Extracellular Dopamine and Amphetamine After Systemic Amphetamine Administration: Comparison to the Behavioral Response

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Vol. 282, Issue 2, 591-596, 1997

Extracellular Dopamine and Amphetamine After Systemic Amphetamine Administration: Comparison to the Behavioral Response¹

Ronald Kuczenski, William P. Melega, Arthur K. Cho and David S. Segal

Department of Psychiatry, School of Medicine, University of California, San Diego, La Jolla (R.K., D.S.S.) and Department of Medicinal and Molecular Pharmacology, University of California, Los Angeles, Health Sciences Center, Los Angeles, California

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

To further delineate amphetamine-dopamine pharmacokinetic-pharmacodynamic relationships, we examined extracellular levelsof dopamine and amphetamine in caudate-putamen after the s.c.administration of 8 mg/kg amphetamine. In a parallel group ofanimals, we also assessed caudate-putamen tissue levels of thedrug. Extracellular concentrations of the transmitter and thedrug exhibited similar temporal profiles, each achieving maximumconcentrations within 30 min of drug administration. Tissue levelsof amphetamine exhibited a similar, although slightly earliertime to maximum levels. The concentrations of amphetamine anddopamine in the extracellular fluid and amphetamine in tissuerapidly declined with similar rates of elimination. In contrastto the temporal profiles for both dopamine and amphetamine, stereotypedbehaviors achieved maximum intensity at about 60 min. In addition,although transmitter and drug declined almost 10-fold from maximumvalues over the 4-hr interval after amphetamine administration,stereotyped behaviors persisted for at least 3 hr before abating.The results of these studies confirm our previous observationthat the temporal profiles for stereotyped behaviors and extracellulardopamine are dissociated, and also extend this dissociation toextracellular amphetamine. In addition, although there was a closecorrespondence between dopamine and amphetamine within each experimentalanimal, individual animals exhibited a broad range of maximaldopamine responses, suggesting a differential responsiveness toamphetamine.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

The DA transporter plays a prominent role in the dopaminergic effects of stimulants such as COC and AMPH (Kuczenski and Segal,1994). Thus, the quantitative features of the drug-induced DAresponse should parallel the synaptic drug concentration at theneuronal membrane. In fact, after COC administration, there isa close temporal correspondence between the extracellular DA responseand extracellular COC (Pettit et al., 1990), and, by inference,the synaptic concentrations of these substances. Although comparabledirect comparisons between extracellular DA and AMPH kineticshave not been available, our previous pharmacokinetic-pharmacodynamicstudies of postmortem tissue levels of AMPH and caudate-putamenextracellular DA suggested a similar AMPH concentration-dependentDA efflux process (Melega et al., 1995). Thus, at least afterthe peak drug response and throughout subsequent elimination times,the temporal profile of the extracellular DA response paralleledthat of brain AMPH levels (Melega et al., 1995).

Recently, however, Clausing et al. (1995) characterized extracellular AMPH dynamics in rat caudate-putamen after s.c. administrationof a wide range of AMPH doses. Those authors reported a temporalpattern of extracellular AMPH that included peak AMPH concentrationsat 60 min after drug administration. In contrast, maximum tissuelevels of AMPH and extracellular DA concentrations have generallybeen reported to occur at substantially earlier times. These datasuggest a profound dissociation between extracellular AMPH andDA and would provide evidence that extracellular AMPH may notplay a primary role in the extracellular DA response. However,interpretation of their results is difficult because they didnot concomitantly evaluate the extracellular DA response profile.It is possible, therefore, that using their experimental procedures,the extracellular DA peak may have occurred at correspondinglylater times, correlating with extracellular AMPH. Alternativelythe extracellular DA response may be dissociated from extracellularAMPH concentrations, and be more closely linked to intracellularactions of the drug.

To evaluate these possibilities, we concurrently examined extracellular concentrations of AMPH and DA in caudate-putamen,as well as tissue levels of the drug, after the s.c. administrationof AMPH. Our results indicate that extracellular AMPH and DA exhibithighly correlated temporal patterns.

