Dopamine Transporter Activity in the Substantia Nigra and Striatum Assessed by High-Speed Chronoamperometric Recordings in Brain Slices

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Vol. 287, Issue 2, 487-496, November 1998

Dopamine Transporter Activity in the Substantia Nigra and Striatum Assessed by High-Speed Chronoamperometric Recordings in Brain Slices¹

Alexander F. Hoffman, Carl R. Lupica and Greg A. Gerhardt

Departments of Pharmacology (A.F.H., C.R.L., G.A.G.) and Psychiatry (G.A.G.), the Neuroscience Training Program (C.R.L., G.A.G.), and the Rocky Mountain Center for Sensor Technology (G.A.G.), University of Colorado Health Sciences Center, Denver, Colorado

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

High-speed chronoamperometric measurements were used to measure clearance of locally applied dopamine (DA) in rat brain slicescontaining the substantia nigra (SN) or striatum. A comparisonof DA signals of similar amplitudes between brain regions revealedthat DA clearance was more rapid in the striatum than in the SN,consistent with the known greater distribution of the dopaminetransporter (DAT) in the striatum. To clarify the role of theDAT in mediating DA clearance within the SN, slices were superfusedwith uptake inhibitors with different selectivities for the variousmonoamine transporters. In the SN, both cocaine and nomifensinesignificantly increased the amplitude and time course of the DAelectrochemical signal. However, neither the serotonin transporter(SERT) inhibitor citalopram nor the norepinephrine transporter(NET) inhibitor desipramine (DMI) produced significant effectson DA clearance. In addition, cocaine and nomifensine affectedthe clearance parameters of the DA electrochemical signal to asimilar extent in both the striatum and the SN, further confirmingthe functional role of the DAT in both brain regions. Local applicationsof d-amphetamine resulted in slow, prolonged DA-like electrochemicalsignals in both the SN and striatum, although the amplitude ofthe evoked response was larger within the striatum. In contrast,KCl-evoked depolarizations yielded rapid, detectable DA-like signalsonly within the striatum. Taken together, these data demonstratethe functional role of DAT in mediating DA clearance and releasewithin both the striatum andSN.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

The nigrostriatal DA pathway is an important component of basal ganglia circuitry, which has been postulated to play a criticalrole in the initiation and maintenance of motor behaviors (Graybiel,1995). Loss of nigrostriatal DA function leads to the clinicalmanifestations of Parkinson's disease (PD) in humans, which includerigidity, tremor and bradykinesia (Hornykiewicz and Kish, 1987).In both human PD and in animal models of the disease, replenishmentof midbrain DA levels, especially within the striatum, has beenshown to ameliorate many of the symptoms of the illness. However,the failure of DA replacement strategies to completely restorenormal motor function in individuals affected with PD has ledseveral investigators to reconsider the current model of DA andits role within the basal ganglia. In particular, there has beena renewed focus on the role of DA in "extrastriatal" nuclei withinthe basal ganglia, such as the subthalamic nucleus, globus pallidusand SN. A growing body of literature supports the concept thatDA signaling within the SN may modulate basal ganglia output,thereby contributing to various motor behaviors (Robertson andRobertson, 1989; Hudson et al., 1993; Tseng et al., 1997). Thus,while the importance of DA within the striatum remains unequivocalunder both normal and pathophysiological conditions, there isevidence to suggest that investigations of DA regulation withinother areas of the basal ganglia would enhance our current understandingof movement and movementdisorders.

The high-affinity DAT is a primary regulator of DA signaling at mammalian synapses and is known to be localized to both thesomatodendritic and axonal processes of midbrain DA neurons (Ciliaxet al., 1995; Nirenberg et al., 1996b). In particular, DAT hasbeen shown to exist on cell bodies of the SNc, as well as on dopaminergicdendrites within the SNr (Coulter et al., 1995; Nirenberg et al.,1996b). The DAT, SERT and NET are related members of a superfamilyof Na⁺- and Cl-dependent neurotransmitter transporters, which are importanttargets for both drugs of abuse and antidepressant compounds (Girosand Caron, 1993; Amara and Kuhar, 1993). Blockade or reversalof DAT-mediated transport results in an elevation of extracellularDA levels and has been shown to underlie the neurobiological actionsof several major psychomotor stimulants, including cocaine andamphetamine (Giros et al., 1996). The contribution of DAT to DArelease and clearance has been most clearly established withinterminal regions, such as the striatum and nucleus accumbens,which are enriched in DAT relative to NET and SERT. However, anatomicstudies suggest that DAT may also play a role in mediating somatodendriticDA clearance and have led some investigators to postulate thatDAT reversal may represent a primary means of somatodendriticDA release (Nirenberg et al., 1996b). Given the potential importanceof DA released within the SN to influence motor behaviors, aswell as the known role of DAT in central DA regulation, functionalstudies pertaining to the actions of DAT within the SN are clearlyofinterest.

