice-coldsucrose using a glass homogenizer and Teflon pestle. The preparationwas separated by centrifugation at 1000 × g for 10 min at 4°C,and the resulting supernatant was centrifuged at 35,000 × g for20 min at 4°C. The P2 pellet was resuspended in 10 volumes ofwater at 4°C and centrifuged at 8000 × g for 20 min at 4°C. Finally,the supernatant and buffy layer on the pellet were removed andcentrifuged at 35,000 × g for 20 min at 4°C. The final pelletwas collected and frozen at $-$ 70°C as the crude mitochondrial fractionenriched in synaptic membranes. For the binding assay, the tissuefraction was thawed on ice and suspended in 10 volumes of 50 mMTris·HCl/2.5 mM CaCl₂ buffer, pH 7.4, and centrifuged at 35,00× g for 10 min at 4°C. This wash was repeated two further times.After the final wash, the pellet was resuspended in the Tris·HCl/CaCl₂buffer and 250 µl, 0.4 mg of protein, was removed for the assay.[butyl-4-³H]-( $-$ )-Baclofen (New England Nuclear Research Products, Boston,MA; 32 Ci/mmol), 20 nM/250 µl, and various concentrations of racemicbaclofen, GABA and (S)-( $-$ ) or (R)-(+)-HA-966 were added in a 100-µlvolume and allowed to incubate for 20 min at room temperature.Nonspecific binding was determined by the addition of GABA, 100µM/µl, instead of test compounds. The bound and free [³H]-( $-$ )-baclofen was separated by filtration through Whatman GF/Bpaper, presoaked in 0.1% bovine serum albumin, using a BrandelCell Harvester. Filters were washed three times with ice-coldbuffer, air dried and counted after adding scintillation fluid.Total counts were corrected for nonspecific binding, and IC₅₀values were calculated from triplicate determination in two separateexperiments for each ligand tested, except (R)-(+)-HA-966, forwhich only one experiment was performed.

Biochemical and statistical analyses. DA and DOPAC values were determined from the tissue samples using HPLC-EC, as described by Elsworth et al. (1989) and Morrowet al. (1995b). Briefly, frozen brain regions were sonicated inice-cold 0.1 N perchloric acid, and the precipitated protein wasremoved by centrifugation at 4°C. The supernate was assayed fordihydroxybenzylamine (an internal standard for catecholamines),DOPAC, DA, 5-HIAA and 5-HT by HPLC-EC. Because of the low levelsof DOPAC and DA in the cortex, the mPFC samples were preparedas described above, and an aliquot was removed to determine thelevels of DOPAC and DA. The aliquot was brought to ~pH 8.4 with3 M Tris buffer and extracted onto acid-prepared alumina (SigmaChemical), and the catechols were eluted from the alumina with0.1 M oxalic acid. The concentrated sample containing the internalstandard, DOPAC and DA was quantified using the HPLC setup specifiedabove. Protein content of the sample was estimated from pelletusing the folin-phenol method. DOPAC and DA were quantified againstexternal standards after correcting for any loss using the internalstandard dihydroxybenzylamine. The concentration of the transmitteror metabolite was divided by the amount of protein in the sampleand metabolic activity, or utilization, was calculated by dividingthe metabolite value by the parent value (DOPAC/DA).

ANOVA with Duncan's range test or Student's t test were used for analysis of single timepoint data. In all cases, a valueof P < .05 was considered significant. Multiple timepoint datafrom the behavioral sensitization to cocaine and conditioned fearexperiments were analyzed by repeated measures ANOVA using Duncan'srange test to determine group differences. Where significant effectswere observed, the individual timepoints of repeated measuresdata were examined using one-way ANOVA with Duncan's range testto determine specific differences.

