Glutamatergic Afferents from the Hippocampus to the Nucleus Accumbens Regulate Activity of Ventral Tegmental Area Dopamine Neurons

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The Journal of Neuroscience, July 1, 2001, 21(13):4915-4922

Glutamatergic Afferents from the Hippocampus to the Nucleus Accumbens Regulate Activity of Ventral Tegmental Area Dopamine Neurons
Stan B. Floresco, Christopher L. Todd, and Anthony A. Grace
Departments of Neuroscience and Psychiatry, University of Pittsburgh, Pittsburgh, Pennsylvania 15260

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Several studies have shown that the mesolimbic dopamine (DA) system is strongly influenced by the ventral subiculum (vSub)of the hippocampus. To examine whether this occurs by activationof DA neuron firing, the effects of chemical stimulation of thevSub on ventral tegmental area (VTA) DA neuron activity were examinedusing extracellular single-unit recordings. Infusions of NMDAinto the vSub increased the number of spontaneously firing DAcells recorded per electrode track, while having no effect onfiring rate or burst firing. This response was abolished by intranucleusaccumbens (NAc) infusions of the glutamate receptor antagonistkynurenic acid. This effect did not involve the prefrontal cortex,because infusions of tetrodotoxin into the prefrontal cortex didnot affect the increase in spontaneously active DA cells. Infusionsof either kynurenic acid into the NAc or tetrodotoxin into thevSub decreased the firing rate and burst firing of DA neuronswithout altering the number of spontaneously active DA neurons.These data show that glutamatergic afferents from the vSub tothe NAc exert a potent excitatory effect on VTA DA neurons, influencingboth DA neuron population activity and the regulation of the firingproperties of these neurons. As a result, dysfunctions in hippocampalcircuitries may contribute to the hyperexcitable state of theDA system that is present inschizophrenia.

Key words: ventral subiculum; ventral tegmental area; nucleus accumbens; NMDA; glutamate; dopamine; rat

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The nucleus accumbens (NAc) is a central component of the basal ganglia that is positioned to integrate signals arising fromlimbic and cortical areas and to modulate motor output relatedto goal-directed behavior (Groenewegen et al., 1991; Mogensonet al., 1993). A prominent, excitatory glutamatergic input tothe medium spiny neurons of the NAc arises from the ventral CA1/subiculum(vSub) region of the hippocampus (Groenewegen et al., 1987; Broget al., 1993), and these inputs are in close apposition to dopaminergicprojections arising from the ventral tegmental area (VTA) (Totterdelland Smith, 1989; Sesack and Pickel, 1990). Electrophysiologicalstudies have demonstrated that mesoaccumbens dopamine (DA) transmissionexerts a powerful neuromodulatory influence over hippocampal inputsto the NAc. Stimulation of the VTA, or direct activation of DAreceptors by exogenous application of DA agents, can either inhibitor facilitate neural activity of NAc neurons driven by hippocampalinput (Yang and Mogenson, 1984, 1986, 1987; DeFrance et al., 1985;Pennartz et al., 1992, 1994; Gonon and Sundstrom, 1996). Moreover,behavioral studies have shown that DA transmission in the NAcalso exerts modulatory control over behaviors that are mediatedby hippocampal-ventral striatal circuits (Burns et al., 1993,1996; Wu and Brudzynski, 1995; Floresco et al., 1996; Bardgettand Henry, 1999; Floresco and Phillips, 1999).

Recent neurochemical studies show that the hippocampus in turn can influence DA release in the ventral striatum. Thus, chemicalor electrical stimulation of the vSub produces robust and sustainedincreases in extracellular DA levels in the NAc (Blaha et al.,1997; Brudzynski and Gibson, 1997; Legault and Wise, 1999; Taepavarapruket al., 2000). However, the mechanisms by which these effectsoccur remain in dispute. The ability to abolish vSub-stimulatedmesoaccumbens DA efflux by blockade of glutamate receptors inthe NAc suggests that these increases in DA release may be mediatedprimarily by glutamate receptor-mediated mechanisms localizedwithin the ventral striatum (Blaha et al., 1997; Taepavarapruket al., 2000). In contrast, Legault et al. (2000) have shown thatthe increase in mesoaccumbens DA after infusion of NMDA into thevSub can be blocked by application of glutamate antagonists inthe VTA. The observation that this increase is accompanied byan increase in DA efflux in the VTA and changes in DA neuron firingsuggests that the vSub may also modulate NAc DA via changes inDA neuronactivity.