Despite the anatomical evidence that DAT plays a major role in DA clearance, biochemical studies have suggested that SERTand/or NET may also contribute to DA uptake in the SN (Kelly etal., 1985; Simon and Ghetti, 1993). However, these studies relyon prolonged incubation of dissociated tissue with [³ H]DA and may therefore be less applicable to physiological conditions.In contrast, in vivo voltammetric recording techniques have beendeveloped that allow for fast (<1 sec) and sensitive (nM) detectionof DA release and uptake (Kawagoe et al., 1993). In anesthetizedanimals, DA uptake can be assessed by locally applying small (pmol)amounts of DA from a micropipette attached 250 to 300 µm froma carbon fiber electrode. The parameters of the DA electrochemicalsignal, detected by high-speed chronoamperometry, are then usedto describe DA uptake. Additionally, a variety of pharmacologicalmanipulations have been shown to modulate the DA signal in a mannerconsistent with loss of DAT activity (Cass et al., 1993a; Casset al., 1993b; Cass and Gerhardt, 1995). Recently, using thisapproach in the SN of anesthetized rats, we have shown that DAT-mediatedDA clearance can be modulated by uptake inhibitors and 6-hydroxydopaminelesions of the nigrostriatal pathway (Hoffman and Gerhardt, 1998).Although such recordings in the intact animal are clearly feasible,there are technical issues, such as localization of probe placement,which make these studies more demanding. In contrast, the brainslice preparation allows for both ease of access to discrete anatomicsites such as the SN, as well as controlled delivery of drugstotissue.

In the present study, we used high-speed chronoamperometric recording techniques in rat brain slices to address several questionsregarding somatodendritic DA regulation. First, we compared theproperties of DA uptake and clearance in the SN with those seenin the striatum to determine if base-line clearance propertiesdiffered between the two regions. Next, SN slices were superfusedwith DAT, NET or SERT uptake inhibitors to determine which transporter(s)were responsible for DA clearance in this brain region. The effectsof DAT inhibitors in the SN were compared with the effects ofthese same drugs in the striatum. Finally, we compared stimulus-evokedrelease between the SN and striatum using KCl-evoked depolarizationand d-amphetamine-evoked DArelease.

	Materials and Methods

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Drugs and drug solutions. DA, cocaine hydrochloride and d-amphetamine sulfate were purchased from Sigma Chemical (St. Louis, MO). DMI and nomifensinemaleate were purchased from Research Biochemicals (Natick, MA).Citalopram was generously provided by Dr. Alan Frazer. Uptakeinhibitors were prepared as fresh 100× stocks dissolved in distilledH₂O and were bath-applied to the slices by a Razel pump (ModelA99).

Slice preparation. All animal protocols were approved by the University of Colorado Institutional Animal Care and Use Committee. Young Sprague-Dawleyrats (50-75 g) were anesthetized with halothane and decapitated.The brains were rapidly removed and chilled in ice-cold aCSF (126mM NaCl, 2.9 mM KCl, 1.5 mM MgCl₂, 2.5 mM CaCl₂, 1.4 mM NaH₂PO₄,10 mM glucose and 25 mM NaHCO₃, 200 µM ascorbate), which was continuouslybubbled with a 95% O₂/5% CO₂ mixture. After blocking the tissue,the brains were mounted in a chilled, aCSF-filled chamber, andcoronal sections (300 µm thickness) were cut using a vibratomeSeries 1000 (Technical Products International, St. Louis, MO).Sections containing the brain regions of interest, with respectto bregma, were as follows: striatum, AP $-$ 0.26 to +1.7 mm; SN,AP $-$ 6.04 to $-$ 4.8 mm; hippocampus AP $-$ 4.52 to $-$ 3.14 mm; dorsalraphe, $-$ 8.0 to $-$ 7.3 mm (Paxinos and Watson, 1986). Slices wereincubated in oxygenated aCSF at 22°C for at least 1 hr beforeelectrochemical recordings. During the recordings, slices werecontinuously superfused with oxygenated aCSF solution at a rateof 2 ml/min. All recordings were carried out at 32° to 33°C.

Electrochemical recordings. High-speed chronoamperometric measurements were carried out using an IVEC-10 system (Medical Systems, Greenvale, NY). Square-wavepulses of 0.00 to +0.55 V, with respect to a Ag/AgCl referenceelectrode, were applied to the working electrode for 100 msecand repeated 5 times per sec (Gratton et al., 1989). The resultingoxidation current (measured during the 0 to +0.55 V step) andreduction current (measured during the +0.55 V to 0 step) weredigitally integrated during the last 80 msec of each pulse. Singlecarbon fiber electrodes (AVCO Specialty Materials, Lowell MA;100 µm length × 30 µm o.d.) were coated with Nafion using thehigh temperature coating procedure previously described (Hebertet al., 1996). All electrodes were calibrated using 2 to 10 µMincrements of DA before each experiment and were both linear (r² $>=$ .997) and selective ( $>=$ 500:1) for DA vs. either DOPAC or ascorbate.Based on the measured detection limit of the electrodes, DA signalshad to achieve amplitudes of 20 ± 2 nM (n = 30) to obtain a signal-to-noiseof ratio of >3. Extracellular changes in DA concentration wereexpressed quantitatively based on the pre-experiment DA calibrationcurves (Gerhardt et al., 1988). In a few experiments, electrodeswere calibrated with serotonin (5-HT), using the "delayed pulse"protocol previously described (Luthman et al., 1997).

