Inhibition of Mitochondrial Complex II Induces a Long-Term Potentiation of NMDA-Mediated Synaptic Excitation in the Striatum Requiring Endogenous Dopamine

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The Journal of Neuroscience, July 15, 2001, 21(14):5110-5120

Inhibition of Mitochondrial Complex II Induces a Long-Term Potentiation of NMDA-Mediated Synaptic Excitation in the Striatum Requiring Endogenous Dopamine
Paolo Calabresi¹^,², Paolo Gubellini¹^,³, Barbara Picconi¹^,², Diego Centonze¹^,², Antonio Pisani¹^,², Paola Bonsi¹^,², Paul Greengard⁴, Robert A. Hipskind⁵, Emiliana Borrelli⁶, and Giorgio Bernardi¹^,²
¹ Clinica Neurologica, Dipartimento di Neuroscienze, Università di "Tor Vergata," Rome 00133, Italy, ² Fondazione Santa Lucia IRCCS, Rome 00179, Italy, ³ Istituto di Neuroscienze e Medicina Molecolare, Consiglio Nazionale delle Ricerche, Rome 00133, Italy, ⁴ Laboratory of Molecular and Cellular Neuroscience, Rockefeller University, New York 10021, New York, ⁵ Institut de Génétique Moléculaire, Centre National de la Recherche Scientifique (CNRS)-Unité Mixte de Recherche 5535, Montpellier 34293, France, and ⁶ Institut de Génétique et de Biologie Moléculaire et Cellulaire, CNRS-Institut National de la Santé et de la Recherche Médicale-ULP, CU de Strasbourg 67404, France

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Abnormal involuntary movements and cognitive impairment represent the classical clinical symptoms of Huntington's disease(HD). This genetic disorder involves degeneration of striatalspiny neurons, but not striatal large cholinergic interneurons,and corresponds to a marked decrease in the activity of mitochondrialcomplex II [succinate dehydrogenase (SD)] in the brains of HDpatients. Here we have examined the possibility that SD inhibitorsexert their toxic action by increasing glutamatergic transmission.We report that SD inhibitors such as 3-nitroproprionic acid (3-NP),but not an inhibitor of mitochondrial complex I, produce a long-termpotentiation of the NMDA-mediated synaptic excitation (3-NP-LTP)in striatal spiny neurons. In contrast, these inhibitors had noeffect on excitatory synaptic transmission in striatal cholinergicinterneurons and pyramidal cortical neurons. 3-NP-LTP involvesincreased intracellular calcium and activation of the mitogen-activatedprotein kinase extracellular signal-regulated kinase and is criticallydependent on endogenous dopamine acting via D2 receptors, whereasit is negatively regulated by D1 receptors. Thus 3-NP-LTP mightplay a key role in the regional and cell type-specific neuronaldeath observed inHD.

Key words: D2 dopamine receptors; Huntington's disease; striatum; succinate dehydrogenase; synaptic plasticity; excitotoxicity

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Huntington's disease (HD) is an autosomal dominant neurodegenerative disorder that typically afflicts individuals in midlife(Price et al., 1998; Reddy et al., 1999). The symptoms includeinvoluntary choreiform movements, psychiatric disturbances, anddementia. The primary brain region affected in HD is the striatum:neuronal loss and glial proliferation are seen at early stagesof this disease, and they progress during the course of illness.In this pathological condition striatal spiny neurons are selectivelylost, whereas large cholinergic interneurons are spared (Ferranteet al., 1985).

Recently, electrophysiological experiments have demonstrated that striatal spiny neurons show an enhanced sensitivity to theNMDA receptor activation in transgenic and knock-in mouse modelsof HD (Levine et al., 1999). Interestingly, these mice did notshow differences in sensitivity to AMPA or kainate. These observationssuggest a selective relationship between the genetic alterationunderlying HD and NMDA receptor function. Accordingly, an abnormalNMDA-mediated synaptic function has been observed in hippocampalslices obtained from a YAC mouse model for HD (Hodgson et al.,1999).

