Properties of Dopamine Release and Uptake in the Songbird Basal Ganglia

doi:10.1152/jn.01053.2004

Properties of Dopamine Release and Uptake in the Songbird Basal Ganglia

Samuel D. Gale¹ and David J. Perkel²

¹Graduate Program in Neurobiology and Behavior and ²Departments of Biology and Otolaryngology, University of Washington, Seattle, Washington

Submitted 6 October 2004; accepted in final form 10 November 2004

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Vocal learning in songbirds requires a basal ganglia circuittermed the anterior forebrain pathway (AFP). The AFP is notrequired for song production, and its role in song learningis not well understood. Like the mammalian striatum, the striatalcomponent of the AFP, Area X, receives dense dopaminergic innervationfrom the midbrain. Since dopamine (DA) clearly plays a crucialrole in basal ganglia–mediated motor control and learningin mammals, it seems likely that DA signaling contributes importantlyto the functions of Area X as well. In this study, we used voltammetricmethods to detect subsecond changes in extracellular DA concentrationto gain better understanding of the properties and regulationof DA release and uptake in Area X. We electrically stimulatedCa²⁺- and action potential–dependent release of an electroactivesubstance in Area X brain slices and identified the substanceas DA by the voltammetric waveform, electrode selectivity, andneurochemical and pharmacological evidence. As in the mammalianstriatum, DA release in Area X is depressed by autoinhibition,and the lifetime of extracellular DA is strongly constrainedby monoamine transporters. These results add to the known physiologicalsimilarities of the mammalian and songbird striatum and supportfurther use of voltammetry in songbirds to investigate the roleof basal ganglia DA in motor learning.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

The neurotransmitter dopamine (DA) plays an important role inthe function of basal ganglia circuits in motor control andlearning. One such circuit is the anterior forebrain pathway(AFP) in songbirds, which is required for song learning in juvenilesand plasticity of adult song but not for song production (Bottjeret al. 1984; Brainard and Doupe 2000; Scharff and Nottebohm1991; Sohrabji et al. 1990; Williams and Mehta 1999). The firstcomponent of the AFP is the basal ganglia nucleus Area X. Likethe mammalian striatum, Area X receives glutamatergic projectionsfrom pallial areas (the premotor nucleus HVC, used as a propername, and the AFP output nucleus the lateral magnocellular nucleusof the anterior nidopallium, LMAN; nomenclature following Reineret al. 2004) and a dense dopaminergic projection from the midbrainventral tegmental area (VTA; Fig. 1; Bottjer 1993; Lewis etal. 1981). The essential role of the AFP in song learning andadult song plasticity and the known functions of basal gangliaDA in motor control and learning in mammals lead to the hypothesisthat DA may play a key part in the song learning process orother functions of Area X. Consistent with an important rolefor DA in information processing in Area X, DA modulates theexcitability of the major cell type (the spiny neuron) in AreaX and also the strength of excitatory synaptic inputs to thesecells (Ding and Perkel 2002, 2004; Ding et al. 2003).

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FIG. 1. Simplified diagram of the song system. HVC (used as a proper name) projects to the robust nucleus of the arcopallium (RA) as part of the motor pathway for song production. HVC also projects to RA indirectly via the anterior forebrain pathway, which includes Area X, the medial portion of the dorsolateral nucleus of the anterior thalamus (DLM), and the lateral magnocellular nucleus of the anterior nidopallium (LMAN). Dopaminergic inputs to Area X originate in the ventral tegmental area (VTA).

In mammals, DA neurons fire spontaneously at a slow rate andtransiently burst in response to salient events such as rewardor reward predicting stimuli (Hyland et al. 2002

; Schultz 1998

).Burst firing enhances accumulation of extracellular DA (Cherguiet al. 1994

) and presumably causes the phasic increases in extracellularDA concentration observed in the striatum of behaving rats (Cheeret al. 2004

; Phillips et al. 2003

; Robinson et al. 2002

; Roitmanet al. 2004

). Ultimately, the dynamics of extracellular DA concentrationdepends critically on local factors that vary among differentregions of the brain: the density of DA release sites, the rateof DA uptake through transporter proteins, and the state ofrelease-regulating neurotransmitter receptors on DA axon terminals.These factors influence whether DA acts via phasic (subsecond)signaling, slower fluctuations and/or by tonic influence onDA receptors.