Electrode-pipette assemblies were constructed by attaching single-barrel pipettes (o.d. 1 mm; i.d. 0.58 mm; A-M Systems, Everett,WA) to each electrode. The electrode and pipette were attachedvia sticky wax at a tip distance of 200 to 250 µm; pipette tipdiameters were 10 to 15 µm. The assembly was lowered into thedesired recording site(s) so that the tip of the recording electrodewas positioned at a depth of 100 to 150 µm from the surface ofthe tissue. Recordings within the SN were performed in the medialregion of the structure, encompassing both the SNc and SNr. Solutionswere applied via pressure ejection (10-25 psi, 0.5-5 sec) usinga PPS-2 pneumatic pressure system (Medical Systems, Greenvale,NY). For the clearance experiments, single-barrel pipettes contained200 µM DA (or 5-HT) in 0.9% NaCl with 100 µM ascorbate. This concentrationof DA, when locally applied in volumes of 25 to 200 nl, producesextracellular levels of DA ranging from 0.05 to 3 µM (Gerhardtand Palmer, 1987

). In release experiments, single-barrel pipetteswere filled with a solution of either 2 mM d-amphetamine sulfate,dissolved in 0.9% NaCl, or with an excess K⁺ solution (70 mM KCl, 79 mM NaCl and 2.5 mM CaCl₂ in distilledH₂O). All drug solutions were adjusted to pH 7.4 beforeuse.

DA clearance experiments. DA was locally applied at 5-min intervals to establish a stable base-line ( $<=$ 10% variation in the measured signal parameters).After three such base-line signals were obtained, uptake inhibitorswere added to the bath at the desired concentration; subsequentDA applications were performed every 5-min. When drug effectswere seen, maximal effects were observed 10-min after drug application.Washout of drug effects within 20 to 30 min was observed in many,but not all,cases.

DA release experiments. Local pressure applications of either d-amphetamine or KCl were performed in multiple sites in several slices, to obtain alarge number of signals for analysis. Although the pressure xtime parameters varied between experiments (15-20 psi, 2-4 sec),our experience utilizing these single-barrel pipettes and pressure× time parameters suggests that volume outputs are likely to be50 to 200 nl. Identification of the endogenous signal as "DA-like"was based on the red/ox ratio of the electrochemical signal (Grattonet al., 1989; Gerhardt, 1995). Typical in situ red/ox ratios werebetween 1 and 1.4 for DA, 0.05 and 0.1 for 5-HT and 0 forascorbate.

Signal parameters. For each individual signal, the following parameters were analyzed: (1) peak amplitude of the obtained signal; (2) T₈₀, thetime for the signal to rise and decay by 80% from peak amplitude;and (3) clearance rate (T_c, in µM/sec), defined by the changein DA concentration between the T₂₀ and T₆₀ time points (e.g.,the slope of the linear portion of the decay curve). These parameterswere selected based on previous work from our laboratory thathas characterized the effects of uptake inhibitors on these portionsof the electrochemical signal (Cass et al., 1993a, 1993b; Cassand Gerhardt, 1995) (Hoffman and Gerhardt, 1998). In addition,these parameters were chosen because they are known to primarilyreflect DA uptake, rather than metabolism or diffusion (Cass etal., 1993b). The red/ox ratio, calculated by dividing the reductioncurrent by the oxidation current at the peak of the response,was also analyzed for each signal. For the d-amphetamine-evokedrelease experiments, the rise time of the signal to peak amplitudewas alsoanalyzed.

Statistical analysis. Linear regression analysis was performed using Prism version 2.01 (GraphPAD Software, San Diego, CA). For the experimentswith the uptake inhibitors, base-line parameters were definedat each site by averaging three reproducible signals to yielda single value at a given recording site. Changes in these parametersafter drug application were expressed as a percentage change fromthe base-line and were analyzed using a two-tailed Student's ttest (hypothetical mean of 100%). Comparisons among the striatum,cortex and SN were performed using a one-way ANOVA followed byTukey-Kramer post-hoc comparisons. All other comparisons wereperformed using a two-tailed Student's t test. In all tests, P< .05 was defined as statistically significant. Statistical analyseswere performed using SigmaStat 2.0 (Jandel Scientific Software,San Rafael, CA) or Instat 2.04 (GraphPADSoftware).

	Results

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Comparisons of Base-line DA Clearance Properties Among Different Brain Regions

Previous studies utilizing high-speed chronoamperometric recordings in acutely anesthetized rats have shown that DA clearancecan differ dramatically among various brain regions, and we havehypothesized that these differences relate to the distributionand activity of DAT sites (Cass and Gerhardt, 1995; Hoffman andGerhardt, 1998). To confirm this hypothesis in the slice preparation,we collected a large number of electrochemical signals from threebrain regions $---$ cortex, striatum and SN $---$ known to differ in the numberand/or activity of DAT sites. The clearance rates and time coursesof signals of equivalent amplitude were then used to compare DAuptake in the variousareas.

Substantia nigra versus striatum. To compare properties of DA clearance between the SN and striatum, we examined clearance rates (T_c) and time courses (T₈₀)of electrochemical signals over several amplitude ranges in eachbrain region. A total of 181 signals from the striatum and 284signals from the SN were used in the analysis. Red/ox ratios forlocally applied DA signals averaged 1.18 ± 0.02. There was considerablevariability in the other observed parameters of the electrochemicalsignals, perhaps owing to the exact location of the recordingelectrode from experiment to experiment. To facilitate the analysis,signals were arbitrarily grouped into the following amplituderanges (in µM): <.5, 0.5 to 1, 1 to 1.5, 1.5 to 2, 2 to 3, 3 to4 and 4 to 8. The resulting clearance rates and time courses werethen plotted against the amplitude ranges. The results of thisanalysis are shown in figure 1. As shown in figure 1A, in boththe SN and striatum, increases in signal amplitude resulted inlinear increases in the observed rate of DA clearance (r² = .995 and .963 for the SN and striatum, respectively). However,the slope of the line was significantly (P < .05) lower in theSN, relative to the striatum, indicating a reduced clearance rateover the entire amplitude range. Similarly, for all signal amplitudestested, the time courses of the electrochemical signals were significantly(P < .05) longer in the SN, relative to the striatum (fig. 1B).

