Novel Ca2+ Dependence and Time Course of Somatodendritic Dopamine Release: Substantia Nigra versus Striatum

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The Journal of Neuroscience, October 1, 2001, 21(19):7841-7847

Novel Ca²⁺ Dependence and Time Course of Somatodendritic Dopamine Release: Substantia Nigra versus Striatum
Billy T. Chen and Margaret E. Rice
Departments of Physiology and Neuroscience and Neurosurgery, New York University School of Medicine, New York, New York 10016

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Somatodendritic release of dopamine (DA) in midbrain represents a novel form of intercellular signaling that inherently differsfrom classic axon-terminal release. Here we report marked differencesin the Ca²⁺ dependence and time course of stimulated increases in extracellularDA concentration ([DA]_o) between the substantia nigra pars compacta(SNc) and striatum. Evoked [DA]_o was monitored with carbon-fibermicroelectrodes and fast-scan cyclic voltammetry in brain slices.In striatum, pulse-train stimulation (10 Hz, 30 pulses) failedto evoke detectable [DA]_o in 0 or 0.5 mM Ca²⁺ but elicited robust release in 1.5 mM Ca²⁺. Release increased progressively in 2.0 and 2.4 mM Ca²⁺. In sharp contrast, evoked [DA]_o in SNc was nearly half-maximalin 0 mM Ca²⁺ and increased significantly in 0.5 mM Ca²⁺. Surprisingly, somatodendritic release was maximal in 1.5 mMCa²⁺, with no change in 2.0 or 2.4 mM Ca²⁺. Additionally, after single-pulse stimulation, evoked [DA]_o instriatum reached a maximum (t_max) in <200 msec, whereas in SNc,[DA]_o continued to rise for 2-3 sec. Similarly, the time for [DA]_oto decay to 50% of maximum (t₅₀) was 12-fold longer in SNc thanstriatum. A delayed t_max in SNc compared with striatum persistedwhen DA uptake was inhibited by GBR-12909 and D₂ autoreceptorswere blocked by sulpiride, although these agents eliminated thedifference in t₅₀. Together, these data implicate different releasemechanisms in striatum and SNc, with minimal Ca²⁺ required to trigger prolonged DA release in SNc. Coupled withlimited uptake, prolonged somatodendritic release would facilitateDA-mediated volume transmission inmidbrain.

Key words: calcium; dopamine; dopamine transporter; substantia nigra pars compacta; voltammetry; volume transmission; synaptic transmission

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Dopamine (DA) neurons of the substantia nigra pars compacta (SNc) send axon projections to the dorsal striatum via the medianforebrain bundle (Fallon et al., 1978). Importantly, these midbraincells release DA from somata and dendrites, known as somatodendriticrelease (Geffen et al., 1976; Nieoullon et al., 1977; Rice etal., 1994; Jaffe et al., 1998), as well as from axon terminalsin striatum. Both somatodendritic and terminal release are criticalfor the control of movement mediated by the basal ganglia (Robertsonand Robertson, 1989; Timmerman and Abercrombie, 1996; Crocker,1997).

Logic might dictate that somatodendritic release is mediated by a novel mechanism, given the novel source of release. However,no known characteristics contradict the original proposal by Geffenet al. (1976) that release in SNc is vesicular and mediated byexocytosis, as it is in striatum. Indeed, somatodendritic DA releaseis depolarization and Ca²⁺dependent (Geffen et al., 1976; Cheramy et al., 1981; Rice etal., 1994, 1997) and reserpine-sensitive (Elverfors and Nissbrandt,1991; Rice et al., 1994; Heeringa and Abercrombie, 1995). Otherpharmacological agents, including DA-releasing drugs such as amphetamine,DA transport inhibitors, and D₂ autoreceptor antagonists, causeparallel increases in extracellular DA concentration ([DA]_o) inSNc and striatum, although to a lesser extent in SNc (Santiagoand Westerink, 1992; Heeringa and Abercrombie, 1995; Cragg andGreenfield, 1997; Cragg et al., 1997; Hoffman and Gerhardt, 1999).

In particular, evidence for the Ca²⁺ dependence of release is often taken as confirmatory of vesicular release, because Ca²⁺ entry is required for exocytosis (Douglas and Rubin, 1963; Simonand Llinás, 1985; Burgoyne and Morgan, 1995; Catterall, 1999).Influx of Ca²⁺ promotes vesicle fusion via molecular machinery that includesthe vesicle membrane proteins synaptobrevin and synaptotagmin,and the presynaptic membrane proteins syntaxin and SNAP-25 (synaptosomal-associatedprotein of 25 kDa) (Jahn and Südhof, 1994; Catterall, 1999).Moreover, the amount of transmitter released depends on extracellularCa²⁺ concentration ([Ca²⁺]_o), with increased Ca²⁺ entry and enhanced release in elevated [Ca²⁺]_o (Dodge and Rahamimoff, 1967). Consistent with classical exocytosis,axon-terminal DA release in striatum increases with increasing[Ca²⁺]_o both in vivo (Moghaddam and Bunney, 1989) and in vitro (Chenet al., 2001).