A method of selectively measuring DA release with subsecondtemporal resolution seems imperative for understanding the propertiesand functions of DA signaling in the songbird basal ganglia.In mammals, such measurements have been achieved in brain slicesand in vivo using voltammetric methods in which endogenouslyreleased DA is oxidized on the surface of a carbon fiber, andthe resulting current is recorded (reviewed in Robinson et al.2003). We applied these techniques to songbirds to determinewhether we could reliably measure DA release in Area X and ifthe factors regulating the extracellular concentration of DAare similar in the mammalian and songbird striatum. From brainslices of Area X, we electrically stimulated Ca²⁺- and actionpotential–dependent release of an electroactive substanceidentified as dopamine by the shape of the voltammetric waveform,electrode selectivity, and by anatomical, neurochemical, andpharmacological evidence. The properties and regulation of DArelease and uptake in Area X are similar to those reported previouslyin the mammalian striatum. These results extend the wealth ofexisting physiological and anatomical evidence for a high degreeof similarity between avian and mammalian basal ganglia andverify that voltammetry will be a useful technique to measureDA release with high temporal resolution in Area X of songbirdsin vivo.

METHODS

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ABSTRACT
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Care of birds and preparation of brain slices

All procedures were approved by the University of WashingtonInstitutional Animal Care and Use Committee. Adult (>90 daysold) male zebra finches were obtained from commercial suppliersand housed in groups of five or fewer on a 13/11-h light/darkcycle. Food and water were available at all times. Brain sliceswere prepared as described in detail by Stark and Perkel (1999).Birds were anesthetized with isoflurane and decapitated. Thebrain was removed and immersed in an ice-cold solution containing(in mM) 119 NaCl, 2.5 KCl, 1.3 MgSO₄, 1 NaH₂PO₄, 16.2 NaHCO₃,2.5 CaCl₂, 11 D-glucose, and 10 HEPES. Coronal or parasagittalslices 300–400 µm thick were cut with a vibratingmicrotome. Slices were stored in artificial cerebrospinal fluid(ACSF), which was made of the same components described abovefor the slicing solution except for replacement of HEPES withan additional 10 mM NaHCO₃. The ACSF was initially $~$ 35°Cwhen the slices were transferred and allowed to cool to roomtemperature. All solutions were continuously bubbled with agas mixture of 95% O₂-5% CO₂. Slices were left for at least1 h before use.

Electrochemical recordings

To construct carbon fiber electrodes (CFEs), a single carbonfiber (15 mm long, 11 µm diam; P-25, Amoco, Tustin, CA)was inserted into the small end of a standard plastic P200 pipettetip. The plastic around the carbon fiber was melted with a heatingcoil in such a way that the pipette tip could be pulled by handto a shank that sealed around the carbon fiber. The exposedcarbon fiber tip was cut to a length of 30–50 µmby hand with a scalpel blade. The electrode was filled with2 M KCl.

For recordings, slices were submerged in a small, illuminatedchamber and perfused (2–3 ml/min) with ACSF warmed to32°C. The borders of Area X were clearly visible througha dissecting microscope. The tip of the CFE was gently loweredinto the slice to a depth of 50–150 µm. A bipolar,stainless steel stimulating electrode was inserted about 100µm from the CFE. DA release was elicited by single 0.1-msshocks (60–70 V amplitude) controlled by a stimulus isolationunit (Isoflex, AMPI, Jerusalem, Israel). Signals were amplifiedwith a MultiClamp 700A amplifier in voltage-clamp mode and digitizedwith a Digidata 1322A (Axon Instruments, Foster City, CA). Theelectrode potential, stimulation, and data acquisition werecontrolled using Clampex 9.0 software (Axon Instruments). Forconstant potential amperometry (CPA), the CFE was held at +0.4V; signals were low-pass filtered at 100 Hz and sampled at 10kHz. For fast-scan cyclic voltammetry (FCV), the CFE was heldat –0.4 V and a triangular waveform (–0.4 to 1 Vand back at 300 V/s, a total of 9.33 ms) was applied every 100ms (10 Hz); signals were low-pass filtered at 2 kHz and sampledat 20 kHz. Background-subtracted cyclic voltammograms (current-voltageplots) were made by subtracting the average of the current recordedfor 10 voltammetric scans (1 s) prior to stimulation from thecurrent recorded for each voltammetric scan after stimulation.Changes in DA concentration were quantified by plotting thepeak oxidation current (converted to DA concentration as describedbelow) of the voltammograms corresponding to each 100 ms-spacedtime-point after stimulation. Data were analyzed and plottedusing Clampfit 9.0 (Axon Instruments) and IGOR (Wave Metrics,Lake Oswego, OR).