	Results

Top Abstract Introduction Methods Results Discussion References

(S)-( $-$ )-HA-966 and restraint stress. The administration of (S)-( $-$ )-HA-966 (1, 3 or 5 mg/kg i.p.), 50 min before killing, did not alter basal DA utilization (DOPAC/DA)in the mPFC (fig. 1, top) or striatum (data not shown) of nonstressedanimals. In addition, treatment with (S)-( $-$ )-HA-966 (1, 3 or 5mg/kg i.p.) did not alter the level of DA, itself, in the mPFC,NAS or striatum (data not shown). The levels of DOPAC and DA,respectively, in the saline control rats were as follows: mPFC,0.129 ± 0.029 and 0.673 ± 0.142, and NAS, 13.39 ± 2.25 and 92.54± 10.91 ng/mg protein. Basal DA metabolism in the NAS in nonstressedrats was increased by the highest dose of (S)-( $-$ )-HA-966 tested,5 mg/kg, but not by lower doses. After 30 min of restraint, DAmetabolism was elevated in both the mPFC and NAS of saline-treatedrats [fig. 1, PFC: F_(7,50) = 4.83, P < .001; NAS: F_(7,50) = 2.69,P < .05]. No change in the DOPAC/DA ratio was observed in thestriatum (data not shown). However, (S)-( $-$ )-HA-966 blocked thestress-induced increase in DA metabolism in the mPFC in a dose-dependentmanner. The highest dose tested completely blocked the stress-inducedDA metabolism in the mPFC, whereas (S)-( $-$ )-HA-966 at 3 mg/kg onlyblunted this stress response; the stress-induced increase in ratstreated with 3 mg/kg (S)-( $-$ )-HA-966 was significantly differentfrom the saline/stress group (P < .05) as well as the (S)-( $-$ )-HA-966,3 mg/kg nonstressed control (P < .05). At 1 mg/kg, (S)-( $-$ )-HA-966failed to alter the stress-induced DA metabolism in the mPFC.This relationship between the dose of (S)-( $-$ )-HA-966 and the stress-inducedresponse in DA metabolism was not observed in the NAS. The highestdose of (S)-( $-$ )-HA-966 tested blocked the stress-related increasein DA utilization in the NAS and shifted the base-line DA metabolismin the nonstressed controls. Lower doses of (S)-( $-$ )-HA-966 werewithout effect on the stress-activated DA metabolism in the NAS.

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Fig. 1. The effect of (S)-( $-$ )-HA-966 on basal and restraint stress-induced DA metabolism (DOPAC/DA). Rats were treated with (S)-( $-$ )-HA-966,1, 3 or 5 mg/kg i.p., or saline and, after 20 min, placed intoa wire restraint apparatus or left in the home cage for 30 min(hatched and open bars, respectively). Top, in the mPFC, (S)-( $-$ )-HA-966dose-dependently blocked the stress-induced increase in DA metabolism(n = 5-11 for each group). Bottom, in the NAS, restraint stressincreased DA metabolism in the NAS of rats treated with salineand (S)-( $-$ )-HA-966, 1 and 3 mg/kg. The highest dose of (S)-( $-$ )-HA-966tested, 5 mg/kg, increased DA metabolism in the nonstressed controlgroup (P < .05). Stress failed to increase DA turnover furtherin rats treated with 5 mg/kg (S)-( $-$ )-HA-966 (n = 6-14 for eachgroup). *, P < .05 vs. the appropriate nonstressed control. +,P < .05 vs. the saline/stress group.

Effect of (S)-( $-$ )-HA-966 on aversive conditioning. Several significant effects were noted during the extinction period in previously conditioned rats treated with (S)-( $-$ )-HA-966with regard to treatment [treatment: F_(3,20) = 10.75, P < .0005]and the interaction of treatment and time [F_(27,234) = 2.01, P> .05) but not with time [F_(9,234) = .60, P > .05]. As expected,prior conditioning, tone plus foot shock, resulted in evidenceof fear responses in rats during the extinction phase, when thesubjects were presented with the tone by itself. This was indicatedby an increase in immobility during the 1-min period after thetones for the 30-min test period (fig. 2, top, P < .05). On thetest day, the saline and (S)-( $-$ )-HA-966 control rats remainedmobile during and after exposure to the tone (fig. 2, top). (S)-( $-$ )-HA-966/conditionedrats were significantly less immobile than the saline/conditionedrats at several time points, indicating a less fearful reactionto the conditioned tone (fig. 2, top, P < .05). In addition, fear-inducedimmobility in the (S)-( $-$ )-HA-966/conditioned rats was not differentfrom the nonconditioned, saline control rats at several time points(fig. 2, top, P > .05). Based on these results, we conclude thatthe (S)-( $-$ )-HA-96 blunted, but did not block, fear-induced immobility.Furthermore, fear conditioning increased defecation [fig. 2, bottom,F_(3,26) = 4.56, P < .05]. Prior administration of (S)-( $-$ )-HA-966did not alter defecation in nonshocked control rats and blockedfear-induced defecation in conditioned rats (fig. 2, bottom, P> .05).