Somatodendritic DA release in SNc also requires Ca²⁺. In contrast to striatal release, however, evoked DA release in SNc persistsin low-Ca²⁺ media (Hoffman and Gerhardt, 1999). Indeed, prolonged incubationin Ca²⁺-free media plus EGTA is required to inhibit release by 90% (Riceet al., 1994, 1997), suggesting a potential difference in theCa²⁺ dependence of somatodendritic versus terminalrelease.

Despite apparently strong pharmacological support for similar mechanisms of somatodendritic and axon terminal release, thediscrepancy in Ca²⁺ dependence indicated that additional investigation was necessary.To this end, we evaluated [DA]_o evoked during pulse-train stimulationin varying [Ca²⁺]_o in striatum and SNc in guinea pig brain slices. Additionally,real-time monitoring of DA release after single-pulse stimulationpermitted comparison of the time course of somatodendritic versusterminal release; contributions from differences in DA transporter(DAT) activity and D₂ autoreceptor regulation were alsoassessed.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Slice preparation and solutions. Male Hartley guinea pigs (150-250 gm) were deeply anesthetized with 40 mg/kg pentobarbital(intraperitoneally) and decapitated. All animal handling procedureswere in accordance with National Institutes of Health guidelinesand were approved by the New York University School of MedicineAnimal Care and Use Committee. Coronal striatal and midbrain slices(400 µm) were prepared as described previously (Rice et al., 1997;Chen et al., 2001) using a Vibratome (Ted Pella, St. Louis, MO).Slice coordinates for midbrain were between 7.3 and 8.3 mm anteriorto the interaural line (Smits et al., 1990). All slices were cutin ice-cold HEPES-buffered artificial CSF (ACSF) containing (inmM): 120 NaCl, 5 KCl, 20 NaHCO₃, 6.7 HEPES acid, 3.3 HEPES salt,2 CaCl₂, 2 MgSO₄, and 10 glucose (saturated with 95% O₂-5% CO₂).After cutting, slices were bisected and then allowed to recoverin HEPES-buffered ACSF for at least 1 hr at room temperature beforebeing transferred to a submersion recording chamber (Warner Instruments,Hamden, CT). Once in the recording chamber, slices were equilibratedfor an additional 30 min with ACSF, which contained (in mM): 124NaCl, 3.7 KCl, 26 NaHCO₃, 0, 0.5, 1.5, 2.0, or 2.4 CaCl₂, 1.3MgSO₄, 1.3 KH₂PO₄, and 10 glucose (saturated with 95% O₂-5% CO₂).Chamber temperature was maintained at 32°C with a flow rate of1.2 ml/min. The influence of DA uptake and D₂ autoreceptor activationon the time course of evoked [DA]_o was examined using the selectiveDAT inhibitor GBR-12909 (0.3 and 2 µM) (Bull et al., 1990; Cragget al., 1997, 2001) and the D₂ antagonist sulpiride (1 µM) (Craggand Greenfield, 1997; Chen et al., 2001).

Microelectrodes and voltammetric instrumentation. Carbon-fiber electrodes made from 7-8 µm carbon fibers (type HM, unsized,Courtaulds) were spark-etched to a tip diameter of 2-4 µm (MPBElectrodes; Queen Mary and Westfield College, London, UK). Thevoltammetric method used for all experiments was fast-scan cyclicvoltammetry (FCV). Data were obtained using a Millar Voltammeter(PD Systems International, West Molesey, UK), with data acquisitioncontrolled by Clampex 7.0 software (Axon Instruments, Foster City,CA), which imported voltammograms to a personal computer via aDigiData 1200B analog-to-digital converter board (Axon Instruments).Scan rate for FCV was 800 V/sec, with a sampling interval of 100msec controlled by an external timing circuit. Scan rage was $-$ 0.7V to +1.3 V (vs Ag/AgCl). Voltammograms were obtained in two-electrodemode, with an Ag/AgCl wire in the recording chamber as the referenceelectrode. Electrodes were calibrated in the recording chamberat 32°C with 0.5-2 µM DA in all media used in a given experiment(Kume-Kick and Rice, 1998; Chen and Rice, 1999), e.g., ACSF withvarying Ca²⁺ concentration and/or containing GBR-12909 plus sulpiride. Wehave reported previously that DA concentrations are stable inoxygenated ACSF at 32°C in the recording chamber (Kume-Kick andRice, 1998). Evoked [DA]_o was calculated using post-experimentDA calibration factors (typically 2-3 nA/µM) to convert measuredoxidation current to concentration. Although a relatively highlevel of GBR-12909 (10 µM) can alter electrode sensitivity toDA (Davidson et al., 2000), the lower concentrations used in thepresent studies had noeffect.