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Fig. 1. Comparison of DA clearance parameters in striatal ( $open circle$ ) and SN ( $bullet$ ) slices. Signals between 0.2 and 8 µM were sorted into amplitude ranges to simplify the analysis. All data points represent the mean ± S.E.M. of at least 10 data points per range. A, Clearance rates were linear with respect to amplitude over this range in both brain regions (r² = .96 and r² = .99 for the striatum and SN, respectively). However, rates of clearance were significantly lower in the SN than in the striatum (slope difference, P < .05). B, T₈₀ values for the same amplitude range. The elevations (intercepts) of the lines were significantly (P < .05) different between the SN and striatum, indicating that time courses were slower in the SN over the tested range of amplitudes.

Striatum vs. cortex. As an additional comparison of DAT function among brain regions, we compared signals of equivalent amplitude in the striatumand cortex. A total of 42 signals (amplitude range, 0.2-10 µM)were collected from regions of the cortex overlying the striatum.Subsequently, an equal number of signals, over the same amplituderange, were selected from the striatum and SN to yield the same(mean) amplitude value. The results are shown in table 1. Forsignals of equivalent mean amplitude, the time course was significantly(P < .05) prolonged, and the clearance rate was significantly(P < .05) reduced in the cortex and SN, relative to the striatum.Additional experiments, in which the same recording assembly wasused in both the striatum and cortex of the same slices, revealedthat these differences were not due to variability in the electrode-pipetteassembly (data not shown).

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TABLE 1
Comparison of DA clearance in the striatum, cortex and substantia nigra
Comparison of DA electrochemical signals of equivalent amplitude in the striatum, SN and cortical tissue overlying the striatum. Data represent the mean ± S.E.M. of the observed parameters (n = total number of signals). An equal number of signals were collected from each brain region and were matched by amplitude to produce an equivalent mean amplitude value. For signals of similar amplitude, DA clearance rates (T_c) were significantly (^a P < .05) lower in the cortex and SN than in the striatum. In addition, the time course (T₈₀) of the signal was significantly (^a P < .05) longer in the cortex and SN than in the striatum. Comparisons were performed using a one-way ANOVA followed by a Tukey-Kramer post-hoc analysis.

Effects of Uptake Inhibitors on DA Clearance

The results outlined above suggest that DA clearance differs across brain regions in a manner consistent with known differencesin DAT density. However, to more conclusively demonstrate therole of DAT in mediating the cessation of the DA electrochemicalsignal, we used uptake inhibitors which are known to interferewith DAT function. In these experiments, DA was locally appliedat 5-min intervals to obtain a minimum of three reproducible base-lineelectrochemical signals. DA clearance was then monitored at 5-minintervals during and after bath application of uptake inhibitors.Changes after drug application were represented as a percentagechange from the base-line, which was defined as 100%. Averagebase-line signals were $<=$ 2 µM in amplitude in all experiments,since we have previously found that DA signals in this concentrationrange are consistently modulated by uptake inhibitors (Cass andGerhardt, 1995; Hoffman and Gerhardt, 1998).

Cocaine. Although cocaine has similar affinity for all three major amine transporters, it is believed that most of its neurobiologicaleffects are related to inhibition of DAT function (Cass et al.,1993a; Giros et al., 1996). We therefore compared the actionsof this drug on DA electrochemical signals in both the striatumand SN. A representative experiment in a striatal slice is shownin figure 2. After establishing a stable base-line signal, cocaine(50 µM) was superfused onto the slice for 10-min. This resultedin a potentiation of both the amplitude and time course (T₈₀)of the signal, which gradually returned to base-line after cessationof drug delivery. Figure 3A shows a summary of the effects ofcocaine on the observed signal parameters in both the SN and striatum.In both brain regions, cocaine significantly potentiated boththe amplitude and time course of the electrochemical signal. Theclearance rate parameter (T_c) was not significantly affected bythe drug.

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Fig. 2. Representative effect of cocaine on DA clearance in a striatal slice. Local application of DA at 5-min intervals produced reproducible base-line signals, as shown. Cocaine (50 µM) was applied for a 10-min period, indicated by the solid bar. The last signal in the trace shows a partial washout of the drug effect. The inset plot shows the last base-line signal and 10-min post-cocaine signal on an expanded time scale, to highlight the differences in the time course after drug application.

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Fig. 3. Summary of the effects of cocaine and nomifensine on measured DA clearance parameters in brain slices. The black bars represent drug effects in the SN, and the striped bars represent drug effects in the striatum. Since base-line clearance parameters differed between the two regions, all data represent the percentage change from the average of three reproducible base-line signals (mean ± S.E.M.). A, In both the SN (n = 11) and striatum (n = 18), cocaine significantly potentiated the amplitude and time course (T₈₀) of the electrochemical signal. B, Nomifensine also potentiated the amplitude and time course of the signal in the SN (n = 14) and striatum (n = 14). Significant differences are shown at the *P < .05, ** P < .01 and *** P < .001 level.

Nomifensine. The effects of cocaine on the DA electrochemical signal are consistent with the previously reported effects of this drug onDAT activity (Cass et al., 1993a; Cass et al., 1993b). To extendthis finding, we used the DAT/NET inhibitor nomifensine in boththe SN and striatum. Figure 4 shows a representative effect ofnomifensine (5 µM) on the DA signal in both the striatum and SN.Similar to cocaine, nomifensine potentiated both the amplitudeand time course of the electrochemical signal in both brain regions.A summary of the effects of nomifensine is shown in figure 3B.