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Fig. 2. The effect of treatment with (S)-( $-$ )-HA-966 fear conditioning. Rats were treated with (S)-( $-$ )-HA-966 [(S)-( $-$ )-HA] or saline,placed into the test chamber and given 10 tones plus foot shock(Conditioned) or 10 tones alone (Control). The next day, ratswere returned to the chamber and exposed to 10 tones alone. Top,fear-induced immobility in control and conditioned rats treatedwith saline or (S)-( $-$ )-HA-966. During this extinction test, nofoot shocks were delivered. Treatment with (S)-( $-$ )-HA-966 on theconditioning day significantly reduced fear-induced immobility(n = 8 for each group). Bottom, effect of (S)-( $-$ )-HA-966 on fear-induceddefecation. The number of fecal boli remaining in the cage afterthe test session was significantly increased in saline-treated,conditioned rats. (S)-( $-$ )-HA-966 treatment reduced the effectof fear conditioning, so defecation did not differ between theconditioned and control groups treated with (S)-( $-$ )-HA-966 (n= 8 for each group). * and +, P < .05 vs. the saline control andsaline conditioned groups, respectively.

As expected, treatment with (S)-( $-$ )-HA-966 (5 mg/kg i.p.) did not alter the level of DA, itself, in the mPFC, NAS core orshell or the striatum (data not shown). The levels of DOPAC andDA, respectively, in the saline control rats were as follows:mPFC, 0.111 ± 0.005 and 0.664 ± 0.042; NAS core, 26.09 ± 1.41and 149.8 ± 9.6; and NAS shell, 19.43 ± 1.45 and 139.0 ± 8.1 ng/mgprotein. Fear conditioning increased DA metabolism (DOPAC/DA)in the mPFC and the NAS shell, as expected [figs. 3, top, and4, top; mPFC: F_(3,28) = 6.42, P < .005, NAS shell: F_(3,28) = 3.11,P < .05]. In contrast to published studies on other stressors,30 min of a conditioned stress increased DA turnover in the NAScore [F_(3,28) = 3.13, P < .05], in addition to the NAS shell.Treatment with (S)-( $-$ )-HA-966 (5 mg/kg i.p.) on the conditioningday prevented the stress-induced increase on the extinction dayin DA utilization in all regions activated by stress: mPFC, NASshell and NAS core. (S)-( $-$ )-HA-966 did not significantly alterDA metabolism in any region tested of the nonstress control rats.Nevertheless, a tendency for an increase in DA metabolism wasnoted in both the NAS core and shell, which failed to reach significance(fig. 4). Neither conditioning nor (S)-( $-$ )-HA-966 had any effecton DA metabolism in the striatum (data not shown). Elevated 5-HTmetabolism was noted only in the mPFC in response to this aversiveconditioning paradigm [fig. 3, bottom: F_(3,26) = 4.72, P < .01].Prior treatment with (S)-( $-$ )-HA-966 did not significantly alterbasal or fear-induced activation of 5-HT metabolism. These dataindicate that (S)-( $-$ )-HA-966 given during the conditioning wasable to prevent fear-induced increase in DA, but not 5-HT, metabolismin each of the regions activated.

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Fig. 3. The effect of prior treatment with (S)-( $-$ )-HA-966 on conditioned fear-induced increases in DA and 5-HT metabolism in the mPFC.Rats were conditioned as described for figure 2. Rats were killedimmediately after the test session, and the mPFC was dissectedand analyzed for monoamine content by HPLC-EC. DA and 5-HT metabolismwas increased in conditioned rats. Treatment with (S)-( $-$ )-HA-966on the conditioning day prevented the increase in DA, but not5-HT, utilization. *, P < .05 vs. the same treatment, nonstresscontrol (n = 7 or 8 for each group).

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Fig. 4. The effect of treatment with (S)-( $-$ )-HA-966 on conditioned fear-induced increases in DA and 5-HT metabolism in the core andshell subdivisions of the NAS. Rats were conditioned as describedfor figure 2 and killed immediately after the test session, andthe NAS core and shell were dissected and analyzed for monoaminecontent by HPLC-EC. Conditioned rats displayed an increase inDA metabolism in both the core and shell subdivisions of the NAS.Prior treatment with (S)-( $-$ )-HA-966 prevented the fear-inducedincrease in DA turnover in both regions. *, P < .05 vs. the sametreatment, nonstress control (n = 7 or 8 for each group).