Electrical stimulation. Bipolar stimulating electrodes were made from Teflon-coated platinum wire (50 µm bare, 75 µm coated)with tip separation of ~50 µm. The electrode was placed on theslice surface with the carbon-fiber microelectrode positionedbetween the electrical poles and inserted 50-100 µm into the slice,as described previously (Rice et al., 1997; Chen et al., 2001).Pulse-train (10 Hz, 30 pulses) and single-pulse stimulation wereused to evoke DA release. Pulse duration was 100 µsec for trainsand 1000 µsec for single pulses; pulse amplitude was 0.4-0.8 mA.With these stimulating electrodes and protocols, evoked DA releasein SNc is tetrodotoxin sensitive (data not shown), as it is instriatum (Chen et al., 2001). This contrasts with the tetrodotoxininsensitivity of DA release elicited using larger stimulatingelectrodes and higher stimulus intensity in our previous studiesin midbrain and striatum (Rice et al., 1997).

Experimental design. In striatum, consistent evoked [DA]_o can be elicited with repetitive local stimulation (Bull et al.,1990; Chen et al., 2001). Here, striatal DA release was evokedat 10 min intervals in both pulse-train and single-pulse experiments.For Ca²⁺-dependence studies in striatum, the third of three consistentevoked increases in [DA]_o was included in data averages for each[Ca²⁺]_o. For initial uptake and autoreceptor studies in striatum, one-pulsecontrol records were obtained, and then GBR-12909 plus sulpirideapplied. Maximal effects were seen after 1 hr. For subsequentstudies in striatum, slices were preincubated for 1 hr in theseagents, and the third of three consistent records was used indata averages; similar results were obtained with both protocols.The contralateral hemisphere served as the control for experimentsin which preincubation was used. In SNc, maximal release is seenwith the first stimulus and then progressively decreases withrepetition (Rice et al., 1997). Thus, for measurements in SNcwith varying Ca²⁺, pulse-train-evoked DA release was obtained in medial SNc ina given [Ca²⁺]_o; a different [Ca²⁺]_o was tested on the contralateral side. For single-pulse studieswith GBR-12909 and sulpiride in SNc, one hemisphere of a givenmidbrain slice was superfused with the drugs for 1 hr; the contralateralside served as the paired control and was superfused with ACSFfor 1 hr before release waselicited.

Drugs and chemicals. Sulpiride, DA, and components of ACSF and HEPES-ASCF were obtained from Sigma (St. Louis, MO); GBR-12909was from Research Biochemicals (Natick, MA). All solutions weremade immediately beforeuse.

Statistical analysis. All data are given as means ± SEM, in which n is the number of slices. Differences in evoked [DA]_o invarying Ca²⁺ were assessed using one-way ANOVA, followed by Kruskal-Wallispost hoc analysis of maximum evoked [DA]_o. Differences in thetime course of increases in [DA]_o between SNc and striatum andafter DAT and autoreceptor inhibition in each region were assessedusing t test comparisons of time of maximum [DA]_o (t_max) of thetime after the stimulus at which [DA]_o had decayed to 50% of themaximum (t₅₀).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Under most conditions examined, absolute levels of evoked [DA]_o differed between SNc and striatum. To facilitate comparisonsamong different conditions between regions, therefore, the datawere normalized with respect to a defined control condition foreach region (100%). Data are illustrated as percentage of control,with peak [DA]_o for each condition indicated in the text. Foranalysis of the Ca²⁺ dependence of release, maximum evoked [DA]_o in 1.5 mM Ca²⁺ in striatum or in SNc was considered to be 100% for that region,because that was the concentration in which [DA]_o was maximalinSNc.