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Fig. 4. Representative effects of nomifensine on DA clearance in A, a striatal slice and B, a SN slice. In both cases, the solid black line shows the last of three reproducible base-line signals taken before drug application. The broken line shows the effect of a 10-min bath application of nomifensine (5 µM). Note that, although the base-line signals are of similar amplitude in the two brain regions, the time courses are different.

Effects of SERT and NET inhibitors. The similarity of the effects of cocaine and nomifensine on DA clearance in the striatum and SN would suggest that DAT playsa major role in DA clearance in both brain regions. However, ithas also been argued that DA clearance in the SN may be mediatedby SERT and NET, which are also inhibited by cocaine and nomifensine,respectively (Hyttel, 1982; Richelson and Pfenning, 1984). Toexamine this possibility, we tested the effects of the NET inhibitorDMI (200 nM) and the SERT inhibitor citalopram (500 nM). To ensurethat inhibitors were effective at these concentrations, we testedthe effects of citalopram on 5-HT clearance in the dorsal raphe,a region of high SERT density (Gehlert et al., 1995). In thisexperiment, 5-HT was substituted for DA in the micropipette, andclearance was monitored as described for DA. As shown in figure5A, a 10-min bath application of citalopram potentiated the 5-HTelectrochemical signal, consistent with an inhibition of SERTfunction. The effects of DMI on NET-mediated DA clearance weretested in the CA3 region of the hippocampus. Although the DA signalwas relatively prolonged in this area, consistent with a low DATdensity, DMI effectively potentiated the signal in this region(fig. 5B). The effects of DMI and citalopram were confirmed in2 or 3 additional slices from each region (data not shown). Asshown in figure 6, neither citalopram nor DMI significantly affectedthe measured DA clearance parameters in the SN.

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Fig. 5. Effects of SERT and NET inhibition. A, Recording from a slice containing the dorsal raphe. 5-HT (200 µM barrel concentration) was locally applied at 5-min intervals to achieve three stable base-line signals. These signals were averaged together to yield the lighter tracing shown. Following a 10-min application of the SERT inhibitor citalopram (500 nM), the signal was potentiated (darker trace). B, Recording from the CA3 region of a hippocampal slice. Local application of DA at 5-min intervals resulted in 3 reproducible signals, averaged together to yield the lighter trace. The NET inhibitor DMI (200 nM) was applied for 10-min, resulting in a potentiation of the signal (darker trace).

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Fig. 6. Summary of the effects of uptake inhibitors in SN slices. Data are represented as in figure 4. Both cocaine (50 µM; n = 11) and nomifensine (5 µM; n = 14) significantly potentiated the amplitude and time course of the electrochemical signal (*** P < .001; ** P < .01). Neither DMI (200 nM; n = 9) nor citalopram (500 nM; n = 7) affected any of the measured signal parameters.

Comparison of DA and 5-HT Red/ox Ratios In Situ

We and others have previously used the red/ox ratio of the chronoamperometric recording to distinguish among various monoaminesthat oxidize at similar potentials (Gratton et al., 1989; Luthmanet al., 1997). In our DA clearance studies, it was noted thatin situ red/ox ratios for DA were markedly higher than previouslyreported and were consistently higher than red/ox ratios observedin vitro. Aware of reports that 5-HT may be the predominant electroactivespecies detected within the rat SN (Rice et al., 1994; Iravaniand Kruk, 1997), we wanted to ensure that this higher red/ox ratiofor DA would not preclude discrimination between endogenouslyreleased DA and 5-HT in situ. Therefore, we measured the red/oxratios of exogenously applied 5-HT signals in the dorsal rapheor SN, collected during the course of the clearance experimentsdescribed above. A total of 111 signals were analyzed, and theaverage red/ox ratio of 5-HT signals was found to be 0.08 ± 0.01(mean ± S.E.M.). In vitro calibrations of electrodes (n = 5) againstboth DA and 5-HT revealed that these electrodes were more sensitivefor 5-HT (68 ± 7 picocoulombs/µM) than for DA (26 ± 1 picocoulombs/µM).

Effects of KCl and d-Amphetamine on DA Release

The results outlined above suggest a common role for DAT-mediated DA clearance in both the striatum and SN. However, it hasalso been suggested that the DAT may play an important role inDA release under certain circumstances and that DAT-mediated effluxmay be one way in which somatodendritic DA release occurs (Nirenberget al., 1996b). Therefore, we compared the effects of KCl-evokeddepolarization and d-amphetamine-evoked efflux on DA release inthe SN andstriatum.

KCl-evoked release. Previous data have shown that local application of small amounts of KCl from a micropipette produces an electrochemical signalthat is identical to that observed after local application ofDA (Gratton et al., 1989; Hebert et al., 1996). Using local applicationof 70 mM KCl (15-20 psi, 2-3 sec in all cases), a total of 103signals were obtained from striatal slices. The red/ox ratio ofthese signals (1.50 ± 0.04) was nearly identical to that observedwhen DA was applied locally within the striatum (1.30 ± 0.03,n = 181), confirming the DA-like nature of the electrochemicalsignal. Although there was heterogeneity in the amplitude of theresponses, the signals were then grouped into amplitude ranges,similar to the DA clearance studies. As shown in figure 7, whenthe clearance rates of these KCl-evoked DA responses were comparedto the clearance rates of locally applied DA signals over thesame amplitude range, no significant differences were observed.Similarly, the T₈₀ values between endogenous and exogenous DAsignals were not statistically different over the same amplituderange (data not shown). Interestingly, application of KCl in theSN did not produce any detectable electrochemical signals (n =12).