CFEs were calibrated (at the end of a day of experiments) toconvert current to approximate DA concentration. The CFE tipwas carefully lowered into the end of the glass tube (1.1 mmID) from which fresh ACSF perfused the slice. A 5-s "pulse"of 1–5 µM DA or norepinephrine (NE) dissolved inoxygenated ACSF was allowed to pass through the perfusion tubingand over the CFE, and the current change was recorded with CPAor FCV. CPA calibration without attempting to mimic the extracellularascorbic acid concentration in brain tissue typically underestimatesthe sensitivity of the electrode by an order of magnitude (Kawagoeand Wightman 1994; Schmitz et al. 2001; Venton et al. 2002).Therefore only the peak oxidation current measured with FCVwas used to estimate DA concentration in this paper, and CPAmeasurements are reported in units of current. Our CFEs wereabout three times more sensitive to DA than NE.

Slices were stimulated once every 2.5 min to allow full recoveryfrom paired-pulse depression (see RESULTS and DISCUSSION). Drugs(diluted to their final concentration in the ACSF perfusingthe slice chamber) were applied after the peak amplitude ofthe signal was stable for at least three consecutive stimulations.

For comparisons of peak DA release and decay time constant amongArea X, medial striatum (MSt), and lateral striatum (LSt), DArelease was recorded at 13 locations in the striatum of eachparasagittal slice. Area X was divided into four quadrants togive four of the locations. Six locations were in the MSt outsideof Area X (2 anterior, 1 ventral, and 3 posterior to Area X).Three locations were dorsal but not anterior to the globus pallidusand considered to be in the LSt. The CFE and stimulating electrodeswere positioned at each location (in pseudorandom order) andDA release was evoked by single shock stimulation as describedabove. The peak amplitude of DA release and decay time constantwere determined from a single trace taken after the amplitudewas stable for three consecutive stimulations (as describedfor drug experiments above). The values of peak DA release anddecay time constant at each location within a region (Area X,MSt, and LSt) were averaged to obtain a single value for eachregion in the slice. These are the values plotted and used forstatistical analysis. DA uptake in the mammalian striatum ismodeled according to Michaelis-Menten kinetics to determinethe maximum rate of uptake (V_max). However, we do not know thevalue of K_m (binding affinity) for the DA transporter in birdsor even whether just a single transporter contributes to DAdecay in the zebra finch striatum. We instead fit the latterpart of the decay phase (beginning at the concentration reachedat the location with the smallest amplitude of DA release) toa single exponential to determine the decay time constant (seeFig. 5A).

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FIG. 5. A: example FCV recordings from Area X (circles), MSt outside of Area X (triangles), and LSt (squares). Stimulation occurred at 1 s. Latter parts of the decay phase are fit to a single exponential (shown with solid lines) beginning at the same concentration (see METHODS). B: peak DA release in the Area X, medial striatum (MSt), and lateral striatum (LSt) are plotted as open circles and are connected by lines for measurements made in the same slice (n = 8). Mean value for each area is indicated by an open bar. Error bars represent SE. C: decay time constants in Area X, MSt, and LSt plotted as in B.

Measurement of monoamine tissue content

For tissue content measurements, a 400- to 500-µm-thickcoronal slice within the anterior and posterior borders of AreaX was prepared as described above. While the slice was stillimmersed in the ice-cold slicing solution, a square piece oftissue within the medial-lateral and dorsal-ventral bordersof Area X was dissected with a sharp scalpel under a dissectingmicroscope. The dissected piece of tissue was transferred toa plastic tube and frozen on dry ice. A similar-sized pieceof tissue was cut from the pallium dorsal to Area X in the sameslice. Tissue samples remained frozen at –80°C oron dry ice until analyzed for monoamine content. Monoamine levelswere measured by HPLC with electrochemical detection at theNeurochemistry Core Lab in Vanderbilt University's Center forMolecular Neuroscience (http://www.mc.vanderbilt.edu/root/vumc.php?site=neurosci&doc=697)and are reported as amount of monoamine (ng) per amount of totalprotein (mg) in the tissue sample.

Statistics

Prism 3.0 (Graph Pad Software, San Diego, CA) was used for statisticaltesting with the tests indicated in RESULTS and DISCUSSION.All tests were two-tailed. P < 0.05 was considered significant.Values of n for a given experiment indicate number of slices,and no more than two slices from a single bird were used forthe same type of experiment.

Drugs

Atropine, baclofen, carbachol, CdCl₂, clonidine, desipramine,DA, fluvoxamine, GBR-12935, mecamylamine, nicotine, nomifensine,NE, pargyline, quinpirole, TTX, and yohimbine were purchasedfrom Sigma (St. Louis, MO). (1S,3R)-1-aminocyclopentane-1,3-dicarboxylicacid (APCD), (RS)-3,5-dihydroxyphenylglycine (DHPG), maprotiline,pilocarpine, and sulpiride were purchased from Tocris (Ellisville,MO).