One caveat in this analysis is the lack of evidence of a direct projection from the hippocampus to the VTA. As such, it islikely that the modulation of DA cell body activity by the vSuboccurs via a polysynaptic circuit. As noted above, the vSub sendsa dense projection to the NAc (Groenewegen et al., 1987; Broget al., 1993). Moreover, the NAc can influence DA neuron activityby both a direct projection to the VTA and an indirect projectionvia the ventral pallidum (Zahm and Heimer, 1990). The vSub alsosends a projection to the medial prefrontal cortex (mPFC) (Condeet al., 1995), which in turn sends excitatory glutamatergic projectionsto the VTA, although this projection only innervates the mesocorticalDA neurons (Carr and Sesack, 2000). Because of these anatomicalconsiderations, the present study was conducted to assess therole of the vSub in the modulation of firing activity of DA neuronsin the VTA and the neural circuits that mediate these effects.Initial extracellular recording experiments used infusions ofeither NMDA or tetrodotoxin (TTX) into the vSub to assess theeffects of stimulation or inactivation of the vSub on the spontaneousactivity and firing characteristics of DA neurons. Subsequentpharmacological manipulations of the NAc and the mPFC were conductedto elucidate the potential neural pathways by which the vSub wouldinfluence mesolimbic DA neuron activity. Understanding the mechanismsby which the hippocampus may modulate DA cell body activity mayhave important implications for understanding the etiology ofschizophrenia, which has been proposed to be linked to both hippocampaldysfunction and hyperexcitability of the DA system (Bogerts, 1993).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Subjects and surgery. All experiments were performed on male Sprague Dawley rats (Hilltop, Scottsdale, PA). Animal care andsurgical procedures were performed in accordance with the guidelinesoutlined in the National Institutes of Health Guide for the Careand Use of Laboratory Animals and were approved by the InstitutionalAnimal Care and Use Committee of the University of Pittsburgh.Rats weighing between 290 and 450 gm were deeply anesthetizedwith chloral hydrate (400 mg/kg, i.p.) and placed in a stereotaxicapparatus (Narishige, Tokyo, Japan), with the incisor bar setat $-$ 3.3 mm. Core body temperature was monitored by a rectal probeand maintained at 35°C by a thermostatically controlled heatingpad. Supplemental anesthetic was administered intraperitoneallyby constant infusion via a syringe pump (Razel model A-99) ata rate of 10-30 mg · kg¹ · hr¹. In all surgical preparations, the scalp was incised, and holeswere drilled in the skull overlying the VTA and the vSub regionof the hippocampus. All rats were implanted with 23 gauge guidecannulas directed to a location ~2 mm dorsal to the vSub (anteroposterior, $-$ 6.0 mm from bregma; mediolateral, +5.3 mm from the midline; anddorsoventral, 4.0 mm from the dura). Subsets of rats were alsoimplanted with guide cannulas directed ~1 mm dorsal to eitherthe NAc (anteroposterior, +1.4 mm from bregma; mediolateral, 1.3mm from the midline; and dorsoventral, $-$ 6.0 mm from the dura)or the mPFC (anteroposterior, +3.0 mm from bregma; mediolateral,+0.7 mm from the midline; and dorsoventral, $-$ 3.0 mm from thedura).

Drugs and drug microinfusions. NMDA (0.25 and 0.75 µg), TTX (1 µM), the broad-spectrum glutamate receptor antagonist kynurenicacid (10 µg), and Dulbecco's buffer were all obtained from Sigma(St. Louis, MO). NMDA was dissolved in Dulbecco's buffer, TTXwas dissolved in deionized water, and kynurenic acid was dissolvedin one drop of 0.1 M NaOH, to which Dulbecco's buffer was added.The pH of the kynurenic acid solution was then adjusted to ~7.4with 0.1 M HCl. The doses of NMDA used in the present study weresimilar to those used by Legault and Wise (1999), and the doseof kynurenic acid was the same as that used by Blaha et al. (1997).

NMDA or TTX was infused into the vSub through a 30 gauge injection cannula that protruded 2.0 mm past the end of the guide.Infusions were delivered at an injection volume of 0.5 µl over2 min. Subsets of rats received intra-NAc infusions of kynurenicacid at a rate of 1.0 µl over 1 min or intra-mPFC infusions ofTTX at a rate of 0.5 µl over 1 min via an injection cannula thatprotruded 0.8 mm past the end of the guide. In these experiments,infusions into the NAc or the mPFC were administered 3 min beforeinfusions of NMDA into thevSub.