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Fig. 7. Comparison of clearance rates for locally applied DA signals ( $bullet$ , solid line) and KCl-evoked releases (

, broken line). Signals were compared over the same amplitude range; each data point represents at least 10 individual signals. For both the DA applications (r² = .97) and the KCl-evoked responses (r² = .98), clearance rates were linear over the observed amplitude range. Note the juxtaposition of the regression lines. Linear regression analysis revealed that the slopes and intercepts of the lines were not significantly different. The inset plot shows representative oxidation current signals produced by local application of DA (solid line) and 70 mM KCl (broken line). Signals were chosen to be of similar amplitude to more directly compare clearance rates and time courses.

d-Amphetamine-evoked release. Although the DAT normally acts to remove DA from the extracellular space, amphetamine-like drugs are able to promote DA effluxfrom neurons via a reversal of DAT activity (Sulzer et al., 1993).Given our findings here which suggest that DAT is a major regulatorof DA clearance in the SN and striatum, it was of interest tous to compare the actions of d-amphetamine on DA release in thesetwo regions as well. In these experiments, d-amphetamine (2 mMbarrel concentration) was locally applied via pressure ejection(15-20 psi, 2-4 sec). Representative signals from the striatumand SN are shown in figure 8. In both brain regions, d-amphetamineapplication resulted in a slow, prolonged increase in the electrochemicalsignal, which decayed over several min. In the striatum, the timecourse of the d-amphetamine-evoked signal was markedly differentthan that seen after KCl application (fig. 8B). On average, d-amphetamine-evokedsignals achieved higher amplitudes in the striatum than in theSN, resulting in longer rise times and overall time courses inthe former region. However, the red/ox ratios were found to beDA-like in both regions, confirming the identity of the electroactivespecies as DA. A summary of all d-amphetamine-evoked signals fromboth the SN and striatum is shown in table 2.

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Fig. 8. Representative examples of DA release in midbrain slices. A, Signals from the striatum and SN were obtained by pressure ejection (20 psi × 2 sec in both cases) of a 2 mM d-amphetamine solution. For clarity, only the oxidation current signal is shown, although both signals had red/ox ratios that were DA-like in nature. Note the prolonged time course of the signal in both brain regions and the higher amplitude of the signal in the striatum. B, For comparison, a single KCl-evoked response (solid line) from a striatal slice is superimposed with a d-amphetamine-evoked signal (broken line). Signals were chosen to be of approximately the same peak amplitude; however, note the temporal differences between the responses.

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TABLE 2
Comparison of d-amphetamine-evoked electrochemical signals in rat midbrain slices
Summary of the observed signal parameters for d-amphetamine-evoked release in striatal and SN slices. Data represent the mean ± S.E.M. of all signals (n = total number of signals). Local application of d-amphetamine (2 mM, 15-20 psi × 2-4 sec) in both the SN and striatum resulted in slow, prolonged signals in both brain regions. Peak amplitudes, clearance rates and rise times were significantly lower in the SN, compared with the striatum (^a P < .05, ^b P < .01, ^c P < .001; two-tailed Student's t test). The rise time reflects the time from drug application to peak amplitude, and the red/ox ratio is indicative of the DA-like nature of the electrochemical signal.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

In the present study, high-speed chronoamperometric recordings were performed in rat brain slices to compare DA clearanceand release between the SN and striatum. These data representthe first time that the technique of pressure ejection of DA andchronoamperometric measurements of DA clearance has been appliedin brain slices containing the SN and striatum and confirm andextend previous studies performed in anesthetized rats (Hoffmanand Gerhardt, 1998; Cass et al., 1993a, 1993b). First, we foundthat, over a range of DA concentrations, the capacity for DA clearanceis significantly lower in the SN, compared to the striatum. Second,the uptake inhibitors cocaine and nomifensine potentiated theamplitude and time course of the DA electrochemical signal toa similar extent in both brain regions. These results, coupledwith the finding that selective inhibition of SERT and NET withinthe SN did not affect DA clearance, strongly support our hypothesisthat the DAT is the major contributor to DA clearance within theSN. Third, local application of d-amphetamine promoted DA releasein both nigral and striatal slices, although larger mean signalamplitudes were obtained within the striatum. Finally, we reportthat local applications of KCl produced detectable DA-like signalsin striatal slices, but not within theSN.