One characteristic of HD is an expanded glutamine stretch in the protein encoded by the HD locus. However, mutated Huntingtinprotein has yet to be directly linked to bioenergetic defectsand excitotoxic mechanisms, two pathological events that seemto play a major role in HD (Browne et al., 1997). In fact, thecorticostriatal projection represents one of the major glutamatergicpathways in the brain (Graybiel, 1995; Calabresi et al., 1996a),and an abnormal release of glutamate from this pathway seems toplay a pathogenic role in HD (Greene and Greenamyre, 1996; Greeneet al., 1998). Interestingly, an impaired complex II mitochondrialactivity is a prominent metabolic alteration in HD (Gu et al.,1996). Accordingly, accidental or experimental systemic administrationof the irreversible SD inhibitor 3-nitropropionic acid (3-NP)mimics the pathology of this genetic disorder in rats, nonhumanprimates, and humans (Ludolph et al., 1991; Wullner et al., 1994;Palfi et al., 1996). Furthermore, the reversible complex II inhibitormalonic acid produces similar effects (Greene et al., 1993). Thus,enhanced glutamatergic transmission may trigger neurodegenerationin postsynaptic neurons, the energy metabolism of which is compromisedbecause of impaired SD activity (Greene and Greenamyre, 1996).

Using corticostriatal brain slice preparations (Calabresi et al., 1998), we have studied the electrophysiological effectsof the pharmacological blockade of SD by either 3-NP or methylmalonicacid (MMA), another rather selective inhibitor of SD (McLaughlinet al., 1998), on glutamatergic EPSPs. Here we demonstrate thatendogenous dopamine (DA) is required to produce a long-term enhancementof NMDA-mediated glutamatergic transmission in striatal spinyneurons but not in striatal cholinergic interneurons or corticalpyramidal neurons. Our data suggest that a synaptic mechanismmight possibly underlie cell type-specific neuronal vulnerabilityinHD.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiological experiments. Corticostriatal coronal slices 270 µm thick were prepared from adult Wistar rats and miceand kept in saline solution containing (in mM): 126 NaCl, 2.5KCl, 1.2 MgCl₂, 1.2 NaH₂PO₄, 2.4 CaCl₂, 11 glucose, and 25 NaHCO₃)at 35°C gassed with 95% O₂/5% CO₂. The pH of the bathing solutionwas 7.4. Intracellular recording electrodes (30-60 M $Omega$ ) were filledwith 2 M KCl. An AxoClamp 2B amplifier was used to monitor thecellular activity, which was displayed and stored by a digitalsystem. In single-electrode voltage-clamp mode, the switchingfrequency was 3 kHz. The head-stage signal was monitored continuouslyon a separate oscilloscope. In some experiments, 100 mM BAPTAwas added to the pipette solution to buffer intracellular calcium.In other experiments, 50 mM QX-314, a lidocaine derivative thatblocks action potential discharge without affecting excitatorysynaptic potentials (Calabresi et al., 1994), was used to blockaction potential discharge during current-induced membrane depolarizationof the recorded neurons. Striatal spiny neurons and striatal cholinergicinterneurons were distinguished by their electrophysiological,morphological, and immunohistochemical characteristics as describedpreviously (Kawaguchi et al., 1995; Calabresi et al., 2000). Theelectrophysiological characteristics of prefrontal and frontalcortical neurons have been described previously (Siniscalchi etal., 1997).

For synaptic stimulation, bipolar electrodes were used and were located in the white matter between cortex and striatum, whenrecordings were performed from striatal neurons. Conversely, thestimulating electrode was placed close (0.5-3 mm) to the recordingelectrode in the direction of deep cortical layers when recordingswere made from cortical pyramidal neurons (Calabresi et al., 1996b).The stimulation frequency was 0.1 Hz. Usually the intensity ofstimulation to monitor EPSP amplitude was adjusted to producesynaptic potentials with amplitudes ranging between 5 and 10 mV.Quantitative data on EPSP modifications are means ± SEM expressedas percentage of EPSP amplitude at the onset of drug administration(t = 0). Student's t test (for paired and unpaired observations)was used to compare EPSP amplitude before and after pharmacologicaltreatments.