Effect of (S)-( $-$ )-HA-966 on base-line and cocaine-induced locomotion. Several significant differences were noted between (S)-( $-$ )-HA-966- and saline-treated rats during the acquisition of cocainesensitization [treatment: F_(5,28) = 18.77, P < .0001, time: F_(2,56)= 5.20, P < .01, and interaction: F_(10,56) = 3.49, P < .01]. Insaline controls, the highest dose of (S)-( $-$ )-HA-966 tested, 5mg/kg, significantly diminished locomotion compared with the saline/salinecontrols (fig. 5, P < .05). A closer examination of the individualdays indicated that (S)-( $-$ )-HA-966, 5 mg/kg, significantly reducednovelty-induced locomotion in saline controls on the first dayonly (fig. 5, day 1, P < .05) but not on the subsequent days,(day 3, P > .05 and day 5, P > .05), indicating that some adaptationto the motoric effects of (S)-( $-$ )-HA-966 had occurred. The lowerdose of (S)-( $-$ )-HA-966, 3 mg/kg did not affect base-line locomotionin saline controls on any day monitored: days 1, 3 and 5 (fig.5, P > .05).

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Fig. 5. The effect of chronic exposure to (S)-( $-$ )-HA-966 on base-line and cocaine-induced locomotion in rats. Rats were given (S)-( $-$ )-HA-966,3 or 5 mg/kg i.p., or saline, placed into a locomotor testingapparatus for 30 min, given saline or cocaine, 15 mg/kg i.p.,and immediately returned to the chamber for 60 min. Total locomotoractivity, as measured by a photocell system, in this 60-min periodwas used for analysis. This protocol was repeated for a totalof 5 consecutive days with the exception that on days 2 and 4,rats were left in the home cage and not monitored for locomotoractivity. The highest dose of (S)-( $-$ )-HA-966 tested significantlylowered locomotor activity on day 1 compared with saline and (S)-( $-$ )-HA-9663 mg/kg in rats not receiving cocaine. As expected, cocaine administrationsignificantly increased locomotion in control rats. (S)-( $-$ )-HA-966,5 mg/kg, prevented the cocaine-induced increase in locomotionon all 3 days tested. The lower dose of (S)-( $-$ )-HA-966, 3 mg/kg,prevented cocaine-induced locomotion on day 5 only. * and +, P< .05 vs. the saline control and the same treatment, noncocainecontrol, respectively (n = 5-7 for each group).

The repeated administration of cocaine resulted in an increasing locomotor response (fig. 5, P < .05). An examination of eachday separately indicated that cocaine significantly increasedlocomotion in saline-treated rats every day tested [day 1: F_(5,28)= 4.39, P < .005; day 3: F_(5,28) = 7.52, P < .0005; day 5: F_(5,28)= 18.60, P < .0001]. Cocaine-induced locomotion only significantlyincreased on days 1 and 3 for rats treated with (S)-( $-$ )-HA-966,3 mg/kg. Cocaine administration failed to significantly increaselocomotor behavior in rats treated with (S)-( $-$ )-HA-966, 5 mg/kgon any day tested (P > .05). After 7 days, during which no cocaineor (S)-( $-$ )-HA-966 was administered, rats were administered anacute cocaine challenge, and several differences were noted [fig.6, treatment: F_(5,28) = 2.93, P < .05, time: F_(5,25) = 52.12,P < .0001 and interaction: F_(25,140) = 3.86, P < .0001]. Ratspreexposed to cocaine had an augmented locomotor response to thechallenge dose of cocaine compared with the saline preexposedcontrols (fig. 6, P < .05). Coadministration of (S)-( $-$ )-HA-966,at 3 or 5 mg/kg, with the chronic cocaine exposure prevented thebehavioral locomotor sensitization to a subsequent challenge doseof cocaine on the test day (fig. 6, P < .05). This indicates thatconcurrent exposure of (S)-( $-$ )-HA-966 during chronic cocaine administrationcan prevent the development of behavioral sensitization to cocaine.

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Fig. 6. The effect of a cocaine challenge on rats previously exposed to cocaine and (S)-( $-$ )-HA-966. Rats were treated for 5 consecutivedays with (S)-( $-$ )-HA-966 and cocaine as described for figure 5.After 7 drug-free days, rats were returned to the test chamberfor 30 min; cocaine, 15 mg/kg, was administered at time 0; andlocomotor activity was monitored for an additional 60 min. Enhancedcocaine-induced motoric activity, or locomotor sensitization,was observed in rats previously exposed to cocaine (sal/coc) comparedwith the saline controls (sal/sal). Prior administration of (S)-( $-$ )-HA-966,5 or 3 mg/kg, with cocaine [( $-$ )HA-5/coc and ( $-$ )HA-3/coc, respectively]prevented locomotor sensitization to cocaine. *, P < .05 vs. thesame treatment control (n = 5-7 for each group).