	Materials and Methods

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Rats obtained from Simonsen Laboratories (Gilroy, CA; 275-300 g) were maintained four per cage on a 14/10 hr light-dark cycle(lights on at 5:00 A.M.) under standard laboratory conditions,with ad libitum access to food and water for 2 wk before drugtreatment. Animals were then stereotaxically implanted with bilateralguide cannulae using procedures previously described in detail(Kuczenski and Segal, 1989). Guide cannulae extended 2.6 mm belowthe surface of the skull and were aimed at the caudate-putamen(1.0 mm anterior to bregma, ± 2.8 mm lateral and 6.2 mm belowdura). After surgery, animals were housed individually and allowedat least 1 wk to recover before receiving any treatment. Amphetaminewas dissolved in saline and was administered subcutaneously ina volume of 1 ml/kg body weight at about 10:00 A.M. Doses referto the free base.

Each rat was placed in an experimental chamber and the dialysis probes were inserted on the day before treatment (3:00-4:00P.M.) to allow for acclimation to the test environment and foradequate equilibration of the dialysis probes. The behavioralchambers, described in detail elsewhere (Segal and Kuczenski,1987; Kuczenski and Segal, 1989), were sound-proofed and maintainedon a 14/10 hr light-dark cycle (lights on at 5:00 A.M.), withconstant temperature and humidity. Animals had continuous accessto food and water. Throughout the behavioral response after drugadministration, each dialyzed animal was videotaped for subsequentquantitation of drug-induced stereotyped behaviors. Concentricmicrodialysis probes were constructed of Spectra/Por hollow fiber(molecular weight cut-off 6000, o.d. 250 µm) as previously described(Kuczenski and Segal, 1989). The length of the active probe membranewas 3 mm. Probes were perfused with artificial cerebrospinal fluid(147 mM NaCl, 1.2 mM CaCl₂, 0.9 mM MgCl₂, 4.0 mM KCl) deliveredby a microinfusion pump (1.5 µl/min) via 50 cm of micro-line ethylvinyl acetate tubing connected to a fluid swivel. Dialysate fromone probe for each rat was used for neurotransmitter analyses,and from the opposite probe (counter-balanced) for AMPH analyses.Dialysate was collected through glass capillary tubing into vialsfor neurotransmitter analyses containing 20 µl of 25% methanol,0.2 M sodium citrate, pH 3.8. Under these conditions, dialysateDA, 5-HT, and metabolites were stable throughout the collectionand analysis interval. Dialysate for AMPH analyses was collectedinto empty vials and frozen until analysis. Samples were collectedoutside the experimental chamber to avoid disturbing the animal.Individual probe recoveries were estimated by sampling a standardDA solution in vitro and were around 10%. At the end of the experiment,each animal was perfused with formalin for histological verificationof probe placements.

Dialysate samples were collected every 10 or 20 min, and were assayed for DA, DOPAC, homovanillic acid, 3MT and 5-hydroxyindoleaceticacid by high-pressure liquid chromatography with electrochemicaldetection. In all experiments, solutions of standard revealeda clean separation between 3MT and 5-HT. The high-pressure liquidchromatography with electrochemical detection consisted of a 100mm × 4.6 mm ODS-C18 3m column (Regis, Morton Grove, IL) maintainedat 40°C. Mobile phase (0.05 M citric acid, 7% methanol, 0.1 mMNa₂EDTA and 0.2 mM octane sulfonate adjusted to pH 4.0-4.5) wasdelivered at 0.8 ml/min by a Waters (Milford, MA) model 510 pump.Amines were detected with a Waters 460 detector with a glassycarbon electrode maintained at +0.65 V relative to a Ag/AgCl referenceelectrode. The quantitation limits for DA were near 2 to 3 fmol.Concentrations were estimated from peak areas using a Waters Maxima820 data station.