Combined electrophysiological and optical recordings. A single slice was transferred into a recording chamber, mounted onthe stage of an upright microscope (Axioskop FS, Zeiss) equippedwith a 60×, 0.90 numerical aperture (NA) water immersion objective(LUMPlan FI, Olympus), and fully submerged in a continuously flowingKrebs' solution (33°C, 3 ml/min) gassed with 95% O₂/5% CO₂. Thetip of sharp microelectrodes was filled with 1 mM bis-fura-2 (hexapotassiumsalt; Molecular Probes, The Netherlands) in 200 mM KCl. The shankof the electrode was backfilled with a 2 M KCl solution. Aftercell impalement, cells were loaded with bis-fura-2 by injecting0.1-0.5 nA negative current through the recording pipette. Electroderesistance dropped from initial values of 120-150 to 35-45 M $Omega$ .Fluorescence of bis-fura-2 was elicited by a 75 W Xenon lamp bandpass-filteredat 340 and 380 nm. Emission light was filtered (500 nm) and thendetected by a charge-coupled device camera (Photonic Science).Pairs of 340 and 380 nm images were acquired at intervals of 3-6sec. Analysis of the data was performed off-line [IonVision (ImproVision)and Microcal Origin 4.1 (Microcal Software), running on PowerMac8100 and on a PC, respectively]. Pairs of 340 and 380 nm imageswere background subtracted where backgrounds were regions freeof dye fluorescence, and ratio images were obtained. Levels ofintracellular calcium concentration are expressed as ratio values(ranging from 0.4 to 0.8).

Drugs. Drugs were applied by dissolving them to the desired final concentration in the saline Ringer's solution and by switchingthe perfusion from control saline to drug-containing saline. Inaddition, slices were incubated in 30 µM bicuculline to avoidcontamination of glutamatergic EPSPs by depolarizing GABA-mediatedpotentials. The pH of the Ringer's solution containing 3-NP orMMA was adjusted to 7.4 with NaOH. AMPA, D( $-$ )-2-amino-5-phosphonopentanoicacid (APV), 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX), SCH 23390,L-sulpiride, and forskolin were from Tocris Cookson. Quinpirole,SKF 38393, and PD 98059 were from RBI (Natick, MA). BAPTA, bicuculline,nifedipine, 3-NP, NMDA, MMA, and tetrodotoxin (TTX) were fromSigma (St. Louis, MO), and UO126 was from Alexis. Intracellularapplication of 100 µM H89 for a period lasting at least 20 minafter the beginning of the recordings did not significantly changeeither the amplitude or the time course of EPSPs, the membranepotential, or the input resistance of the neurons (p > 0.05 forall the measuredparameters).

Preparation of 6-OHDA-denervated rats and D2 KO mice. To obtain unilateral nigrostriatal lesions, rats (anesthetized with45 mg/kg body weight pentobarbitone, i.p.) were injected with6-OHDA (8 µg/4 µl of saline containing 0.1% ascorbic acid) viaa Hamilton syringe through a cannula inserted just rostral tothe substantia nigra using stereotaxic coordinates (Paxinos andWatson, 1986). Twenty days later, the rats were tested with apomorphine(0.5 mg/kg, s.c.), and contralateral turns were recorded withautomatic rotometers for 3 hr. Only those rats that consistentlymade at least 200 contralateral turns were used for the electrophysiologicalstudies. Rats were anesthetized with diethyl ether, and braindissection confirmed that the nigrostriatal pathway was lesioned.This was established by the observation of a >95% loss of DA neuronsin the substantia nigra compacta, and the almost complete absenceof DA terminals in the striatum. This was monitored by using amonoclonal antibody for tyrosine hydroxylase (Calabresi et al.,1993b; Centonze et al., 1999).