As expected, rats exposed to cocaine failed to gain weight as rapidly as the saline controls during the chronic phase of thisexperiment (data not shown). Interestingly, rats given repeateddoses of (S)-( $-$ )-HA-966, 5 mg/kg without cocaine, also failedto gain weight as rapidly as the saline controls over the 5-dayperiod [table 1, days 1-5, F_(3,22) = 5.51, P < .01]. This effectwas primarily due to the suppression of weight gain during theinitial period, days 1 to 3 [F_(3,22) = 5.24, P < .01], but notduring the later period, days 3 to 5 [F_(3,22) = .64, P > .05].The lower dose of (S)-( $-$ )-HA-966, 3 mg/kg, as well as the positiveenantiomer, (R)-(+)-HA-966, 15 mg/kg, did not alter weight gainduring repeated exposure (P > .05). The suppression of weightgain did not continue after the drugs were discontinued (datanot shown). The effect of weight gain does not appear to be relatedto short-acting locomotor effects of (S)-( $-$ )-HA-966. The administrationof (S)-( $-$ )-HA-966 occurred 7 to 10 hr before the beginning ofthe dark cycle, when the rats would do most of their feeding.

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TABLE 1
Weight gain during repeated HA-966 treatment
Rats were treated for 5 continuous days with saline, (R)-(+)-HA-966 or (S)-( $-$ )-HA-966. Rats were weighed immediately beforeadministration of drug, and the weight gain over the select periodwas obtained by simple subtraction. No cocaine was administeredto any of the animals during the chronic treatment period indicatedabove. Rats treated with the highest dose of (S)-( $-$ )-HA-966 gainedweight slower during the 5-day period compared with the salinecontrols and those treated with the lower dose of (S)-( $-$ )-HA-966and (R)-(+)-HA-966 [F_(3,22) = 5.51, P < .05]. This effect wasdue to the initial effect of the (S)-( $-$ )-HA-966, (5 mg/kg/day)on weight gain between days 1 and 3 [F_(3,22) = 5.24, P < .05].No difference in weight gain between the groups was noted betweendays 3 and 5 [F_(3,22) = .64, P > .05].

Effect of the enantiomers of HA-966 on GABA_B binding. Neither (S)-( $-$ ) nor (R)-(+)-HA-966 displaced [³H]-( $-$ )-baclofen from the cortical tissue preparations at relevant concentrations(table 2). Racemic baclofen and GABA displaced [³H]-( $-$ )-baclofen at approximately the expected concentrations.The results of this study indicate that it is unlikely that theactions of (S)-( $-$ )-HA-966 are mediated directly through the baclofenbinding site of the GABA_B receptor.

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TABLE 2
IC₅₀ values for (R)-(+)- and (S)-( $-$ )-HA-966 displacement of [³H]( $-$ )-baclofen
A crude mitochondrial fraction enriched in synaptic membranes was prepared from rat cerebral cortex tissue. The values shownare the averages of duplicate experiments, except (R)-(+)-HA-966,which was assayed only once.

	Discussion

Top Abstract Introduction Methods Results Discussion References

(±)-HA-966 has been available for >35 years and has been clinically tested for the treatment of extrapyramidal motor disorders.Now that the distinct enantiomers have been resolved, the meansby which (±)-HA-966 achieves its range of actions can be clarified.This report demonstrates that (S)-( $-$ )-HA-966 can block stress-inducedactivation of behavior, stress-induced increases in dopaminergicsystems and locomotor sensitization to cocaine. However, the siteof action of (S)-( $-$ )-HA-966 remains uncertain, as it does notappear, as suggested, to be the baclofen binding site of the GABA_Breceptor. The actions of the positive enantiomer, although similar,which are generally attributed to the NMDA/glycine receptor complex,show several differences compared with (S)-( $-$ )-HA-966 (Morrowet al., 1993). These data do not support the hypothesis that normalizingDA cell firing rates in anesthetized rats is a likely means bywhich both enantiomers produce behavioral effects in consciousrats.