For AMPH analyses, dialysate samples were diluted with 0.5 ml of 10% sodium carbonate solution and 0.1 ml of a solution ofdeuterated internal standard (AMPH-d3), followed by the additionof 6 ml of isopropanol:dichloromethane (1:4). The mixture wasshaken, centrifuged and the organic phase was collected and evaporatedunder a stream of nitrogen. The residue was dissolved in 0.05ml of acetonitrile and the AMPH was derivatized by addition of0.1 ml of trifluoroacetic anhydride, followed by heating at 60°Cfor 15 min. The mixture was then evaporated to remove excess trifluoroaceticanhydride and reconstituted in acetonitrile for injection intothe gas chromatography/mass spectrometry system.

Samples of caudate-putamen tissue were collected from groups of four animals each at 5, 10, 20, 30, 60, 120 and 240 min afterdrug administration. For analysis of AMPH in brain tissue, weighedsamples were homogenized in 0.5 ml of a 0.4 N perchloric acidsolution containing internal standard, 1% EDTA and 0.15% sodiummetabisulfite. The homogenate was centrifuged and the supernatantwas alkalinized with 10% sodium carbonate and extracted with isopropanol-dichloromethane.The extract was derivatized for gas chromatography/mass spectrometryanalysis as described above.

Analyses were performed on a HP5971A gas chromatography/mass spectrometry system with fused silica capillary column coatedwith methylsilicone as described previously (Melega et al., 1995).Standard curves of AMPH, ranging in concentration from 25 to 500pmol/sample were run with each analysis. The slopes of the standardcurves had standard deviations of less than 5%.

Drug-induced neurochemical effects were statistically evaluated using one- or two-way repeated measures analysis of variance.Group/time comparisons were made using t tests with Bonferronicorrections. Amphetamine and DA concentrations were analyzed forrates of change and the apparent rate constants between the differentcompartments were compared. The concentration vs. time data obtainedfor brain tissue, plasma and dialysate were fitted by nonlinearregression procedures to an empirical two exponential expression,reflecting a first order appearance and elimination from the compartmentbeing monitored (Welling, 1986) using the AR program of BMDP (1985)and the rate constants estimated. Because these estimates fitthe entire time course to a common expression, a more robust estimateof individual kinetic parameters can be obtained.

Camp<IT>=</IT>A*kel/(kapp<IT>−</IT>kel)*(e(<IT>−</IT>kel*time)<IT>−</IT>e(<IT>−</IT>kapp*time))

Where k_el and k_app are rate constants for the appearance of AMPH and A is a constant reflecting dose and an apparent volume.)

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Preliminary studies were conducted to compare the caudate putamen dialysate DA responses to AMPH on the left and right sidesof the brain. The s.c. administration of 8 mg/kg AMPH resultedin a pattern of changes in extracellular DA and its metabolites,which was typical to this dose range, including a rapid, approximately30-fold increase in DA, a 20-fold increase in 3MT and a decreasein DOPAC to values near 25% of baseline values. This pattern andthe quantitative features of the responses were identical in theright and left caudate-putamen (data not shown). Comparisons ofthe DA responses (n = 8) on the two sides of the brain revealedhighly significant correlations for both the DA peak response(R² = 0.90, P < .001) and the area under the curve (0-120 min) (R² = 0.70, P < .01).

After administration of 8 mg/kg AMPH, dialysate AMPH and DA concentrations, determined from opposite sides of the brains ofthe same animals, exhibited parallel temporal profiles (fig. 1).Both achieved maximum concentrations at about 30 min, then graduallydeclined with half lives of about 45 min (table 1). The meantimes to peak dialysate concentration for DA and for AMPH (31.8± 2.8 and 30.5 ± 1.3 min, respectively) were essentially the same.The temporal profile for AMPH in caudate-putamen tissue is presentedin figure 2. The time to peak tissue level (22.4 ± 1.5 min) wassignificantly earlier than those for both dialysate measures.T_max values and rate constants for the appearance and eliminationfor DA in dialysate, and for AMPH tissue and dialysate levelsare summarized in table 1.

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Fig. 1. Temporal pattern of extracellular DA (TOP) and AMPH (BOTTOM) concentrations after s.c. administration of 8 mg/kg AMPH. Valuesrepresent mean ± S.E.M. of the concentration, not corrected forindividual probe recoveries. DA and AMPH were assayed in samplescollected concurrently from probes located in caudate-putamenon opposite sides of the brains of the same animals. The temporalaxis depicts the time interval during which each sample was collected.