RESULTS AND DISCUSSION

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

Measurement and identification of synaptic DA release

A single shock from a stimulating electrode positioned neara CFE held at constant potential (0.4 V) in Area X reliablycaused a rapid rise in current well above noise that generallydecayed back to baseline in <1 s (Fig. 2A). No response wasobserved when the CFE was held at 0 V. Similar events recordedwith FCV revealed a background-subtracted voltammogram (current-voltagecurve) similar to the voltammogram obtained from DA or NE dissolvedin ACSF (Fig. 2B, inset). The current at the peak oxidationpotential measured with FCV changed with a time course similarto the current change measured with CPA (Fig. 2B). However,the time to peak and the decay of the FCV signal were slightlyslower than those of the CPA signal because of adsorption ofanalyte to the CFE between FCV scans (Bath et al. 2000; Ventonet al. 2002).

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FIG. 2. Examples of dopamine (DA) release measured after single-shock stimulation in Area X slices with constant potential amperometry (CPA) (A) and fast-scan cyclic voltammetry (FCV) (B). Stimulation occurred at 1 s. Example cyclic voltammograms are shown in the inset of B for DA release in Area X (solid line) and for exogenous DA during calibration (dashed line).

The shape of the voltammogram strongly suggested we were measuringrelease of DA and/or NE (DA and NE produce very similar voltammograms).In mammals, it is commonly assumed that CFEs solely measureDA, and not NE, release in the striatum because CFEs are aboutthree times more sensitive to DA than NE (see METHODS) and thedensity of DA innervation and DA tissue content are much greaterthan those of NE in the striatum (DA:NE content is 100:1 inthe caudate and 10:1 in the nucleus accumbens of rats; Garriset al. 1993

; Kuhr et al. 1986

). Similarly, in zebra finches,the tyrosine hydroxylase (TH; the rate-limiting enzyme in thesynthesis of both DA and NE) positive fibers that project heavilyto Area X originate from cell bodies in VTA that are TH positivebut not positive for dopamine- ${beta}$ -hydroxylase (D ${beta}$ H; an enzyme involvedin conversion of DA to NE and thus a marker of noradrenergicneurons), and lesions of VTA completely abolish catecholaminehistofluorescence in Area X (Bottjer 1993

; Lewis et al. 1981

;Mello et al. 1998

). D ${beta}$ H-positive fibers are sparse in Area Xand surrounding striatal areas (Mello et al. 1998

). We directlymeasured monoamine content in tissue homogenate from Area Xand from pallium located dorsal to Area X (a region with muchlighter TH immunostaining) using liquid chromatography. Levelsof NE, serotonin (5-hydroxytryptamine, or 5-HT), and the 5-HTmetabolite 5-hydroxyindole-3-acetic acid (5-HIAA) were not significantlydifferent in Area X and pallium (P > 0.4, paired t-test),whereas, as expected, levels of DA and its metabolites dihydroxyphenylaceticacid (DOPAC) and homovanillic acid (HVA) were significantlygreater in Area X than in pallium (P < 0.05; Fig. 3). DAwas on average 40 times more abundant than NE in Area X (P <0.0001, paired t-test; Fig. 3). This result is qualitativelythe same as that of Harding et al. (1998)

, who found DA wasabout five times more abundant than NE in Area X in 90-day oldzebra finches (the difference in absolute amounts of DA andNE measured here and by Harding et al. might be due to differencesin release and metabolism of catecholamines while handling thebird or during tissue collection). Thus the zebra finch striatumseems to receive, like the striatum of mammals and other birds(Reiner et al. 1994

), a very dense DA innervation and a relativelysparse noradrenergic innervation. Although tissue content isonly a measure of what may potentially be released by localstimulation in brain slices (for instance, it does not distinguishbetween neurotransmitter in the releasable pool of vesiclesversus storage pools; Garris and Wightman 1994

), the highersensitivity of CFEs for DA than NE, anatomical data, and relativeamounts of DA and NE contained in Area X suggest that the CPAand FCV signals resulting from electrical stimulation in AreaX are a measure of DA release and that NE is unlikely to makemore than a small contribution to these signals.

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FIG. 3. Mean tissue content of DA, NE, 5-HT, and the metabolites DOPAC, HVA, and 5-HIAA from Area X (solid bars) and pallium located dorsal to Area X (open bars) from 6 adult zebra finches. Error bars represent SE.

To ask whether the DA release we evoked is dependent on actionpotentials and Ca²⁺ entry, we used CPA to measure the peak amplitudeof DA release after blocking action potentials with TTX (2 µM),preventing Ca²⁺ entry by removing Ca²⁺ from the ACSF bathingthe slice, or blocking voltage-gated Ca²⁺ channels with Cd²⁺ions (100 µM CdCl₂). TTX (n = 6), removal of extracellularCa²⁺ (n = 6), or Cd²⁺ (n = 3) all significantly reduced thepeak amplitude of evoked DA release by 80–100% (P <0.001, t-test), and the effects of Ca²⁺ removal and Cd²⁺ wereat least partially reversible (Fig. 4). Thus, in Area X as inmammalian striatal slices, local electrical stimulation elicitsCa²⁺- and action potential–dependent release of DA.