Extracellular recordings and experimental protocol. Extracellular recording microelectrodes were constructed from 2.0-mm-outer-diameterborosilicate glass capillary tubing (WPI) using a vertical micropipettepuller (Narishige). The tips of the electrodes were broken backagainst a glass rod to an ~1 µm tip diameter and filled with 2M NaCl containing 2% Pontamine sky blue dye. The in vitro impedanceof the microelectrodes ranged from 5 to 10 M $Omega$ as measured at 135Hz using a Winston Electronics BL-1000 impedance meter. Afterdrilling a burr hole overlying the VTA, the dura was resected,and the electrode was lowered into the VTA (coordinates, +3.6mm anterior from lambda, 1.0 mm lateral from the midline, and6.5-9 mm ventral from the brain surface) with a hydraulic microdrive(Kopf model 640). The electrode signal was amplified, filtered,and discriminated from noise using a combination amplificationand window discrimination unit for extracellular recording (Fintronics,Orange, CT) and displayed on an oscilloscope (Tektronics, Wilsonville,OR). The data were acquired, stored, and analyzed using custom-designedcomputer software (Neuroscope) running on an Intel-based personalcomputer with a data acquisition board interface (Microstar Laboratories,Bellevue,WA).

Immediately after infusions into the vSub, a recording electrode was lowered into the VTA. The electrophysiological propertiesof spontaneously active DA neurons were sampled in the VTA bymaking six to nine vertical passes of the electrode through theDA cell body region. These tracks were made in a predefined pattern,with each track separated by 200 µm. A typical experiment wouldtake 2-3 hr to complete all nine tracks. DA neurons were identifiedusing established electrophysiological criteria described by Graceand Bunney (1983). Specific electrophysiological characteristicsinclude a slow irregular or bursting discharge pattern, an initialsegment-somatodendritic break in the positive phase, and a long-duration(2-4 msec) biphasic action potential waveform. After an individualDA neuron was isolated, its spontaneous activity was recordedfor 2-3 min. Three parameters of activity were sampled, the firstbeing the number of spontaneously active DA neurons recorded perelectrode track. The validity of this index as a reliable measureof DA neuron activity change has been discussed previously (Westand Grace, 2000). This index has been shown to be reliable andconsistent across animals and across laboratories (Bunney andGrace, 1978; Chiodo and Bunney, 1983; White and Wang, 1983). Furthermore,treatments that increase or decrease the number of spontaneouslyactive DA neurons per electrode track have been shown to provokecorresponding changes in DA efflux (Moore et al., 1998). The othertwo parameters of activity that were sampled were the basal firingrate and the proportion of spikes fired by the DA neurons thatoccurred in bursts. The onset of a burst was defined as the occurrenceof two spikes with an interspike interval <80 msec, and the terminationof a burst was defined as the subsequent occurrence of an interspikeinterval >160 msec (Grace and Bunney, 1983). The percentage ofspikes in bursts (% SIB) was calculated by dividing the numberof spikes occurring in bursts by the total number of spikes occurringin the same period oftime.

Histology. At the end of each experiment, the recording site was marked via iontophoretic ejection of Pontamine sky blue dyefrom the tip of the recording electrode (30 µA constant currentfor 20-30 min). After dye ejection, brains were removed and fixedin formalin for at least 48 hr. The brains were then immersedin phosphate-buffered sucrose solution (25%) until saturated.The tissue was sectioned into 40 µm coronal slices, mounted, andstained with cresyl violet to enable histological determinationof recording electrode and cannula infusionsites.

Data analysis. The number of spontaneously active DA neurons observed per electrode track, the basal firing rates of all DAneurons, and the % SIB were calculated as an average value foreach rat and analyzed using three separate one-way ANOVAs withtreatment group as the between-subjects factor. Multiple comparisonswere made using two-tailed Dunnett's tests. Analyses of the distributionof firing rates and % SIB of all DA neurons across all rats indifferent treatment groups were assessed using Kolmogorov-Smirnovtwo-sampletests.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Histology

The locations of the tips of the cannulas were confirmed to lie within the vSub, the NAc, and the mPFC (Fig. 1). All ratshad infusions that were localized primarily within the ventralCA1 and subicular regions of the ventral hippocampus, with someplacements encroaching on the entorhinal cortex or medial dentategyrus. The data from these rats did not differ from the data ofrats with placements that were exclusively in the vSub. Infusionsof kynurenic acid into the NAc were localized to the medial shellregion, whereas infusions of TTX into the mPFC were localizedto the prelimbic or infralimbic cortex. Both of these regionsreceive a dense projection from the vSub (Brog et al., 1993; Condeet al., 1995).