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TABLE 1
Pharmacokinetic parameters^a

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Fig. 2. Temporal pattern of caudate-putamen tissue levels of AMPH (top) and the oral stereotypy response (bottom) after s.c. administrationof 8 mg/kg AMPH. Values represent the mean ± S.E.M. The dashedline (top) represents the temporal profile of dialysate AMPH concentrationsreproduced from the data of figure 1. The behavioral data anddialysate AMPH were obtained from the same animals, whereas tissueAMPH levels were obtained from a separate, parallel group of animals.The temporal axis (bottom) depicts the time interval during whichthe behavior was expressed.

The behavioral responses of the dialysis animals consisted of a multiphasic locomotor response that included a prolonged periodof intense focused stereotypies, consisting primarily of continuouslicking and biting, typical to this dose. The time course of thestereotypy response is presented in figure 2.

The relationship between dialysate AMPH and DA concentrations for individual animals is presented in figure 3. Each of thefour animals exhibited a direct relationship between the two substancesas a function of time, with correlation R² values ranging from 0.72 to 0.92. However, the slopes of thebivariate plots varied by a factor of 4 to 5 (table 2). Thus,although the DA response was proportional to the extracellularAMPH concentration for each animal, the magnitude of the extracellularDA response exhibited wide individual differences.

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Fig. 3. Relationship between caudate-putamen extracellular DA and extracellular AMPH for individual animals after the s.c. administrationof 8 mg/kg AMPH. The slopes and intercepts for the linear regressionlines are summarized in table 2.

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TABLE 2
Correlation between dialysate AMPH and DA concentrations^a

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Our results indicate that, after the s.c. administration of AMPH, the caudate-putamen extracellular DA response and extracellularAMPH concentrations, as detected by microdialysis, closely paralleleach other. Both the transmitter and the drug achieved maximalconcentrations at near 30 min after AMPH administration, and bothsubstances exhibited equivalent elimination rates. Those data,together with the highly significant correlations between DA andAMPH concentrations for individual animals, are indicative ofa rapidly equilibrating AMPH concentration-DA response relationship,and suggest an intimate concentration-dependent association betweendrug levels in the extracellular space and DA response. It isnoteworthy that parallel temporal profiles have also been reportedfor extracellular concentrations of COC and DA after systemicCOC administration. Because COC enhances DA transmission strictlythrough its interaction with the DA transporter at the extracellularsurface of the neuronal membrane, a close correspondence betweenextracellular COC and DA would be expected. A similar associationwould also be predicted for AMPH, based on an accelerative exchange-diffusionmechanism of action of AMPH at DA terminals (Fischer and Cho,1979); i.e., the drug-induced exchange of DA should be directlyproportional to the extracellular AMPH concentration.

The dynamics of extracellular AMPH and DA demonstrated both similarities to and differences from tissue AMPH. First, all threemeasures exhibited equivalent rate constants of elimination. Thesedata extend to extracellular AMPH, our previous observation ofa parallel decay of AMPH from brain tissue and plasma (Cho etal., 1973; Melega et al., 1995) and lead to the suggestion that,especially at the later time points, all three compartments ofAMPH are in rapid equilibrium. Perhaps not surprisingly, extracellularDA exhibited a similar rate constant of elimination, indicatinga close association between brain drug levels and the transmitterresponse. However, peak tissue AMPH was much higher than peakvalues for extracellular. AMPH, and tissue appeared to achievepeak values at times earlier than those for both extracellularAMPH and DA. With respect to the former, because of its high lipophilicity,the free base of AMPH readily penetrates cellular boundaries.In addition, as has been observed for other similar amines (Sawadaet al., 1994; Sato and Koshiro, 1995), the cationic species ofthe drug would be expected to accumulate in glia and neurons by"trapping" in the more acidic environs of the cytoplasmic milieu,as well as by ion pair formation with intracellular anions, e.g.,Ericinska et al., 1987; Zaczek et al., 1990). In support of thenotion that AMPH accumulates in brain tissue, we have previouslyshown that in i.v. administration of AMPH leads to a steady-statecaudate-putamen tissue/plasma ratio of AMPH concentrations betweeneight and ten (Melega et al., 1995; Cho et al., 1973). In ourstudy, assuming that probe recovery for AMPH was similar to DA(about 10%), the tissue/extracellular AMPH ratio also would beapproximately 10. As a consequence, especially at later times,the tissue AMPH pool must represent a drug reservoir and the netmovement of drug likely proceeds from tissue to extracellularspace to plasma.