Comparison with the effects of (R)-(+)-HA-966. One goal of these studies was to contrast the effects of (S)-( $-$ )-HA-966 with its enantiomer, (R)-(+)-HA-966. The results ofthis current study and work by others are summarized in table3. Shepard et al. (1995) proposed that the two enantiomers sharea common mechanism of action, possibly through GABA_B receptors.Based on this finding and current investigation in this laboratory,we proposed that (R)-(+)-HA-966 could block stress-induced changesin DA neurotransmission by normalizing mesocortical DA neuronalfiring rates (Morrow et al., 1993). As the (S)-( $-$ ) enantiomerwas shown to be more potent at this effect than the (R)-(+)-HA-966(Shepard et al., 1995), we tested (S)-( $-$ )-HA-966 in several paradigmsin which the efficacy of the (R)-(+) enantiomer was established.Several similarities between the two enantiomers were that (1)both were noted to have anxiolytic-like actions, (2) both wereable to prevent locomotor sensitization to cocaine and (3) bothwere able to block stress-induced mesocortical DA utilization.Nevertheless, several differences were noted between these twocompounds. First, unlike (S)-( $-$ ), (R)-(+)-HA-966 selectively preventedstress-induced activation of the mPFC but not the NAS (Morrowet al., 1993; Goldstein et al., 1994). This selectivity of (R)-(+)-HA-966is likely due to actions on the glycine/NMDA receptor at the levelof the DA cell bodies in the VTA (Morrow et al., 1993). The selectiveblockade of stress-induced DA metabolism in the mPFC and not theNAS was also noted with a low dose of the noncompetitive NMDAantagonist MK-801 (Morrow, et al., 1993), supporting the NMDAreceptor complex as the sight of action of (R)-(+)-HA-966. Second,a suppression of weight gain was noted with (S)-( $-$ ), but not (R)-(+),HA-966 during chronic administration. This effect was not observedafter cessation of (S)-( $-$ )-HA-966 and does not appear to be relatedto the sedation observed with (S)-( $-$ )-HA-966 because no food wasavailable during the experiment. In addition, the dose of (S)-( $-$ )-HA-966was given 7 to 10 hr before nighttime, the active cycle of therat, when most of the feeding is done. Finally, with regard tosedation, a clear difference was observed: in the (S)-( $-$ ) enantiomer,unlike (R)-(+)-HA-966, the sedative dose and the dose effectiveat preventing stress-induced DA changes were similar. In thisreport, a significant decrease in spontaneous locomotor activitywas noted with (S)-( $-$ )-HA-966 at 5 mg/kg but not 3 mg/kg. In contrast,the positive enantiomer of HA-966 at 100 mg/kg did not disruptlocomotor activity in mice (Bristow et al., 1993; Hutson et al.,1991). These data indicate that the effective anxiolytic doseof (R)-(+)-HA-966 (15 mg/kg) is much lower than the sedating dose,whereas with regard to (S)-( $-$ )-HA-966, the sedating and anxiolyticdoses are much more similar. In addition, the dose of the (S)-( $-$ )and (R)-(+) enantiomers required to block the spontaneous firingof midbrain DA neurons was similar to the sedative dose. In thecase of (R)-(+), but not (S)-( $-$ ), -HA-966, this effective dosewas much greater than the dose required to block stress-inducedchanges to DA metabolism (Shepard et al., 1993, 1995). It is curiousthat both enantiomers have similar, but distinct, actions on themesocorticolimbic DA system and related behaviors through, mostlikely, different neurotransmitter systems.

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TABLE 3
A comparison of the biochemical and behavioral effects of the enantiomers of HA-966