The generation of mice lacking D2 receptors has been reported previously (Baik et al., 1995). The intrinsic and synaptic membraneproperties of neurons recorded from D2 lacking striatal sliceswere similar to those recorded from wild-type (WT) mice and controlrats, as reported previously (Calabresi et al., 1997).

Biochemical experiments. Corticostriatal slices (270 µm) were prepared as described above. Slices were maintained in salineRinger's solution and where appropriate preincubated for 15 minwith 10 µM PD98059 in DMSO or 0.1% DMSO alone. Slices were stimulatedwith 100 µM 3-NP or 100 µM 3-NP plus 1 µM L-sulpiride for 15 min,after which the striatum was rapidly homogenized using a microfugetube pestle in 40 µl of extraction buffer (10 mM Tris-HCl, 1%Triton X-100, 50 mM NaCl, 50 mM NaF, 5 µM ZnCl₂, 30 mM sodiumpyrophosphate, 1 mM DTT, titrated to pH 7.05, with freshly addedprotease and phosphatase inhibitors) (Hipskind et al., 1994).Insoluble proteins were removed by centrifugation at 10,000 ×g, 15 min, 4°C, and supernatant proteins were immediately denaturedin 50 mM Tris-HCl, pH 6.8, 2% SDS, 2% glycerol, 1% 2-mercaptoethanol.Western blots containing 8 µg of extract protein per lane wereimmunodetected as described (Bowler et al., 1999) using antiseraspecific for the activated forms of mitogen-activated protein(MAP) kinase and ERKs 1 and 2 activated by phosphorylation onThr 202 and Tyr 204 (Cell Signaling Technology), as well as controlantisera directed against ERKs 1 and 2 (CST). The complexes werevisualized with Renaissance ECL (NEN Life Science Products) andexposure to Kodak XAR-5 film after incubation with HRP-coupledsecondary antibodies. The immunoblot results were confirmed bypull-down kinase assays using the same extracts and recombinantglutathione S-transferase-Elk_308-428.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiology of 3-NP and MMA

In striatal spiny neurons, AMPA receptor-mediated EPSPs were elicited by electrical stimulation of adjacent cortex at a physiologicalconcentration of external magnesium (1.2 mM) and in the presenceof 50 µM APV, an NMDA receptor antagonist. Conversely, NMDA receptor-mediatedEPSPs were evoked in the absence of external magnesium and inthe presence of 10 µM CNQX, an AMPA receptor antagonist (Calabresiet al., 1996a). Interestingly, these NMDA-mediated potentialswere greatly enhanced by a 20 min bath application of 100 µM 3-NP(n = 55; p < 0.001) or 300 µM MMA (n = 46; p < 0.001), whereasthe AMPA-mediated EPSPs were unaffected (3-NP: n = 28, p > 0.05;MMA: n = 24, p > 0.05) (Fig. 1a,b). The potentiation induced by3-NP was dose dependent: in the presence of 10 µM 3-NP (n = 5),the NMDA-mediated EPSP was increased to 131 ± 12% of the controlvalue, whereas in the presence of 30 and 300 µM 3-NP (n = 4 foreach concentration), this synaptic potential was 195 ± 24 and246 ± 16%, respectively, of the control value (data not shown).The toxin-induced potentiation measured in spiny neurons persistedafter the washout of both drugs (Fig. 1a,b). In 10 striatal spinyneurons, the long-lasting recordings allowed us to follow the3-NP-LTP for >60 min after toxin washout. In similar experimentalconditions, we observed that the MMA-induced potentiation lastedfor >60 min (n = 7). In contrast to the results obtained withspiny neurons, striatal large cholinergic interneurons (n = 7;p > 0.05 for both 3-NP and MMA) and cortical pyramidal neurons(n = 5, p > 0.05 for 3-NP; n = 3, p > 0.05 for MMA) showed nochange of NMDA-mediated EPSP amplitude after SD inhibition (Fig.2). Similarly, AMPA-mediated EPSPs of both striatal cholinergicinterneurons (n = 6, p > 0.05 for 3-NP; n = 5, p > 0.05 for MMA)and prefrontal and frontal cortical pyramidal cells (n = 3; p> 0.05 for both 3-NP and MMA) were unaffected by this treatment(Fig. 2).