That tissue AMPH levels remain substantially higher than extracellular and plasma levels does not necessarily conflict withthe suggestion that these three pools are in rapid equilibrium.A rapid equilibrium should exist between the intracellular andextracellular space; i.e., the rate constant for the diffusion-dependentmovement of AMPH out of the cell would be large compared to therate constant for overall elimination, and the decline of braintissue AMPH should parallel the decline from plasma. However,the actual efflux of AMPH from tissue would appear much slower,because this process depends on the concentration gradient ofthe nonionized species of AMPH between intracellular and extracellularcompartments. Thus, despite the rapid equilibrium, intracellulartrapping through ionization and ion-pair formation results inand maintains a net accumulation of the drug in tissue.

Regarding the time delay between extracellular AMPH and DA compared to tissue AMPH, a similar delay was also observed betweenextracellular DA and tissue AMPH after i.v. drug administration(Melega et al., 1995). That peak extracellular DA correspondstemporally with extracellular rather than with tissue AMPH levelswould suggest that the DA response is more closely linked to actionsof the drug at an extracellular rather than an intracellular site,insofar as tissue measures reflect predominantly intracellularaccumulation. However, some evidence suggests that, in the absenceof high resolution sampling intervals, the time to peak drug concentrationmay appear delayed as an artifact of the integrative nature ofthe microdialysate sampling procedure (Patsalos et al., 1995).Therefore, further studies with greater temporal resolution willbe required to address this specific issue.

Our results are not entirely consistent with those of the only other recent report of microdialysate AMPH levels (Clausinget al., 1995). However, those authors reported a peak extracellularAMPH concentration near 2 µM (uncorrected for probe recovery)after s.c. administration of 5 mg/kg AMPH, which is in good agreementwith the similar values we obtained after 8 mg/kg AMPH. However,they also observed a tissue-to-plasma AMPH ratio near 20:1 at50 min after drug administration, which is substantially higherthan the values we have typically observed (Melega et al., 1995;Cho et al., 1973). The source of this discrepancy is not clear.Additionally, those authors reported peak dialysate AMPH concentrationsaround 60 min after drug, as opposed to the 30-min time pointwe obtained. Unfortunately, it is not possible to directly comparethe drug-transmitter relationship that we observed in our studyto their results. For one, Clausing et al (1995) did not concomitantlyevaluate extracellular DA concentrations. In addition, methodologicaldifferences between the two studies may also contribute to theapparent discrepancies. For example, those authors began sampledialysate collection 2 hr after probe insertion, whereas our dialysisprobes were inserted the previous afternoon to allow for overnightequilibration. Differences in the extent of tissue reequilibrationafter probe insertion might affect the dynamics of substancesin the extracellular space. Additionally, those authors notedthat the onset of behavioral activation following AMPH administrationwas delayed 12 to 15 min. In contrast, using our s.c. drug administrationprotocol, we typically observe an onset of locomotor activationwithin 1 to 2 min. Thus, differences in the method of drug administrationmay have influenced the rates of drug absorption and accumulationinto the brain.