Possible involvement of GABA_B and DA neurons. The mechanism of action of (S)-( $-$ )-HA-966 is not clear, although pharmacological evidence at hand suggests that the GABA_Breceptor may be involved. The strongest support for a GABA_B-relatedmechanism for (S)-( $-$ )-HA-966 comes from studies using the GABA_Breceptor antagonist CGP 35348. Shepard et al. (1993) noted thatCGP 35348 could completely antagonize the suppression of DA neuronalfiring induced by (S)-( $-$ )-HA-966. The effects of racemic HA-966,baclofen and $gamma$ -butyrolactone on DA synthesis could also be suppressedwith CGP 35348 (Waldmeier, 1991). Second, the actions of racemicHA-966, as well as (S)-( $-$ )-HA-966, have been associated with thesedative $gamma$ HB. (S)-( $-$ )-HA-966 and the $gamma$ HB both suppress the spontaneousfiring rate of midbrain DA neurons (Nowycky and Roth, 1977; Rothet al., 1973; Shepard and Lehmann, 1992) and have been shown tohave sedative effects at higher doses (Singh et al., 1990; Tunnicliff,1992, a review). In addition, (S)-( $-$ )-HA-966, $gamma$ HB and the GABA_Bagonist baclofen cause an initial increase in DA accumulation,which is believed to be the result of the cessation of impulseflow in DA neurons and the activation of DA synthesis (Nowyckyand Roth, 1977; Waldmeier, 1990). However, in this report, wedid not see any significant displacement of [³H]-( $-$ )-baclofen by either enantiomer of HA-966, indicating thatthe actions of (S)-( $-$ )-HA-966 are apparently distinct from thebaclofen-binding site on the GABA_B receptor. Taking in accountthe positive pharmacological studies using CGP 35348 and thiscurrent negative binding study, two possibilities for the actionsof (S)-( $-$ )-HA-966 seem likely. First, a distinct subtype of theGABA receptors has been observed with poor sensitivity to phaclofenbut high sensitivity to CGP-35348 (Bonanno and Raiteri, 1993).(S)-( $-$ )-HA-966 might bind to this GABA receptor subtype and thushave GABAergic actions without displacing baclofen. Second, becauseof the similarities in pharmacological action between (S)-( $-$ )-HA-966and $gamma$ HB, another possibility is that (S)-( $-$ )-HA-966 acts on theproposed $gamma$ HB transmitter system (Benavisea et al., 1982; Dohertyet al., 1978). Previous radioligand binding studies have indicatedthat $gamma$ HB may be acting through highly specific membrane bindingsites that do not have affinity for GABA or GABAergic agonists(Benavisea et al., 1982; Maitre et al., 1983). The exact natureof the $gamma$ HB binding site is not clear, but it appears to be functionallylinked to GABA_B activity (Broxterman et al., 1981; Engberg andNissbrandt, 1993; Waldmeier, 1991). The possibility that (S)-( $-$ )-HA-966acts at a baclofen-insensitive site of the GABA_B receptor or atthe $gamma$ HB binding site warrants further investigation.

(S)-( $-$ )-HA-966 altered components of locomotor activation. We used doses of (S)-( $-$ )-HA-966 well below those previously reported to cause sedation (Singh et al., 1990). Nevertheless,unlike lower doses, 5 mg/kg (S)-( $-$ )-HA-966 disrupted base-lineand cocaine-stimulated locomotion. An apparent tolerance developedto this effect by the third exposure. In addition, on the firstday of cocaine exposure, (S)-( $-$ )-HA-966 blunted the cocaine-inducedlocomotor activity at the higher dose tested. Neither effect wasnoted with the lower dose of (S)-( $-$ )-HA-966.

Repeated exposure to cocaine has been demonstrated to cause an enhanced sensitivity to the locomotor effects of a subsequentchallenge dose of cocaine, an effect termed behavioral sensitization(Downs and Eddy, 1932

; Post and Contel, 1983

). Although this observationis thought to involve enhanced dopaminergic transmission, a precisemechanism has not been established (see Wise and Leeb, 1993

, forreview). Drugs acting at the GABA_B receptor, as well as otherneurotransmitter systems, have been noted to prevent behavioralsensitization (Kalivas et al., 1988

; Kalivas and Stewart, 1991

).However, these studies used local application of baclofen intothe VTA, which blocked the motoric effects of acute cocaine, inaddition to locomotor sensitization (Kalivas et al., 1988

; Kalivasand Stewart, 1991

). This current study demonstrates that 3 mg/kg(S)-( $-$ )-HA-966, unlike baclofen in previous studies, preventsbehavioral sensitization to cocaine without disrupting the acutemotoric effects of cocaine.

Role of (S)-( $-$ )-HA-966 in behavioral and biochemical stress activation. Interestingly, the doses of (S)-( $-$ )-HA-966 that blocked psychomotor stimulant-induced behavioral sensitization also affectedstress-induced increases in DA metabolism. Several other compoundshave been demonstrated to have both actions, including (R)-(+)-HA-966(Morrow et al., 1993, 1995a, 1995b) and MK-801 (Karler et al.,1990; Morrow et al., 1993; Wolf and Jeziorski, 1993). The highestdose tested, 5 mg/kg, of (S)-( $-$ )-HA-966 prevented behavioral andbiochemical indices of stress activation. Lower doses of (S)-( $-$ )-HA-966blunted the stress activation of DA. However, the highest doseof (S)-( $-$ )-HA-966 was not able to block the stress-induced increasein 5-HT metabolism in the conditioned fear paradigm. The (R)-(+)enantiomer also failed to alter stress-induced changes in 5-HTmetabolism (Goldstein et al., 1994). The significance of the resistanceof the stress response of 5-HT neurons to drug demonstrated tohave aniolytic-like activity is not clear.