Ca²⁺ dependence of evoked DA release in striatum and SNc

In striatum, DA release elicited by a train of 30 pulses delivered at 10 Hz showed a marked dependence on [Ca²⁺]_o (Fig. 1A). Release was below detection limits after 30 minsuperfusion of ACSF with nominally 0 or 0.5 mM Ca²⁺ and then increased progressively with increasing [Ca²⁺]_o. Peak [DA]_o was 0.65 ± 0.05 µM (n = 17) in 1.5 mM Ca²⁺, 1.10 ± 0.13 µM (n = 10) in 2.0 mM Ca²⁺, and 1.81 ± 0.14 µM (n = 6) in 2.4 mM Ca²⁺ (Fig. 1A). Each increase in [DA]_o was significantly higher thanin the previous Ca²⁺ (p < 0.001). Taking maximum evoked [DA]_o in 1.5 mM Ca²⁺ as 100%, increasing Ca²⁺ to 2.0 mM caused an increase in [DA]_o to 170%, with an additionalincrease to 280% in 2.4 mM [DA]_o (Fig. 2). These data suggestan approximately exponential dependence of DA release from striatalterminals on [Ca²⁺]_o.

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Figure 1. Evoked [DA]_o in the presence of varying [Ca²⁺]_o in striatum and SNc. Average evoked [DA]_o during pulse-train stimulation (10 Hz, 30 pulses) in striatum (A) and SNc (B) in 0, 0.5, 1.5, 2.0, and 2.4 mM Ca²⁺. Maximum [DA]_o in 1.5 mM was taken as 100%. In striatum, peak [DA]_o was significantly increased by each step increase in [Ca²⁺]_o (p < 0.001; 0 and 0.5 mM Ca²⁺; data from striatum were pooled). In SNc, significant increases were observed between 0 and 0.5 and 1.5 mM Ca²⁺ (p < 0.01); however, no additional increases were seen in 2.0 or 2.4 mM Ca²⁺. Data are means ± SEM (n = 6-17). The dashed lines indicate 100%, and solid bars indicate the stimulation period. Note the difference in time scale between A and B.

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Figure 2. Ca²⁺ dependence of evoked DA release in striatum and SNc. Data were normalized such that 100% is the average maximum evoked [DA]_o during pulse-train stimulation (3 sec, 10 Hz) in 1.5 mM Ca²⁺. In striatum, evoked [DA]_o increased progressively with increasing Ca²⁺ from 1.5 to 2.4 mM. In contrast, DA release was nearly half-maximal in nominally 0 mM Ca²⁺ in SNc but reached a plateau at 1.5 mM Ca²⁺. Data are means ± SEM (n = 6-17). **p < 0.01 and ***p < 0.001 indicates difference from the response in 1.5 mM Ca²⁺ for each region.

Evoked [DA]_o in the SNc showed a dependence on [Ca²⁺]_o that was opposite to that seen in striatum (Fig. 1B). In SNc, DA releasewas readily detected in nominally 0 mM Ca²⁺, with an average maximum [DA]_o of 0.30 ± 0.06 µM (n = 7) (Fig.1B). Evoked [DA]_o increased significantly when [Ca²⁺]_o was increased to 0.5 mM Ca²⁺ (0.49 ± 0.05 µM; n = 8) and again in 1.5 mM Ca²⁺ (0.78 ± 0.09 µM; n = 14; p < 0.01 for each increase). SomatodendriticDA release was maximal in 1.5 mM Ca²⁺, however, with no additional increases in 2.0 or 2.4 mM Ca²⁺ (0.76 ± 0.12 µM in 2.0 mM Ca²⁺, n = 8; 0.79 ± 0.10 µM in 2.4 mM Ca²⁺, n = 24) (Fig. 1B). This plateau could be clearly seen when [DA]_owas plotted against [Ca²⁺]_o (Fig. 2; again taking evoked [DA]_o in 1.5 mM Ca²⁺ as 100%). This suggests that somatodendritic DA release is relativelyCa²⁺ independent beyond a minimal range of [Ca²⁺]_o required to triggerrelease.

Because [DA]_o is more strongly limited by DA uptake and D₂ autoreceptor activation in striatum than in SNc (Cragg and Greenfield,1997; Cragg et al., 1997, 2001; Hoffman and Gerhardt, 1999), lowrelease in 0 mM Ca²⁺ in striatum could appear to be no release if [DA]_o were keptbelow detection limits by uptake or autoreceptor-mediated inhibition.To test this, we evaluated striatal release evoked by pulse-trainstimulation (10 Hz, 30 pulses) in 0 mM Ca²⁺ in the presence of the DAT inhibitor GBR-12909 (2 µM) (Cragget al., 2001) and the D₂ autoreceptor antagonist sulpiride (1µM) (Cragg and Greenfield, 1997; Chen et al., 2001). Under theseconditions, there was still no detectable increase in evoked [DA]_oin striatum in 0 Ca²⁺ (n = 5; data notshown).