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Figure 1. Histological verification of all recording and infusion sites in the present study. The location of infusions is shown for all rats receiving the following: A, infusions of 0.75 µg of NMDA (black circles) or TTX (gray squares) into the vSub; B, infusions of kynurenic acid into the NAc (gray circles); or C, infusions of TTX into the mPFC (gray squares). Plates are taken from Paxinos and Watson (1997), and the numbers beside each plate correspond to millimeters from bregma.

Effects of infusions of NMDA or TTX into the vSub on DA neuron activity

Infusions of NMDA into the vSub caused a dramatic increase in the number of DA neurons encountered per electrode track. Afterinfusions of 0.25 µg of NMDA, there was a 60.1% increase in thenumber of spontaneously active DA cells, and infusions of the0.75 µg dose caused a 111.2% increase relative to that of vehicle-treatedanimals. Overall, an infusion of NMDA into the vSub is the mostpotent stimulus for activating silent DA neurons reported todate.

Analysis of the number of spontaneously active DA neurons per electrode track for all treatment groups revealed a significanteffect of treatment (F_(6,35) = 13.64; p < 0.001; Figure 2A). Significanteffects of treatment were also observed with respect to both thebasal firing rate data (F_(6,35) = 4.12; p < 0.005) and the % SIB(F_(6,35) = 3.926; p < 0.005). Dunnett's tests revealed that infusionsof either 0.25 µg (n = 6 rats; 104 neurons) or 0.75 µg (n = 7rats; 162 neurons) of NMDA into the vSub increased the numberof spontaneously active DA neurons per electrode track in a dose-dependentmanner, relative to vehicle treatments (n = 6 rats; 65 neurons)(p < 0.05 and 0.01, respectively; Fig. 2A). Interestingly, thisoccurred without a change in either the mean firing rate or the% SIB (Figs. 3A, 4A, respectively). At least part of this effectmay have been caused by activation of silent DA neurons that displayedactivity at substantially lower firing rates, as suggested bydifferences in the firing rate distribution (Kolmogorov-Smirnovtest, p < 0.01; Fig. 3C). Thus, particularly with the low doseof NMDA, there was an apparent increase in the number of slowlyfiring DA neurons. The apparent lack of increase in slowly firingDA neurons after the 0.75 µg dose of NMDA (compared with the 0.25µg dose) suggests that the higher dose of NMDA may have also increasedthe firing rates of DA neurons that would normally be spontaneouslyactive at a lower firing rate after the lower dose of NMDA. Aseparate analysis revealed that there were no differences in thenumber of spontaneously active DA neurons encountered across allnine tracks (F_(8,24) = 0.87; NS). Thus, stimulation of the vSubexerted a robust excitatory influence on the basal level of DAneuron firing in the VTA, as indicated by the increase in thenumber of spontaneously active DA neurons per electrode trackthat were observed after NMDA infusions into the vSub.

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Figure 2. Infusions of NMDA into the vSub increase DA neuron population activity. A, Activation of the vSub led to a dose-dependent increase in spontaneously active DA neurons. The mean number of spontaneously active DA neurons (+SEM) recorded per electrode track from rats receiving vehicle infusions (n = 6 rats; white bar), 0.25 or 0.75 µg of NMDA (n = 6 rats, 7 rats, respectively; black bars), or TTX (n = 6 rats; gray bar) into the vSub is shown. B, Blockade of glutamate transmission in the NAc prevented the activation of VTA DA neuron firing by vSub stimulation in a manner that was independent of the vSub-mPFC pathway. The mean number of spontaneously active DA neurons (+SEM) recorded per electrode track from rats receiving vehicle infusions (same as A; white bar), infusions of kynurenic acid (Kyn) into the NAc in combination with vehicle infusions into the vSub (n = 6 rats; hatched bar), infusions of kynurenic acid into the NAc in combination with 0.75 µg of NMDA into the vSub (n = 6 rats; cross-hatched bar), or infusions of TTX into the mPFC in combination with 0.75 µg of NMDA into the vSub (n = 5 rats; gray bar) is shown. *p < 0.05 and **p < 0.01 versus control; $dagger$ p < 0.05 versus the group receiving 0.75 µg of NMDA.