Since the DAT is believed to be a primary regulator of DA clearance in the nigrostriatal pathway, one of the major goals ofthe present study was to compare DA clearance in both the SN andstriatum. Although radioligand binding (Coulter et al., 1995)and immunocytochemical markers (Ciliax et al., 1995; Nirenberget al., 1996b) have shown that the DAT is present in both brainregions, there remains some controversy as to the functional aspectsof DAT-mediated DA uptake in the SN. Data from studies involving[³H]DA uptake in synaptosomes and slices suggest that a large amountof DA may be taken up by serotonergic and/or noradrenergic terminalswithin the SN (Kelly et al., 1985; Simon and Ghetti, 1993). Givenboth the low levels of NET within the SN (Gehlert et al., 1995)and the poor affinity of SERT for DA (Hoffman et al., 1991), itseems unlikely that DA clearance would be mediated by other transportsystems. In the present study, we report that DA uptake in theSN is mediated by DAT, based on the following lines of evidence.First, direct comparisons of DA clearance in the SN and striatumreveal that, over a range of amplitudes, clearance rates are significantlyslower in the SN than in the striatum. These results are consistentwith the reported 4- to 10-fold greater number of DAT sites withinthe striatum (Coulter et al., 1995), although we cannot, at present,directly equate the differences in the electrochemical parameterswith reported B_max or V_max values for DAT. In addition, DA clearancewas also reduced in the cortex, which contains fewer DAT sitesthan either the striatum or SN (Coulter et al., 1995; Cass andGerhardt, 1995). Second, the results obtained with the uptakeinhibitors clearly demonstrate the role of DAT in mediating DAclearance within the SN. We report that nomifensine and cocainepotentiated the amplitude and time course of the DA electrochemicalsignal in both the SN and striatum, in a manner consistent withprevious chronoamperometric recordings performed in anesthetizedanimals (Cass et al., 1993a, 1993b; Hoffman and Gerhardt, 1998).The similarity of the effects of both of these drugs in striataland nigral slices suggests that a common mechanism (e.g. DAT)is responsible for DA clearance in both regions. To demonstratethat the effects of nomifensine and cocaine were not due to inhibitionof other transporters, we also performed experiments with DMIand citalopram, which are potent and selective inhibitors of NETand SERT, respectively (Hyttel, 1982; Richelson and Pfenning,1984). When applied at concentrations that have previously beenshown to be effective in midbrain slices (O'Connor and Kruk, 1991;Cragg et al., 1997b) and were effective in other brain regionsin the present study, neither of these agents affected DA clearancewithin the SN. Although others have reported effects of DMI onDA uptake within the rostral SN, we found no evidence for NET-mediatedDA uptake in the SN in the present study (Cragg et al., 1997b).It is possible that species, age or methodological differencesare responsible for this discrepancy. However, the data reportedhere corroborate our recent findings in intact animals(Hoffmanand Gerhardt, 1998), and the effects of cocaine and nomifensineare analogous to those seen by Cragg and coworkers using GBR12909(Cragg et al., 1997b). Thus, we conclude that DAT is the majormonoamine transporter responsible for DA clearance within theSN, over the concentration rangestested.

The DA clearance studies reported here suggest that the DAT is responsible for DA uptake in both the SN and striatum. However,it has also been postulated that DAT may also play a significantrole in promoting DA release, since the transporter can operatein a bidirectional manner (Amara and Kuhar, 1993; Eshleman etal., 1994). Recent data regarding the subcellular localizationof both DAT and the vesicular monoamine transporter-2 (VMAT2),have led to the proposal that DAT reversal may represent a significantmode of DA release within the SN (Nirenberg et al., 1996a, 1996b).If, as we have hypothesized, DAT represents a primary mechanismfor DA uptake within the SN, then agents which can promote DATreverse transport would also be predicted to promote DA releasewithin the SN. In particular, basic drugs such as d-amphetamineare believed to promote DA release via a disruption of intracellularDA stores, perhaps through alterations in intracellular pH (Sulzeret al., 1993). The DAT-dependence of amphetamine-evoked DA releasehas been demonstrated in both DAT-expressing cell lines, as wellas in DAT knockout mice (Eshleman et al., 1994; Giros et al.,1996). In vivo microdialysis studies have demonstrated that somatodendriticrelease of DA within the SN is promoted by systemic or local administrationof d-amphetamine (Heeringa and Abercrombie, 1995; Hoffman et al.,1997). In the present study, we locally applied d-amphetaminevia pressure ejection in the SN and striatum, to demonstrate DAT-dependentDA release. Although a relatively high concentration of d-amphetamine(2 mM) was required to produce release, it should be noted thatthe achieved tissue concentration produced via pressure ejectionis 10 to 100 times less than the barrel concentration of the drug(Nicholson, 1985; Gerhardt and Palmer, 1987). In both brain regions,a slow and prolonged DA-like signal was observed after d-amphetamineapplication, although the peak amplitude of the signals was higheron average in the striatum. The larger peak response in the striatumis consistent with both the higher tissue DA content and DAT levelswithin this region, as well as with previous studies which haveshown d-amphetamine-evoked release within this region (Heeringaand Abercrombie, 1995; Hebert et al., 1996). The slow time coursesof the responses are consistent with the known mechanism(s) ofaction of amphetamine derivatives, as has previously been observedin hippocampal slices and in the SNr (Su et al., 1990; Iravaniand Kruk, 1997).

An interesting difference between the present study and previous voltammetric recordings within the SN pertains to the identityof the predominant neurotransmitter released during stimulation.We report that all of the electrochemical responses in both thestriatum and SN were DA-like in nature, as evidenced by red/oxratios which were similar to those seen when DA was locally applied.This was expected for the striatum, which is known to containmore DA terminals than serotonin terminals (Boja et al., 1992;Coulter et al., 1995). However, it has been reported that 5-HTis the predominant electrochemical species detected in the ratSN after either electrical stimulation or d-amphetamine application(Iravani and Kruk, 1997; Rice et al., 1997). In the present study,we found no evidence for d-amphetamine-evoked 5-HT release withinthe SN. This difference cannot be attributed to an inability todetect 5-HT, since the electrodes used in these recordings havegreater sensitivity for 5-HT than DA. As we have shown, the cleardifference in red/ox ratios between DA and 5-HT allows for discriminationbetween these two compounds in situ. Moreover, the fact that KClapplication did not produce detectable 5-HT signals within theSN would seem to indicate that few active 5-HT terminals existwithin our slice preparation. Other methodological issues, suchas the age of the animals, species of animal used, or recordingprotocols used, may contribute to the observed differences. Recentdata have suggested that the relative incidence of DA and 5-HTrelease within the SN may be influenced by age and species (Cragget al., 1997a). The evidence presented here suggests that d-amphetamineis able to promote DA release within both the striatum and SN,in a manner consistent with both DA content and DAT activity inthese brainregions.