Differing time course of evoked [DA]_o in striatum and SNc

A second difference between terminal and somatodendritic DA behavior was indicated by the distinct time course of evoked [DA]_oduring pulse-train stimulation in striatum versus SNc. In striatum,[DA]_o rose to a maximum within the first two to five pulses ofthe train and then decayed during continued stimulation (Fig.1A). In contrast, evoked [DA]_o in the SNc not only increased throughoutthe stimulus train but also continued to rise for 1-2 sec afterthe train ended, with the exception of the response in 0 mM Ca²⁺ (Fig. 1B). To characterize the time courses of these responsesmore fully, we used single-pulse stimulation to evoke DA release;2.4 mM Ca²⁺ was used to ensure reproducible evoked [DA]_o instriatum.

Single-pulse stimulation elicited consistent DA release in both striatum and SNc (Fig. 3). As in pulse-train experiments,the time course of the responses differed markedly between theseregions (Fig. 3A). Whereas the time of maximal evoked [DA]_o (t_max)was <200 msec after stimulus onset in striatum (190 ± 40 msec;n = 8), in SNc, evoked [DA]_o did not reach a maximum for 2-3 secin SNc (2490 ± 460 msec; n = 9) (p < 0.001 for SNc vs striatum).Importantly, the released substance was clearly identified asDA in both regions by the characteristic DA voltammograms recordedat the response maxima (Fig. 3B). The return to baseline was alsomore rapid in striatum than in SNc, with values for t₅₀ (the timeafter stimulus at which maximal [DA]_o had fallen by 50%) of 540± 80 msec (n = 8) in striatum and 6400 ± 240 msec (n = 9) in SNc(p < 0.001; SNc vs striatum).

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Figure 3. Time course of evoked [DA]_o in striatum and SNc after single-pulse stimulation. A, Average evoked [DA]_o by a single pulse (1 msec) in striatum (n = 8) and SNc (n = 9) (error bars have been omitted for clarity; see Fig. 4). The pattern of release differed significantly, as indicated by the difference in the time of maximum [DA]_o (t_max) and time to decay to 50% of maximum (t₅₀) (p < 0.001 for both parameters; see Results for details). B, DA voltammograms recorded at the time of the maximum evoked [DA]_o in striatum and SNc compared with a 1 µM DA calibration voltammogram; these characteristic voltammograms confirm the identity of the released substance as DA (Rice et al., 1997; Chen et al., 2001).

Like [DA]_o amplitude, as discussed above, the duration of stimulated increases in [DA]_o can also be curtailed by DA uptakeand D₂ autoreceptor activation, again with greater efficacy instriatum than in SNc (Cragg and Greenfield, 1997; Cragg et al.,1997, 2001; Jones et al., 1998; Hoffman and Gerhardt, 1999). Toaddress the extent to which these factors might differentiallyinfluence time course in the present studies, we examined twoconcentrations of GBR-12909 (0.3 and 2 µM) (Cragg et al., 1997,2001) in the presence of a single, supramaximal concentrationof the D₂ autoreceptor antagonist sulpiride (1 µM) (Cragg andGreenfield, 1997; Chen et al., 2001). Consistent with the anticipatedeffects of these drugs, evoked increases in [DA]_o elicited bysingle-pulse stimulation were enhanced and prolonged in both striatum(Fig. 4A) and SNc (Fig. 4B). In striatum, peak [DA]_o increasedto ~200% of control in either 0.3 or 2 µM GBR plus sulpiride (p< 0.001; n = 6-8) (Fig. 4A). The enhancement was similar in SNc,with an increase to ~165% of control (p < 0.05; n = 9); in SNc,[DA]_o records in 0.3 and 2 µM GBR-12909 were indistinguishableand were pooled (Fig. 4B).

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Figure 4. Influence of DAT and D₂ autoreceptor inhibition on evoked [DA]_o in striatum and SNc after single-pulse stimulation. In the presence of GBR-12909 (GBR; 0.3 or 2 µM) and sulpiride (sulp; 1 µM), average maximum [DA]_o evoked by a single pulse (1 msec) was significantly higher than in controls in striatum (A; p < 0.001 for both 0.3 and 2 µM GBR-12909; n = 6-8) and SNc (B; p < 0.05 for pooled data from 0.3 and 2 µM GBR-12909; n = 9) (see Results for details). Data are means ± SEM; the average maximum [DA]_o in control conditions was taken as 100% for each region, indicated by the dashed lines.