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Figure 3. Modulation of DA neuron firing rate by the vSub, the NAc, and the mPFC. A, In contrast to the effects on spontaneous activity, activation of the vSub did not change significantly the VTA DA neuron firing rate. Nonetheless, inactivation of the vSub did decrease VTA DA cell firing. The mean firing rate of DA neurons (+SEM) recorded from rats receiving vehicle infusions (white bar), 0.25 or 0.75 µg of NMDA (black bars), or TTX (gray bar) into the vSub is shown. B, Blockade of glutamate transmission in the NAc attenuates the DA neuron firing rate. The mean firing rate of DA neurons (+SEM) recorded from rats receiving vehicle infusions (same as A; white bar), infusions of kynurenic acid into the NAc in combination with vehicle infusions into the vSub (hatched bar), infusions of kynurenic acid into the NAc in combination with 0.75 µg of NMDA into the vSub (cross-hatched bar), or infusions of TTX into the mPFC in combination with 0.75 µg of NMDA into the vSub (gray bar) is shown. *p < 0.05 and **p < 0.01 versus control. C, Distribution of mean firing rates of all DA neurons recorded from rats receiving vehicle injection (C1), 0.25 µg of NMDA (C2) or 0.75 µg of NMDA (C3) into the vSub, or infusions of TTX into the mPFC in combination with 0.75 µg of NMDA into the vSub (C4) is shown. This suggests that the increase in DA cell spontaneous activity after vSub stimulation may be caused by the activation of slow-firing DA neurons.

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Figure 4. Modulation of DA neuron burst firing by the vSub, the NAc, and the mPFC. A, As with firing rate, activation of the vSub did not cause a significant change in DA cell burst firing, although inactivation of the vSub did attenuate bursting. The mean % SIB of DA neurons (+SEM) recorded from rats receiving vehicle infusions (white bar), 0.25 or 0.75 µg of NMDA (black bars), or TTX (gray bar) into the vSub is shown. B, Similarly, glutamate transmission in the NAc also controls basal levels of burst firing of VTA DA neurons. The mean % SIB of DA neurons (+SEM) recorded from rats receiving vehicle infusions (same as A; white bar), infusions of kynurenic acid into the NAc in combination with vehicle infusions into the vSub (hatched bar), infusions of kynurenic acid into the NAc in combination with 0.75 µg of NMDA into the vSub (cross-hatched bar), or infusions of TTX into the mPFC in combination with 0.75 µg of NMDA into the vSub (gray bar) is shown. *p < 0.05 and **p < 0.01, versus control. C, Distribution of % SIB of all DA neurons recorded from rats receiving vehicle injection (C1) or infusions of TTX into the mPFC in combination with 0.75 µg of NMDA into the vSub (C2) is shown.

In contrast to the effects of NMDA, infusions of TTX into the vSub (n = 6 rats; 37 neurons) caused a trend toward a decreasein the number of spontaneously active DA cells per electrode trackrelative to vehicle treatments, but this difference was not statisticallysignificant (p > 0.10; Fig. 2A). However, infusions of TTX intothe vSub caused a significant decrease in the basal firing ratesof DA neurons (p < 0.05; Fig. 3A) and the % SIB (p < 0.05; Fig.4A). These data show that vSub also exerts a tonic excitatoryinfluence over the firing characteristics of VTA DA neurons, assuggested by the decreases in both the firing rate and burstingactivity of DA neurons observed after inactivation of the vSubbyTTX.

Involvement of the NAc and the mPFC in the regulation of DA neuron activity by the vSub

Although there are no direct projections from the vSub to the VTA, there are several potential pathways via which the vSubcould affect DA neuron firing. Thus, the vSub projects to boththe mPFC and the NAc, which provide direct or indirect afferentsto DA neurons (Brog et al., 1993; Conde et al., 1995). This wasassessed by pharmacological manipulations of each of these systems.Infusions of kynurenic acid into the NAc in combination with vehicleinfusions into the vSub (n = 6 rats; 64 neurons) did not altersignificantly the number of spontaneously active DA neurons perelectrode track (Fig. 2B). However, similar to the effects observedafter TTX infusions into the vSub, administration of kynurenicacid into the NAc reduced both the firing rate (p < 0.01; Fig.3B) and the % SIB (p < 0.01; Fig. 4B) of VTA DAneurons.

Infusions of the glutamate receptor antagonist kynurenic acid into the NAc completely abolished the increase in spontaneouslyactive DA neurons per electrode track induced by infusions of0.75 µg of NMDA into the vSub (n = 6 rats; 68 neurons; Dunnett's,p = 1.0; Fig. 2B). One planned comparison confirmed that infusionsof kynurenic acid into the NAc in combination with NMDA in thevSub resulted in significantly fewer spontaneously active DA neuronscompared with NMDA treatments alone [t(11) = 4.04; p < 0.005].This combination of treatments did not alter significantly eitherthe firing rate (Fig. 3B) or the % SIB (Fig. 4B) of the DA neuronssampled.