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FIG. 4. A: example of an experiment showing effect of removing extracellular Ca²⁺ (0 Ca²⁺) or applying TTX on DA release. B: CPA traces from the time-points indicated in A. Stimulation occurred at 1 s. C: inhibition of DA release in all experiments with TTX (n = 6), 0 Ca²⁺ (n = 6), and Cd²⁺ (n = 3).

Regional comparison of DA release and uptake in the avian striatum

The peak DA concentration measured at the CFE depends on thedensity of DA release sites, the amount of DA released at eachsite, and the distance DA diffuses from each release site (largelycontrolled by the rate of DA uptake through transporters). PeakDA release and the rate of DA uptake thus reflect importantproperties of DA signaling and vary across different regionsof the mammalian brain. For instance, in rats, peak DA releaseis greater and DA uptake rate faster by an order of magnitudein the striatum than in the prefrontal cortex and amygdala (Garrisand Wightman 1994). Also, in both the rodent and primate striatum,peak DA release tends to be greater and uptake faster in "motor"compared with "limbic" striatal subregions (Cragg 2003; Cragget al. 2000, 2002; Garris and Wightman 1994; Jones et al. 1995,1996). To determine whether peak DA release and the kineticsof DA uptake are different among Area X and other parts of zebrafinch striatum, we recorded DA release in response to a singleshock in three different regions of the striatum (Area X, MStoutside of Area X, and LSt) in parasagittal slices (n = 8; seeMETHODS). FCV was used so that we could compare peak releaseamplitude in terms of estimated concentration (see METHODS).To compare rate of DA uptake, we fit the latter part of thedecay phase to a single exponential and measured the time constant(see METHODS and Fig. 5A). Peak DA concentration after a singleshock varied from about 0.5 to 2.5 µM (similar to concentrationsobserved in mammalian striatal slices) and was significantlygreater in Area X than MSt and LSt (P < 0.05, repeated measuresANOVA and Tukey's multiple comparisons test; Fig. 5B). Thisis consistent with the greater intensity of TH-expressing fibers(and thus probably denser release sites) in Area X than surroundingstriatum in adult zebra finches (Soha et al. 1996). Greaterfiber density might also result in a greater density of monoaminetransporters and thus faster uptake of DA in Area X, but thedecay time constant was not significantly different among AreaX, MSt, and LSt (P = 0.38, repeated measures ANOVA; Fig. 5C).

Regulation of DA uptake through monoamine transporters

In mammals, DA is rapidly diluted as it diffuses from the releasesite, and thereafter, the time and distance DA travels and interactswith receptors is heavily influenced by the rate of uptake viathe DA transporter (DAT) (Cragg and Rice 2004). To assay theinfluence of monoamine transporters on DA transmission in AreaX, we measured (with CPA) the half-life (time to 50% decay)of DA released by a single shock in the presence of monoamineuptake transporter inhibitors. The DAT inhibitors GBR-12935(GBR; 5 µM, n = 6) and nomifensine (5 µM, n = 5)increased the half-life of DA released in Area X by over 350%,indicating that DA transmission is tightly controlled by uptakethrough the DAT in Area X (both effects P < 0.05, t-test;Fig. 6). Surprisingly, the NE transporter (NET) inhibitors desipramine(1 µM, n = 6) and maprotiline (10 µM, n = 5) atconcentrations that are specific to NET in mammals also substantiallyincreased the half-life of DA released in Area X (by over 800and 300%, respectively; both effects P < 0.01, t-test; Fig. 6).

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FIG. 6. A: example CPA traces before and after applying the DA transporter (DAT) inhibitor GBR. Stimulation occurred at 1 s. B: time course of the effect of GBR averaged over 6 experiments. Error bars represent SE. C: change in half-life of released DA after application of GBR (n = 6), desipramine [Dsp, n = 6, NE transporter (NET) inhibitor], GBR and desipramine (n = 5), maprotiline (Mpr, n = 5, NET inhibitor), GBR and maprotiline (n = 5), nomifensine (Nmf, n = 5, DAT inhibitor), fluvoxamine (Flv, n = 5, SERT inhibitor), and pargyline (Parg, n = 3, MAO-B inhibitor). Individual experiments are plotted with circles. Mean for each group is shown with an open bar, and error bars represent SE. Dashed line indicates 100%.