The changes in time course could best be seen when the curves were normalized, such that maximum [DA]_o for each region andcondition was set to 100% (Fig. 5). In striatum, the entire responsewas prolonged in a dose-dependent manner: in 0.3 µM GBR plus sulpiride,t_max increased to 670 ± 90 msec (n = 6), with an additional increaseto 1700 ± 110 msec (n = 8) in 2 µM GBR plus sulpiride (Fig. 5A).Similarly, t₅₀ increased to 1980 ± 330 msec in 0.3 µM GBR andto 8500 ± 670 msec in 2 µM GBR. All differences in t_max and t₅₀between control and each GBR concentration were significant (p< 0.001) (Fig. 5A). The changes in [DA]_o time course in SNc weremuch less dramatic than those in striatum, with similar effectsin either 300 nM or 2 µM GBR-12909 plus sulpiride, as noted above.Although there was no change in the rising phase of DA records,the falling phase was clearly prolonged (Fig. 5B). In fact, theslightly higher t_max (3180 ± 410 msec; n = 9) did not differ significantlyfrom control (p > 0.05), whereas the 30% increase in t₅₀ to 8320± 550 msec (n = 9) was significantly later (p < 0.01).

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Figure 5. Normalized evoked [DA]_o curves indicate differences in time course between SNc versus striatum. Average [DA]_o evoked by a single pulse in striatum (A) and SNc (B) in the presence and absence of GBR-12909 (GBR) plus sulpiride (sulp), with the maximum for each condition normalized to 100%. In striatum, both the t_max and t₅₀ of evoked [DA]_o increased significantly in GBR-12909 in a concentration-dependent manner (p < 0.001 for each step compared with control; n = 6-8). Although the t₅₀ in SNc was also increased compared with control (p < 0.01; n = 9 for pooled data from 0.3 and 2 µM GBR-12909), t_max was not altered (p > 0.05). C, When normalized curves for evoked [DA]_o in SNc and striatum in maximally effective GBR-12909 plus sulpiride were superimposed on an expanded time scale, the overall time courses were similar (compare with Fig. 3A), with t₅₀ values that did not differ significantly (p > 0.05). The time to reach maximum [DA]_o, t_max, however, remained significantly longer in the SNc (p < 0.01); dashed lines indicate t_max for each region. Data are normalized means; error bars have been omitted for clarity (see Fig. 4).

With complete blockade of the DAT and D₂ autoreceptors, DA overflow curves from striatum and SNc became much more similar(compare Figs. 3A, 5C), primarily because of the much greaterchanges in DA behavior in striatum. Under these conditions, theinitial rising phases of the curves were similar, and the t₅₀values for the two regions were statistically indistinguishable(p > 0.05). In SNc, however, [DA]_o continued to increase afterthe falling phase in striatum had already begun, so that a differencein t_max between terminal and somatodendritic release persisted(Fig. 5C). The average t_max in striatum (1700 msec) was significantlyearlier than the time to reach maximum in SNc (3180 msec) (p <0.01). Moreover, [DA]_o in SNc also remained near this maximumfor a longer period than in striatum, suggesting more sustainedrelease (Fig. 5C).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present comparative studies of the Ca²⁺ dependence and kinetics of DA release in striatum and SNc offer important new insightsinto both axon terminal and somatodendritic processes. Key resultsinclude demonstration of the dependence of evoked [DA]_o in striatumon [Ca²⁺]_o. These data are consistent with previous results showing thatbasal [DA]_o in DA terminal regions is higher when sampled usingmicrodialysis solutions with elevated Ca²⁺ (Moghaddam and Bunney, 1989). Even more intriguing is the relativeindependence of evoked [DA]_o in SNc on [Ca²⁺]_o. Together with the longer time to reach maximum [DA]_o in SNccompared with striatum, even in the presence of complete DAT andautoreceptor blockade, these data argue for different underlyingmechanisms of axon terminal and somatodendriticrelease.

Previous studies have questioned classical exocytotic release in the substantia nigra on anatomical grounds: synaptic sitesavailable for vesicle fusion are rare. Although dendrodendriticsynapses have been described in the SNc (Wilson et al., 1977),these are primarily absent in the SN pars reticulata (SNr) andthus comprise <1% of synaptic input to DA dendrites (Groves andLinder, 1983). Moreover, depolarization-induced DA release canbe elicited from the SNr in isolation (Geffen et al., 1976; Riceet al., 1994), suggesting that dendrodendritic synapses are notrequired for release. Moreover, the number of vesicles in DA somataand dendrites is small. Whereas vesicles are densely localizedin identified DA terminals in striatum (Nirenberg et al., 1996a,1997), there are few vesicles in DA dendrites SNc (Wilson et al.,1977; Groves and Linder 1983; Nirenberg et al., 1996a), implyinga limited source for exocytotic release (Nirenberg et al., 1996a).However, somatodendritic DA is stored in saccules of smooth endoplasmicreticulum (Mercer et al., 1978; Wassef et al., 1981), as wellas in vesicles (Wilson et al., 1977; Groves and Linder, 1983).Consistent with dual storage sites, the vesicular monoamine transporterVMAT2 is expressed in tuberovesicles that appear to be sacculesof smooth endoplasmic reticulum and, less commonly, in vesicles(Nirenberg et al., 1996b). Whether both storage sites contributeto the releasable pool of DA is unknown. Both sites would be susceptibleto the DA-depleting actions of reserpine, an irreversible inhibitorof VMAT2, which weakens the argument that reserpine sensitivityindicates vesicular release (Heeringa and Abercrombie, 1995).