In contrast, inactivation of the mPFC by infusions of TTX, in combination with stimulation of the vSub with 0.75 µg of NMDA(n = 5 rats; 75 neurons), did not block the increase in the numberof spontaneously active DA neurons produced by NMDA infusionsinto the vSub (p < 0.05; Fig. 2B). One planned comparison confirmedthat the number of spontaneously active DA neurons observed inthe mPFC TTX and vSub NMDA group did not differ from that withvSub NMDA treatment alone [t(10) = 1.33; p > 0.20, NS]. However,this combination of treatments did reduce significantly the basalfiring rate and the % SIB recorded from DA neurons (p < 0.05).Accordingly, inactivation of the mPFC by TTX resulted in a significantdifference in the distributions of both the firing rate and %SIB of DA neurons (Kolmogorov-Smirnov test, p < 0.01), increasingthe proportion of neurons that displayed firing rates of <3 Hz(Fig. 3C1,C4) and the proportion of neurons that displayed <10%of their spikes in bursts (Fig. 4C1,C2). This supports a rolefor the mPFC in the regulation of basal firing characteristicsof spontaneously active DA neurons and confirms that infusionsof TTX into the mPFC were sufficient to reduce activity in thiscortical region, as indicated by the decrease in firing ratesand burst firing of these neurons. Thus, the increase in DA neuronactivity, induced by NMDA stimulation of the vSub, is mediatedprimarily by glutamate receptor activity in the NAc, but not byneural activity of the mPFC. Moreover, like neural activity inthe vSub, glutamate receptor tone in the NAc exerts a tonic excitatoryinfluence over the firing characteristics of VTA DA neurons, becauseblockade of these receptors decreases both the firing rate andbursting activity of DA neurons, without influencing the numberof spontaneously active DAneurons.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study demonstrates that the vSub exerts a powerful control over the activity of DA neurons in the VTA and doesso via glutamatergic mechanisms localized within the NAc. NMDA-inducedstimulation of the vSub dramatically increased the number of spontaneouslyactive DA neurons per electrode track, which was completely abolishedafter glutamate receptor blockade in the NAc. This effect wasnot mediated by the hippocampal-cortical-accumbens pathway, becauseinfusions of TTX into the mPFC had no effect on the NMDA-inducedincrease in DA neuron population activity. In addition, the vSubalso exerts a tonic influence (i.e., the basal steady-state levelof activity that is present in the absence of vSub activation)over the firing rate and burst firing of VTA DA neurons. Inactivationof the vSub or glutamate receptor blockade in the NAc decreasedboth of these parameters. In view of these data, it is likelythat the changes in mesoaccumbens DA release after chemical stimulationof the vSub (Brudzynski and Gibson, 1997; Legault and Wise, 1999;Legault et al., 2000) may have been mediated, in part, by increasedfiring of VTA DA neurons. It is interesting to note that basalstriatal DA efflux has been shown previously to correlate stronglywith DA neuron population activity but not to correlate with eitherthe average firing rate or burst firing level of individual nigrostriatalDA neurons of drug-naïve rats (Moore et al., 1998).

Neural pathways mediating vSub control of VTA DA neuron population activity

There are several projection pathways that can potentially mediate subicular regulation of VTA DA cell firing. The observationthat infusions of the glutamate receptor antagonist kynurenicacid into the NAc completely abolished the increase in VTA DAneuron population activity suggests that this pathway involvesglutamatergic afferents to GABAergic medium spiny projection neuronsof the NAc. Moreover, the lack of effect of mPFC inactivationon this response suggests that these effects are mediated by adirect vSub-NAc projection (Groenewegen et al., 1987). Anatomicaland electrophysiological studies point to at least two potentialefferent pathways by which the firing activity of NAc projectionneurons could modulate DA cell body activity, the first beinga direct projection from the NAc to the VTA (Zahm and Heimer,1990; Kalivas et al., 1993). However, it is unlikely that thisprojection mediates the increases in DA neuron activity, becausethis projection is primarily GABAergic (Kalivas et al., 1993)and electrophysiological studies have shown that stimulation ofthe NAc evokes short-latency inhibitory responses in VTA neurons(Maeda and Mogenson, 1980).