Expression of DAT or NET is specific to the cells that synthesizeand release the corresponding neurotransmitter in mammals; however,both DAT and NET can transport either catecholamine (reviewedin Torres et al. 2003

). The NET (located on NE-releasing axons)has a significant role in the uptake of DA in the rat prefrontalcortex, where DA innervation is sparse compared with the striatumand DAT expression is low (Moron et al. 2002

; Mundorf et al.2001

; Sesack et al. 1998

). The NET does not contribute to DAuptake in the mammalian striatum (Cragg 2003

; Cragg et al. 2000

,2002

; Jones et al. 1995

, 1996

). Even in the nucleus accumbensshell, where there is moderate NE innervation and expressionof NET and where DAT expression is less dense compared withthe dorsal striatum and nucleus accumbens core, NET inhibitorsdo not affect DA uptake in normal or DAT knock-out mice (Berridgeet al. 1997

; Budygin et al. 2002

; Delfs et al. 1998

; Nirenberget al. 1997

; Schroeter et al. 2000

). Hence, the possibilitythat NET located on NE axons contributes strongly to DA uptakein Area X seems unlikely given the very high-density of DA fiberscompared with NE fibers. Another possibility is that DA axonsin Area X express two transporters—one pharmacologicallyDAT-like and the other NET-like—that both contribute significantlyto DA uptake. If either of the possibilities stated above weretrue, the combination of a DAT inhibitor and NET inhibitor mighthave greater effect on DA half-life in Area X than either ofthe drugs alone. Co-application of GBR and desipramine (n =5) or GBR and maprotiline (n = 5) had no further effect on DAhalf-life than desipramine or maprotiline alone (P = 0.28 andP = 0.93, respectively, unpaired t-test; Fig. 6), suggestinginstead that both types of drugs (DAT and NET inhibitors) acton the zebra finch DAT. These results show that the spatialand temporal influence of DA in Area X, as in the mammalianstriatum, are strongly restricted by the action of DA transporters.

The 5-HT transporter (SERT) inhibitor fluvoxamine (5 µM,n = 5) and the monoamine oxidase (MAO-B) inhibitor pargyline(20 µM, n = 3) had no effect on DA half-life in Area X(P = 0.86 and 0.53, respectively, t-test; Fig. 6). This is consistentwith our other evidence (most importantly, the shape of thevoltammogram) that 5-HT and DOPAC do not contribute to our CPAand FCV measurements and shows that SERT and MAO-B are not involvedin the rapid decay of extracellular DA in Area X.

Control of DA release by presynaptic neurotransmitter receptors

In mammals, extracellular DA inhibits its own release by bindingto D2 receptors on DA axon terminals. We tested the effect ofthe D2 agonist quinpirole (10 µM) and D2 antagonist sulpiride(10 µM) on the peak amplitude of DA release in Area Xrecorded with CPA. Since DA can activate ${alpha}$ 2 noradrenergic receptors(Cornil et al. 2002; Zhang et al. 1999) and ${alpha}$ 2 receptor agonistsreduce DA release in the mammalian striatum (Trendelenburg etal. 1994; Yavich et al. 1997), we also tested the possibilitythat ${alpha}$ 2 receptors can act as release-regulating autoreceptorson DA terminals in Area X using the ${alpha}$ 2 receptor agonist clonidine(10 µM) and antagonist yohimbine (10 µM). Quinpiroledecreased DA release by $~$ 50% (n = 5, P < 0.0001, t-test; Fig. 7).The effect of quinpirole was significantly reduced by sulpiride(n = 5; P < 0.001, 1-way ANOVA with Tukey's multiple comparisonstest) and was not affected by yohimbine (n = 3, P > 0.05,same test); a small (<10%) but significant effect of quinpiroleon DA release persisted in the presence of sulpiride (n = 5,P < 0.001, t-test). Sulpiride itself increased DA releaseby $~$ 35% (n = 7, P < 0.01, t-test), suggesting that D2 receptorsare tonically active and inhibiting DA release in our slicepreparation. Tonic D2 activation in our slice preparation mightbe the result of constitutive DA release that is independentof the activity of DA cell bodies, which were not present inour slices. Clonidine decreased DA release by $~$ 25% (n = 6, P< 0.001, t-test). The effect of clonidine was blocked byyohimbine (n = 3, P < 0.01, 1-way ANOVA with Tukey's multiplecomparisons test) but not by sulpiride (n = 3, P > 0.05).The block of clonidine by yohimbine was complete (n = 3, P =0.38, t-test). Yohimbine alone had no effect on DA release inArea X (n = 6, P = 0.56, t-test).