Differing Ca²⁺ dependence and kinetics of somatodendritic versus terminal release

In contrast to evoked [DA]_o in striatum, which fell below detectable levels in nominally 0 mM Ca²⁺ even when DA uptake and D₂ autoreceptors were blocked, DA releasein SNc persisted in 0 mM Ca²⁺ (Figs. 1, 2), consistent with earlier studies (Hoffman and Gerhardt,1999). Indeed, evoked [DA]_o was half-maximal in 0 mM Ca²⁺. Moreover, evoked DA release from synaptic terminals in striatumcontinued to increase with increasing [Ca²⁺]_o, whereas somatodendritic release was maximal at 1.5 mM Ca²⁺. These data demonstrate a remarkably limited dynamic range forregulation of somatodendritic release of DA by [Ca²⁺]_o (Fig. 2). Somatodendritic release does require Ca²⁺, however, because evoked release can be primarily eliminatedby extended incubation in 0 mM Ca²⁺ plus 1 mM EGTA and then restored when Ca²⁺ is added back to the medium (Rice et al., 1994, 1997). Together,these results suggest that a minimal level of Ca²⁺ entry may trigger somatodendritic DA release by a process thatis distinct from the classical, Ca²⁺-dependent exocytotic release from axon terminals instriatum.

Additional evidence for differing mechanisms comes from the prolonged time course of release in SNc compared with striatum(Fig. 3). It is well established that both evoked and exogenouslyintroduced increases in [DA]_o in striatum are enhanced and prolongedwhen the DAT is inhibited or eliminated (Bull et al., 1990; Kawagoeet al., 1992; Cass et al., 1993; Cragg et al., 1997; Jones etal., 1998) or when D₂ autoreceptors are blocked (Cass and Gerhardt,1994; Cragg and Greenfield, 1997; Hoffman and Gerhardt 1999).Similar, albeit smaller, increases in evoked [DA]_o in SNc havealso been reported after DAT inhibition (Cragg et al., 1997, 2001)or D₂ antagonism (Cragg and Greenfield, 1997; Hoffman and Gerhardt,1999). The effect of these agents on the time course of evoked[DA]_o in SNc had not been describedpreviously.

As anticipated, the effect of GBR-12909 plus sulpiride on [DA]_o time course was much greater in striatum than SNc (Fig. 4),consistent with the higher expression the DAT in striatum (Donnanet al., 1991; Ciliax et al., 1995; Freed et al., 1995); similarregional comparisons of D₂ autoreceptor expression are not available.The main effect on time course is likely to be from DAT inhibition,however. Indeed, the concentration-dependent effects of GBR-12909on [DA]_o time course in striatum in the presence of constant sulpiridelevels were strikingly similar to the effects of graded DAT losson single-pulse-evoked DA overflow in wild-type versus heterozygousand homozygous DAT knock-out mice (Jones et al., 1998). Moreover,previous studies have shown that D₂ receptor antagonism does notalter peak [DA]_o evoked with brief (100 msec), high-frequencystimulation in either striatum or SNc (Cragg and Greenfield, 1997;Chen et al., 2001), reflecting minimal D₂ receptor occupancy andefficacy within this time window (Singer, 1988). Because of knowninteractions between D₂ activation and DAT activity (Meiergerdet al., 1993; Parsons et al., 1993; Cass and Gerhardt, 1994; Wieczorekand Kruk, 1994; Hoffman et al., 1999), however, sulpiride wasincluded with GBR-12909 in the present studies to prevent possiblesynergisticinteractions.