One issue that we feel merits discussion is our observation of higher in situ red/ox ratios for DA than previously reported.Previously, we have shown that in situ red/ox ratios for DA arebetween 0.5 and 0.8 and are consistent with ratios obtained invitro (Gratton et al., 1989; Hebert et al., 1996). In the presentstudy, we found that in situ red/ox ratios for locally appliedDA signals were typically $>=$ 1. It is possible that part of thisdifference is due to the high-temperature Nafion coating procedurethat we have recently begun to employ (Hebert et al., 1996; Hoffmanand Gerhardt, 1998). However, since in vitro calibrations withDA never yielded these high ratios, it seems more likely thatit is a combination of the microenvironment of the tissue preparationand the surface properties of the electrode which produces thiseffect. A more detailed explanation of this phenomenon is beyondthe scope of the present study, although we suggest that red/oxvalues $>=$ 1 may reflect some adsorption of DA molecules to the surfaceof electrode. Local applications of ascorbate (20 mM barrel concentration)produced signals with red/ox ratios of 0, suggesting that theincrease in red/ox ratios observed in situ is not applicable toall electrochemically active compounds (data not shown). Moreover,the mean red/ox ratio of 0.08 for 5-HT in situ that we reporthere is similar to that previously reported (Luthman et al., 1997).We would emphasize that this higher red/ox ratio does not precludea distinction between DA and 5-HT signals in situ. Indeed, thehigher ratio for DA that we report here appears to enhance thedifference in the red/ox ratio between the two compounds. Therefore,we suggest that the red/ox ratio can still be used to identifycompounds in situ and that the endogenous signals we report herelikely represent DAsignals.

In contrast to d-amphetamine, KCl-evoked DA release is believed to reflect the more classical properties of neurotransmitterrelease, such as Ca⁺⁺ dependence and sensitivity to tetrodotoxin (Elverfors et al.,1997). Electrochemical recordings, performed in the striatum ofanesthetized animals, have shown that local application of smallvolumes of 70 mM KCl produces signals that are identical to signalsproduced after exogenous application of DA (Gratton et al., 1989;Friedemann and Gerhardt, 1992; Hebert et al., 1996). A comparisonbetween endogenous and exogenous signals had not been performedin brain slices, but is necessary to confirm the validity of theDA clearance protocol in this preparation. We now report that,in striatal slices, local applications of KCl produced electrochemicalsignals that were similar to those observed after local applicationsof DA. The inability of locally applied KCl to produce detectableDA signals within the SN may simply be due to the failure of thisparticular stimulus to sufficiently depolarize the dendritic elementsto threshold (Hausser et al., 1995). Within the striatum, theamplitude of the evoked response was variable, perhaps reflectingthe heterogeneous distribution of release sites. However, whenclearance parameters were compared to locally applied DA signalsover the same amplitude range, the KCl-evoked responses were indistinguishablefrom the exogenous DA signals. Temporally, these signals weremuch faster than those produced by d-amphetamine application inthe striatum, consistent with the differential mechanism of actionof these chemical stimuli. Moreover, the red/ox ratios of theKCl-evoked signals were nearly identical to those seen duringlocal application of DA and during d-amphetamine-evoked release.Taken together, the data suggest that endogenous DA release canbe elicited by KCl application in striatal slices, and the similarityof the KCl-evoked and locally applied DA signals serves to furthervalidate DA clearance studies in brainslices.

In summary, we have used high-speed chronoamperometric recordings in brain slices to address the functional role of the DATin the SN and striatum. These data demonstrate the capacity forboth DAT-mediated DA release and reuptake by cell bodies withinthe SN. The clarification of the role of DAT within the SN maybe useful in understanding the regulation of somatodendritic DArelease, both under normal and pathophysiologicalconditions.

	Footnotes

Accepted for publication May 20, 1998.

Received for publication January 27, 1998.

¹ This work was supported by grants NS09199, AG06434 and DA07725. AFH is a recipient of an Advanced Predoctoral Fellowship fromthe PhRMA Foundation and GAG received support from a Level IIResearch Scientist Development Award (MH01245) from the NationalInstitutes of MentalHealth.

Send reprint requests to: Greg A. Gerhardt, Ph.D., Department of Psychiatry, University of Colorado Health Sciences Center, 4200 E. 9th Avenue, Box C268-71, Denver, CO 80262. E-mail: Greg.Gerhardt{at}UCHSC.edu

	Abbreviations

DA, dopamine; SN, substantia nigra; SNc, substantia nigra pars compacta; SNr, substantia nigra pars reticulata; DMI, desipramine; DAT, dopamine transporter; SERT, serotonin transporter; NET, norepinephrine transporter; aCSF, artificial cerebrospinal fluid; 5-HT, serotonin; PD, Parkinson's disease.

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Dopamine Transporter Activity in the Substantia Nigra and Striatum Assessed by High-Speed Chronoamperometric Recordings in Brain Slices1

Dopamine Transporter Activity in the Substantia Nigra and Striatum Assessed by High-Speed Chronoamperometric Recordings in Brain Slices¹