Two points regarding our AMPH pharmacokinetics and the drug-induced behavioral response merit some consideration. First, wehave previously noted the dissociation between the quantitativefeatures of the behavioral and the caudate-putamen and nucleusaccumbens DA responses (for review see Segal and Kuczenski, 1994).This dissociation is most profound in the temporal profiles ofthe stereotypy and DA responses at higher doses of the drug. Consistentwith our past results, this study showed that peak DA concentrationsand the onset of oral stereotypies occurred within the first 30min of the response. However, the magnitude of the stereotypyresponse was maintained during the subsequent 3 hr, although DAconcentrations declined by more than 4-fold to levels that, inresponse to lower doses of the drug, do not promote oral stereotypies.Our results confirm a dissociation between tissue AMPH levelsand the behavior (Kuczenski and Segal, 1994), and extend the dissociationto dialysate AMPH levels as well, i.e., oral stereotypies aremaintained at extracellular AMPH levels that are not typicallyassociated with the production of stereotyped behaviors. Thus,although AMPH levels have a similar time course to DA levels,the behavioral responses do not. That extracellular AMPH and DAlevels follow a parallel time course argues that synaptic DA levelsfollow a similar time course, because the release of DA shouldbe closely dependent on the AMPH concentration. Therefore, thesedata suggest rapid changes in DA-responsive systems that permitoral stereotypies to continue although synaptic DA levels fallbelow levels that are required to initiate these behaviors. Inthis regard, we have recently reported that interruption of ahigh AMPH dose stereotypy response with a low dose of haloperidol(0.1 mg/kg) rapidly terminates the expression of focused stereotypiesand locomotion predominates (Conti et al., 1997), indicating thatcontinued activation of D₂ DA receptors is still required forthe expression of stereotypies. Furthermore, administration ofa low, nonstereotypy producing dose of AMPH (0.5 mg/kg) at theend of a high-dose stereotypy phase reinitiates intense, focusedstereotypies, even though DA levels do not rise to values requiredto initiate stereotypy in a naive animal (R. Kuczenski and D.S. Segal, unpublished data). These observations suggest that DA-responsivepostsynaptic mechanisms responsible for the expression of stereotypedbehaviors may be sensitized during the acute response.

Second, although a high degree of correlation between extracellular AMPH and DA was obtained within each animal, when individualDA responses were evaluated as a function of dialysate AMPH concentrations(table 2), substantial differences in slopes were observed. Theseresults are suggestive of substantial variability in DA responsivity,and these pharmacodynamic differences may contribute to the broadrange of individual differences in behavioral response that wehave previously noted (Segal and Kuczenski, 1987). It is unlikelythat the individual variability in the DA-AMPH relationship thatwe observed is an artifact of sampling from opposite sides ofthe brain, because our previous data (Melega et al., 1995) revealedrelatively small regional variations in AMPH levels after systemicdrug administration. However, a more accurate approach towardevaluating the relative roles of pharmacokinetic and pharmacodynamicfactors in the behavioral response would require the examinationof both AMPH and DA from a single dialysis probe, studies thatare currently in progress.

In summary, in response to systemic AMPH, extracellular DA concentrations are highly correlated with extracellular drug concentrations.These results are consistent with a primary role for extracellularAMPH acting at the DA transporter in the mechanism of action atthe DA terminal, and lend further credence to the view that eventsin the extracellular space provide an accurate reflection of ongoingpsychostimulant drug-transmitter dynamics within the synapticcleft.

	Acknowledgments

The authors thank Molly Roznoski, Joseph Higgins and Debra A. Schmitz for excellent technical assistance.

	Footnotes

Accepted for publication April 1, 1997.

Received for publication October 15, 1996.

¹ This work was supported by research Grants PHS DA-04157, DA-01568, DOE DE-FC03-87ER60616, and PHS Research Scientist AwardMH-70183 (D.S.S.).

Send reprint requests to: Dr. Ronald Kuczenski, Professor of Psychiatry, Psychiatry Department (0603), UCSD School of Medicine, La Jolla, CA 92093.

	Abbreviations

AMPH, D-amphetamine; COC, cocaine; DA, dopamine; DOPAC, 3,4-dihydroxyphenylacetic acid; 3MT, 3-Methoxytyramine; serotonin, 5-HT.

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Extracellular Dopamine and Amphetamine After Systemic Amphetamine Administration: Comparison to the Behavioral Response1

Extracellular Dopamine and Amphetamine After Systemic Amphetamine Administration: Comparison to the Behavioral Response¹