Whereas differences in DA clearance (t₅₀) between striatum and SNc were eliminated when DA uptake and autoreceptor-mediatedsuppression of release were inhibited, a significant differencein t_max remained (Fig. 5C). Because synaptic DA release in striatumpresumably occurs within milliseconds of a stimulus (Garris andWightman, 1995), a t_max of >1 sec presumably reflected the timerequired for diffusion to the electrode from distant sites. Thedifference in t_max between SNc and striatum, however, cannot beexplained by differences in diffusion properties. Although theextracellular volume fraction ( $alpha$ ) is 50% larger in SNc than instriatum (Cragg et al., 2001), this parameter will influence theamplitude of [DA]_o but not its time course. More importantly,the geometric parameter that governs the apparent diffusion coefficientof a substance in tissue, the tortuosity factor $lambda$ , is similarin these regions (Rice and Nicholson, 1991; Cragg et al., 2001)and could not contribute to the twofold difference in t_max.

Implications

In combination, the differences in the Ca²⁺ dependence and time course of DA release in SNc and striatum point to an underlyingdifference in release as well as termination characteristics.The most plausible sources of release differences might be inCa²⁺ entry and/or regulation or in the releasable pool of DA in somataand dendrites versus axon terminals. Indeed, Wilson and Callaway(2000) showed recently that intracellular Ca²⁺ concentration ([Ca²⁺]_i) in DA cells of the SNc builds up slowly during a depolarizingstep induced by current injection and then persists for a secondor more in dendrites and soma when the depolarizing current stops.Time-dependent rather than concentration-dependent Ca²⁺ entry, therefore, might contribute to the relative independenceof evoked [DA]_o in SNc on Ca²⁺ above a certain minimal level. Slow clearance of an increasein [Ca²⁺]_i might also contribute to protracted DA release (Wilson andCallaway, 2000), possibly by facilitating fusion of multiple vesiclesrather than the single vesicle assumed in classic synaptic transmission(Triller and Korn, 1982; Stevens, 1993; Matveev and Wang, 2000)or fusion of additional or alternative structures, such as tuberovesicles,which store DA (Mercer et al., 1978; Wassef et al., 1981; Nirenberget al., 1996b) and conceivably could participate in nonclassicalsomatodendritic release. Release from multiple compartments, i.e.,dendrites and somata (Rice et al., 1994; Jaffe et al., 1998),might also contribute. The behavior of evoked [DA]_o in SNc aftersingle-pulse stimulation is consistent with multiple sources orsites of release. After an initially rapid rise in [DA]_o thatis similar in SNc and striatum (Fig. 5C), the subsequent increasein [DA]_o in SNc is slower and more sustained, such that t_max inSNc occurs after [DA]_o in striatum has already begun to returnto baseline (here by diffusion, because uptake was inhibited)(Fig. 5C).

Regardless of release mechanism, delayed and prolonged increases in [DA]_o in midbrain after a single stimulus have implicationsfor DA as a mediator of volume transmission. In SNc and SNr, DAreceptors on DA cell bodies and dendrites are primarily extrasynaptic(Sesack et al., 1994; Yung et al., 1995; Nirenberg et al., 1996a,1997). Extrasynaptic D₁ receptors are also found on nondopaminergicterminals in these regions (Yung et al., 1995). Physiologicalstudies suggest that somatodendritically released DA acting atthese receptors modulates GABA release from presumed striatonigralGABAergic afferents to SNr (Miyazaki and Lacey, 1998; Radnikowand Misgeld, 1998). Similarly, DA cells in the adjacent ventraltegmental area (VTA) also exhibit somatodendritic release of DA(Iravani et al., 1996; Rice et al., 1997), which can act at extrasynapticreceptors to modulate release of GABA and glutamate in VTA (Cameronand Williams, 1993; Koga and Momiyama, 2000) and which may influenceglutamate-mediated plasticity in VTA neurons (Ungless et al.,2001). Thus, to mediate physiological responses, somatodendriticallyreleased DA relies on extracellular diffusion to reach its sitesof action, which exemplifies volume transmission (Fuxe and Agnati,1991; Rice, 2000). Prolonged somatodendritic release, as shownin the present studies in SNc, combined with limited DA uptakeand D₂ autoreceptor control (Cragg and Greenfield 1997; Cragget al., 1997, 2001), will facilitate DA-mediated volume transmissioninmidbrain.

  FOOTNOTES

Received June 5, 2001; revised July 25, 2001; accepted July 26, 2001.

This study was supported by National Institute of Neurological Disorders and Stroke Grant NS-36362. We appreciate helpfuldiscussions with Dr. M. V.Avshalumov.
Correspondence should be addressed to Dr. M. E. Rice, Department of Physiology and Neuroscience, New York University Schoolof Medicine, 550 First Avenue, New York, NY 10016. E-mail: margaret.rice{at}nyu.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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