A more likely route by which activity in the hippocampal-ventral striatal pathway may modulate DA neuron firing is via theventral pallidum (VP). The NAc sends a dense GABA projection tothe VP, and stimulation of either the NAc or its glutamatergicafferents (including the vSub) can inhibit VP neuronal firing(Jones and Mogenson, 1980; Tsai et al., 1985; Yang and Mogenson,1985, 1987; Chrobak and Napier, 1993). In contrast to the mediumspiny neurons of the NAc, the GABAergic output neurons of theVP are characterized by relatively high rates of spontaneous activity(Jones and Mogenson, 1980; Yang and Mogenson, 1985, 1987; Mogensonet al., 1993), thereby exerting a tonic inhibitory influence overefferent structures. The VP can influence DA neural activity viaa direct projection to the VTA (Swanson et al., 1984; Tsai etal., 1985; Zahm and Heimer, 1990; Mogenson et al., 1993). Althoughthe precise mechanisms by which this could alter VTA DA cell activityin the manner observed here are not known at present, one potentialmechanism that may account for these findings is that stimulationof the vSub would have increased firing of GABAergic projectionneurons of the NAc, causing a decrease in VP neural activity.The decrease in VP activity would then be expected to cause areduction of the GABAergic inhibition over the VTA. It is knownthat the spontaneous activity of DA neurons is not dependent onglutamatergic afferents but instead is driven by an endogenouspacemaker conductance (Grace and Bunney, 1983; Grace and Onn,1989; Kitai et al., 1999). Therefore, we propose that the increasein DA neuron population activity may be caused by a release fromVP GABAergic inhibition (Fig. 5). This activation of normallysilent DA neurons may contribute to the increase in slow firing,spontaneously active DA cells observed after NMDA infusions intothe vSub. We are currently performing experiments to evaluatethis hypothesis.

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Figure 5. A model describing the neural circuitries by which the vSub may modulate DA neuron activity. Stimulation of the vSub by infusions of NMDA activates glutamatergic afferents to the NAc. This in turn is proposed to inhibit the activity of neurons in the VP. As a result, there is a removal of tonic inhibition of neurons in the VTA. In this model, we propose that the VP-VTA projection provides sufficient inhibitory influence to hold a subpopulation of DA neurons in an inactive state. Thus, inhibition of VP firing would lead to an increase in the number of VTA DA neurons firing spontaneously. The question mark beside the VP to VTA path indicates that, although this pathway is known to be present in the rat, its involvement in this response remains speculative at the present time.

The present data suggest that the glutamatergic vSub-NAc pathway also plays a role in regulating the firing parameters ofDA neurons. Inactivation of the vSub with TTX or infusions ofkynurenic acid into the NAc decreased both the firing rate and% SIB of DA neurons without decreasing the number of spontaneouslyactive DA neurons. These effects are similar to those observedafter transection of striatal outputs to nigrostriatal DA neurons,which also caused a decrease in firing parameters of A9 DA neurons(Pucak and Grace, 1994). Although the mechanism by which the basalactivity in the vSub projection to the NAc may regulate firingcharacteristics of DA neurons remains unclear at the present time,one possibility is that it may involve outputs from the NAc tothe VP and subsequently to the pedunculopontine tegmental nucleus(PPTg). The VP sends projections to the PPTg (Swanson et al.,1984; Tsai et al., 1985; Zahm and Heimer, 1990; Mogenson et al.,1993), and previous studies have shown that the PPTg exerts excitatorycontrol over both the firing activity of DA neurons (Kelland etal., 1993; Lokwan et al., 1999) and mesoaccumbens DA efflux viaglutamatergic and cholinergic mechanisms in the VTA (Blaha etal., 1996; Forster and Blaha, 2000). Reducing the activity ofNAc neurons, either by TTX in the vSub or kynurenic acid in theNAc, would cause an increase in VP firing. The finding that thesemanipulations also attenuate burst firing, which has been shownto be dependent on glutamatergic afferents in vivo (Overton andClark, 1997; Kitai et al., 1999), suggests that these alterationsmay be caused by increased inhibition of PPTg neurons, which woulddecrease VTA burstfiring.

These data provide further support for the hypothesis that distinct afferent pathways regulate DA cell population activityand firing rate and burst firing of DA neurons (Pucak and Grace,1994). This dual regulation of DA neuron activity may be mediatedby an interplay between glutamate and GABA afferents projectingto DA neurons. Thus, in those DA neurons that are inactive becauseof a hyperpolarization by VP afferents, one would expect littleeffect of glutamate, because (1) glutamate acts primarily on NMDAreceptors on mesolimbic DA neurons (Karreman et al., 1996) and(2) DA neurons hyperpolarized by VP GABAergic afferents wouldbe unresponsive to NMDA receptor stimulation caused by Mg²⁺ blockade (Mayer et al., 1984). Therefore, glutamate afferentswould only be capable of increasing the firing rate and burstfiring of DA neurons that were previously spontaneously active.However, after the DA neurons became spontaneously active viaremoval of the VP GABAergic inhibition (as would be achieved byactivation of the vSub-NAc pathway), the glutamatergic afferentscould then augment their firing rate and burstfiring.