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FIG. 7. A: average time course of the effects of quinpirole (D2 agonist, open circles, n = 5), sulpiride (D2 antagonist, open squares, n = 7), clonidine ( ${alpha}$ 2 agonist, filled circles, n = 6), and yohimbine ( ${alpha}$ 2 antagonist, filled squares, n = 6). Error bars indicate SE. B: change in peak amplitude of DA release after application of sulpiride (Slp, n = 7), quinpirole (Qnp, n = 5), quinpirole in the presence of sulpiride (n = 5), quinpirole in the presence of yohimbine (Yhm, n = 3), yohimbine (n = 6), clonidine (Cln, n = 6), clonidine in the presence of yohimbine (n = 3), and clonidine in the presence of sulpiride (n = 3). Individual experiments are plotted with circles. Mean for each group is shown with an open bar.

These results indicate that DA release in Area X is inhibitedby activation of D2 and ${alpha}$ 2 receptors. To determine whether endogenouslyreleased DA can activate these receptors and inhibit furtherDA release (autoinhibition), we measured (with CPA) the ratioof the peak amplitude of DA release caused by single shocksseparated by short time intervals (the paired-pulse ratio, orPPR) in normal conditions and in the presence of sulpiride oryohimbine at the same recording position. For intervals closeenough that the second release event occurred during the decayof DA released from the first shock, the amplitude of the secondrelease event was determined by subtracting the record of DArelease caused by a single pulse from the two-pulse record (Cragg2003

; Phillips et al. 2002

). In control conditions, there wasa time-dependent paired-pulse depression (PPD) of DA releasein Area X (maximum $~$ 80% depression at 1 s; Fig. 8, A and B).Sulpiride (n = 5) or yohimbine (n = 5) partially decreased themagnitude of PPD (sulpiride 3 times more so than yohimbine),suggesting that DA release in Area X inhibits its own releaseby activating D2 and, more modestly, ${alpha}$ 2 receptors. The effectof sulpiride on the PPR was significant (P < 0.05, pairedt-test) for the intervals from 0.1 and 3 s, and that of yohimbinefor the intervals from 0.05 to 1 s. To determine the time courseand magnitude of autoinhibition mediated by D2 and ${alpha}$ 2 receptors,we subtracted the PPR measured for each interpulse intervalunder control conditions from the PPR at the same intervalsmeasured after sulpiride or yohimbine application (Fig. 8C).D2 receptor–mediated autoinhibition was activated within50 ms of the first stimulation pulse, reached a maximum at 500ms (accounting for $≤$ 30% of the PPD), and terminated by about5 s after the initial pulse. The time course and magnitude ofD2-mediated autoinhibition measured in Area X slices are similarto measurements in mammalian striatal slices (Phillips et al.2002

). Autoinhibition mediated by ${alpha}$ 2 receptors in Area X followeda similar time course but was weaker (accounting for no morethan 10% of the PPD) and shorter lasting (<2 s). The differencein the magnitudes of the D2 and ${alpha}$ 2 receptor–mediated effectscould be due to receptor numbers, efficiency of activation byDA, and intracellular signaling pathways used. The relativemagnitude of the effect of evoked DA release on D2 and ${alpha}$ 2 receptorsis also influenced by the fact that D2 receptors are alreadypartially activated in the slice, whereas ${alpha}$ 2 receptors are not(Fig. 7).

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FIG. 8. A: paired-pulse ratio (PPR) of peak amplitude of DA release for various interpulse intervals in control conditions (filled circles) and (at the same recording position) in the presence of the D2 receptor antagonist sulpiride (open circles; n = 5). Error bars represent SE. Inset: example traces of DA release in response to paired stimulation (1-s interpulse interval) in the presence and absence of sulpiride. B: same as A except showing the PPR in control conditions (filled circles; different experiments from those in A) and in the presence of the ${alpha}$ 2 receptor antagonist yohimbine (open circles; n = 5). C: time course of D2 (filled circles) and ${alpha}$ 2 (open circles) receptor-mediated autoinhibition of DA release. Each point represents the PPR in control conditions subtracted from the PPR in the presence of drug. Error bars represent SE.