Fear conditioning activated DA metabolism in both the core and shell subdivisions of the NAS, in contrast with several publishedstudies that noted a selective activation in dopaminergic activityafter foot shock in the NAS shell only (Deutch and Cameron, 1992

;Kalivas and Duffy, 1995

). These previous studies using a similarintensity stressor but differ from this current study by (1) durationof stressor and (2) type of stressor. First, we used a longerduration stressor than previous studies. It is quite possiblethat the activation of the subdivisions of the NAS may simplybe temporally distinct, so the NAS shell activates earlier thanthe NAS core. A similar situation was observed im comparing therestraint stress-induced DA metabolism in the whole NAS and themPFC: the onset of activation of the mesocortical DA system wasmore rapid than the mesolimbic, 10 vs. 20 min, respectively (Rothet al., 1988

). By extending the duration of stress in this study,we observe an activation of both the core and shell of the NAS.Neuroanatomic studies have associated the NAS shell and core withthe limbic system and striatum, respectively (Cools et al., 1993

;Deutch and Cameron, 1992

; Heimer et al., 1991

; Zahm, 1991

; Zahmand Heimer, 1990

). This report notes that the activation of theDA projections to both the NAS core and shell can be achievedwithout a relatively intense stressor and without any activationof the striatum, indicating that the dopaminergic neurons projectingto the NAS core activate differently than the nigrostriatal DAneurons and more similar to those DA neurons projecting to theNAS shell. Second, the type of stressor (i.e., psychological vs.physical) may be important in determining the response of thecore and shell subunits of the NAS. It is possible that the useof foot shock stress immediately before killing the rat activatesneuronal pain pathways that may suppress the activation of theNAS core. This is avoided with the use of conditioned fear becauseno painful foot shock is given on the test day.

Conclusion. We report anxiolytic-like actions of the (S)-( $-$ ) enantiomer of HA-966. These actions are similar to those observed with the(R)-(+) enantiomer, a weak partial agonist for the glycine/NMDAreceptor complex, yet have several clear points of distinctionthat seem to indicate a distinct mechanism of action. Althoughthe mechanism of action of (S)-( $-$ )-HA-966 is not clear, it islikely that it acts through the GABAergic neurons, possibly ata $gamma$ HB binding site or a baclofen-insensitive site of the GABA_Breceptor. This compound may represent a novel class of potentialanxiolytic agents with $gamma$ HB-like actions.

	Acknowledgments

(S)-( $-$ )-HA-966 was provided by Research Biochemicals as part of the Chemical Synthesis Program of the National Institute ofMental Health, Contract N01-MH30003.

	Footnotes

Accepted for publication July 15, 1997.

Received for publication March 7, 1997.

¹ This work was supported by United States Public Health Service Award MH14092.

² B. A. Morrow, unpublished observations.

Send reprint requests to: Robert H. Roth, Ph.D., Department of Pharmacology, Box 208066, 333 Cedar Street, New Haven, CT 06520-8066.

	Abbreviations

GABA, $gamma$ -aminobutyric acid; $gamma$ HB, $gamma$ -hydroxybutyric acid; NMDA, N-methyl-D-aspartate; DOPAC, 3,4-dihydroxyphenylacetic acid; DA, dopamine; NAS, nucleus accumbens; mPFC, medial prefrontal cortex; (±)-HA-966, 1-hydroxy-3-aminopyrrolidone-2; 5-HIAA, 5-hydroxyindolacetic acid; 5-HT, serotonin; ANOVA, analysis of variance; HPLC, high-performance liquid chromatography.

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(S)-()-HA-966, a -Hydroxybutyrate-Like Agent, Prevents Enhanced Mesocorticolimbic Dopamine Metabolism and Behavioral Correlates of Restraint Stress, Conditioned Fear and Cocaine Sensitization1

(S)-( $-$ )-HA-966, a $gamma$ -Hydroxybutyrate-Like Agent, Prevents Enhanced Mesocorticolimbic Dopamine Metabolism and Behavioral Correlates of Restraint Stress, Conditioned Fear and Cocaine Sensitization¹