The fact that infusions of TTX into the mPFC did not block the increase in DA neuron population activity induced by infusionsof NMDA into the vSub was not surprising, because the proportionof A10 DA neurons that receive mPFC input represents a minorityof the total neuronal population (Swanson, 1982; Carr and Sesack,2000). Moreover, DA neurons that receive mPFC input do not projectto the NAc but instead send reciprocal projections back to themPFC (Carr and Sesack, 2000). The observed reduction in burstfiring and the firing rate of VTA DA neurons after infusions ofTTX into the mPFC is consistent with a number of studies showingthat cooling or infusions of local anesthetics into the mPFC decreaseburst firing of DA neurons (Svensson and Tung, 1989; Murase etal., 1993), whereas electrical or chemical stimulation of thisregion increases bursting activity by glutamate-dependent mechanisms(Murase et al., 1993; Tong et al., 1996). Taken together, thepresent findings, in addition to previous data, provide importantinsight regarding dissociable mechanisms of hippocampal and corticalregulation of DA neuronactivity.

Modulation of mesoaccumbens DA release by the vSub

The present findings complement previous studies showing that stimulation of the vSub can increase mesoaccumbens DA efflux.Infusions of NMDA into the vSub, similar to those used in thepresent study, produced a substantial increase in NAc DA extracellularlevels (Legault and Wise, 1999; Legault et al., 2000), an effectthat was abolished by reverse dialysis of glutamate receptor antagonistsinto the VTA. This observation complements the present data, inwhich stimulation of hippocampal afferents to the NAc can increasethe population activity of DA neurons, which presumably can enhancemesoaccumbens DA efflux. However, this does not exclude the potentialrole of glutamate-mediated DA release occurring directly in theventral striatum. Thus, blockade of NMDA receptors in the NAcwill block the increase in DA efflux evoked by electrical stimulationof the vSub (Blaha et al., 1997; Taepavarapruk et al., 2000),although NMDA receptors play only a minor role in the glutamate-evokedactivity of NAc neurons (Pennartz et al., 1991; Hu and White,1996). Furthermore, it is known that NMDA receptors are locatedon intervaricose segments of tyrosine hydroxylase-containing neuronalprocesses in the NAc shell (Gracy and Pickel, 1996). Therefore,it is likely that the vSub modulation of DA release in the NAcmay be the result of both a presynaptic mechanism localized withinthe NAc and a polysynaptic mechanism involving the NAc, VP, andVTA. The vSub would thus be in a unique position to regulate boththe tonic and phasic release of DA, the former by presynapticmodulation of DA terminal release (Grace, 1991; Blaha et al.,1997; Taepavarapruk et al., 2000) and the latter by a polysynapticcircuit linking the NAc to the VTA (Zahm and Heimer, 1990; Grace,1991).

Implications for schizophrenia

Dysfunction of the DA system has long been implicated as a primary factor in the pathophysiology of schizophrenia. More recentstudies have suggested that there may be a developmental pathologyof the hippocampus in this disorder (Lipska and Weinberger, 2000),particularly in the ventral regions that project to limbic structures.The present study shows that the vSub is involved in regulatingthe basal firing characteristics as well as the overall activitylevel of VTA DA neurons in the normal rat. If this system is disrupted,particularly early in development, it is likely that tonic controlof VTA DA neuron activity would be affected. Under such conditions,stimuli that cause phasic activation of DA neuron firing may beexpected to have an abnormally large impact on impulse-dependentDA release in limbic structures (Grace, 1991). This could contributeto the heightened DA responsivity observed in rats with developmentaldisruptions of ventral hippocampal circuits (Grace, 2000; Lipskaand Weinberger, 2000).

  FOOTNOTES

Received Jan. 23, 2001; revised April 17, 2001; accepted April 17, 2001.

This work was supported by United States Public Health Service Grants MH 01055, MH 57440, and MH 45156. S.B.F. is a recipientof a Human Frontiers Science Organization postdoctoral fellowship.We thank Drs. Holly Moore and Anthony West for their assistanceand Nicole MacMurdo for her assistance withhistology.
Correspondence should be addressed to Dr. Stan B. Floresco, Department of Neuroscience, University of Pittsburgh, 446 CrawfordHall, Pittsburgh, PA 15260. E-mail: floresco{at}brain.bns.pitt.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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