What is the origin of the substantial D2/ ${alpha}$ 2-independent componentof the PPD? Release of other neurotransmitters besides DA bythe first shock might contribute to time-dependent depressionof subsequent DA release. Glutamate, GABA, and acetylcholine(ACh) can all modulate DA release in the mammalian striatum(Avshalumov et al. 2003

; Rice and Cragg 2004

; Schmitz et al.2002

; Zhang and Sulzer 2003

, 2004

; Zhou et al. 2001

). Nicotine(10 µM, n = 3), the nicotinic receptor antagonist mecamylamine(10 µM, n = 7), the muscarinic receptor agonist pilocarpine(30 µM, n = 3) and antagonist atropine (20 µM, n= 4), and the nonspecific cholinergic agonist carbachol (20–100µM, n = 6) all had no effect on the amplitude of DA releasedby a single shock in Area X (data not shown). Although spontaneouslyactive cholinergic interneurons are present in brain slicesof Area X (Carrillo and Doupe 2004

; Farries and Perkel 2002

),these results suggest that, unlike in mammals (Zhou et al. 2001

),DA release is not regulated by tonic ACh release in Area X.However, these experiments do not definitively rule out thepossibility that release-regulating nicotinic ACh receptorsare present on DA axons in Area X. The group 1 metabotropicglutamate receptor (mGluR) agonist DHPG (100 µM, n = 5),the groups 1 and 2 mGluR agonist ACPD (100 µM, n = 6),and the GABA_B receptor agonist baclofen (30 µM, n = 7)significantly reduced the amplitude of DA released by a singleshock in Area X by 40 ± 9% (SD), 28 ± 11%, and22 ± 11%, respectively (P < 0.01, t-test; data notshown). Activation of mGluR, GABA_B, or other receptors by endogenousneurotransmitter might contribute to the observed PPD. A portionof the autoinhibition-independent PPD might also be due to depletionof docked vesicles at DA synapses after local stimulation inbrain slices. The slow, autoinhibition-independent PPD is lesspronounced in vivo in mammals (Benoit Marand et al. 2001

; Montagueet al. 2004

; Schmitz et al. 2003

Summary and conclusions

We have shown that electrical stimulation in Area X from adultzebra finches results in Ca²⁺- and action potential–dependentrelease of a substance identifiable as DA by the following electrochemical,anatomical, and pharmacological evidence.

1) The shape of the voltammogram obtained with FCV after electricalstimulation in Area X is identical to that of exogenous DA andknown to be unique to DA and NE.

2) The CFEs used are three times more sensitive to DA than NE.

3) Area X receives a rich projection from neurons in VTA thatsynthesize DA but not NE.

4) The tissue content of DA is about 40 times more abundantthan NE in Area X.

5) The half-life of the released substance is dramatically increasedby drugs known to block the uptake of DA through proteins thattransport DA.

6) The released substance inhibits its own release by activatingD2 DA receptors with a time course similar to that of D2 receptor–mediatedautoinhibition of DA release in mammalian striatal slices.

The factors shown to regulate release and uptake of DA in AreaX are very similar to those reported for the mammalian striatum,suggesting a common functional design for DA neurotransmissionin mammalian and songbird basal ganglia. Mammalian DA neuronsspontaneously fire action potentials at a slow rate in vivo;uptake and tonic depression of release by D2 autoreceptors helpset the steady-state extracellular concentration of DA in thestriatum. During burst firing, DA released at short interspikeintervals accumulates faster than uptake can remove it, resultingin a phasic increase in extracellular DA that reaches fartherfrom the release site, has an increased probability of activatinglow-affinity receptors, and transiently reduces (via autoinhibition)subsequent DA release by the slow, tonic discharge of DA neurons.This amplification of extracellular DA in the striatum mightbe important for effectively transmitting the phasic signalrepresented by burst firing of DA neurons.

The temporal dynamics and function of DA signaling in behavingsongbirds are not known. The results presented here lend confidenceto the possibility of using voltammetry to measure changes inextracellular DA concentration with subsecond temporal resolutionin Area X in vivo, although even more caution will be requiredin interpreting the identity of catecholamines contributingto voltammetric signals in vivo. Since DA plays such an importantrole in mammalian basal ganglia function, knowing the conditionsthat cause DA release and the cellular effects of DA in AreaX will likely contribute to understanding how the AFP functionsin songbirds, which may in turn prove useful as a model of basalganglia function in general.

GRANTS

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ABSTRACT
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

This work was supported by National Institute of Mental HealthGrant MH-066128 and a National Science Foundation Graduate Fellowship.

ACKNOWLEDGMENTS

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS AND DISCUSSION
GRANTS
ACKNOWLEDGMENTS
REFERENCES

We thank D.-S. Koh and B. Hille for help with making carbonfiber electrodes, P. Phillips for advice on voltammetry, andP. Phillips and A. Person for comments on previous versionsof this paper.

FOOTNOTES

The costs of publication of this article were defrayed in partby the payment of page charges. The article must therefore behereby marked "advertisement" in accordance with 18 U.S.C. Section1734 solely to indicate this fact.

Address for reprint requests and other correspondence: Samuel D. Gale, Univ. of Washington, Dept. of Otolaryngology, Box 356515, Seattle, WA 98195 (E-mail: samgale{at}u.washington.edu)

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