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Figure 1. Inhibition of mitochondrial complex II but not complex I activity induces LTP in striatal spiny neurons. In spiny neurons, 3-NP enhanced the amplitude of NMDA-mediated corticostriatal EPSPs (in 0 mM Mg plus CNQX), whereas AMPA-mediated potentials (in 1.2 mM Mg plus APV) were unaffected. Traces on the right are an average of four single EPSPs (a). The effect of 3-NP was mimicked by MMA (b). Conversely, rotenone failed to affect either component of excitatory synaptic transmission (c). Calibration in a also applies to b and c. In all the experiments, the resting membrane potential of the recorded cells (dotted lines) was constant and ranged between $-$ 84 and $-$ 86 mV.

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Figure 2. Striatal cholinergic interneurons and cortical pyramidal neurons do not show 3-NP-LTP. In cholinergic interneurons, 3-NP did not enhance the amplitude of either NMDA- or AMPA-mediated corticostriatal EPSPs (a). Resting membrane potential = $-$ 60 mV. Similar lack of effects was observed in cortical pyramidal neurons (b). Resting membrane potential = $-$ 72 mV.

Glutamate NMDA receptors mediated the increase in EPSP amplitude, because APV fully suppressed the EPSPs after 3-NP-LTP inductionin spiny neurons (n = 10) (Fig. 3a). Prolonged application of3-NP in the millimolar range depolarizes cultured neurons (Greeneet al., 1998). In our experiments, the membrane potential of spinyneurons under control conditions ( $-$ 85 ± 5 mV; n = 155) was unaffectedby either 100 µM 3-NP ( $-$ 86 ± 6 mV; n = 97; p > 0.05) or 300 µMMMA ( $-$ 85 ± 5 mV; n = 29; p > 0.05). These toxins also did notaffect the resting input resistance (control: 39 ± 8 M $Omega$ , n = 95;3-NP: 40 ± 9 M $Omega$ , n = 55; MMA: 38 ± 8 M $Omega$ , n = 25) (p > 0.05). Similarly,resting membrane potential (control: $-$ 60 ± 4 mV, n = 14; 3-NP: $-$ 61 ± 5 mV, n = 10; MMA: $-$ 58 ± 4 mV, n = 7; p > 0.05) and apparentinput resistance (control: 158 ± 42 M $Omega$ , n = 14; 3-NP: 163 ± 38M $Omega$ , n = 9; MMA: 153 ± 40 M $Omega$ , n = 5; p > 0.05) of large cholinergicinterneurons were not significantly altered by these toxins. 3-NPand MMA also failed to affect the resting membrane potential (control: $-$ 77 ± 4 mV, n = 14; 3-NP: $-$ 77 ± 3 mV, n = 10; MMA: $-$ 78 ± 5 mV,n = 7; p > 0.05), and input resistance (control: 88 ± 38 M $Omega$ , n= 14; 3-NP: 89 ± 40 M $Omega$ , n = 9; MMA: 87 ± 34 M $Omega$ , n = 5; p > 0.05)of prefrontal and frontal cortical pyramidal neurons (Siniscalchiet al., 1997).

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Figure 3. 3-NP-LTP is caused by enhanced NMDA receptor-mediated synaptic transmission and requires intracellular calcium elevation. Cortically evoked EPSPs after the induction of 3-NP-LTP in spiny neurons were fully suppressed by the NMDA receptor antagonist APV (a). Intracellular injection of the calcium chelator BAPTA fully prevented 3-NP-LTP. Conversely, this form of synaptic plasticity was prevented neither by 10 µM nifedipine nor by 100 nM pirenzepine (b).

Rotenone does not induce LTP

To test whether the potentiation of the NMDA-mediated component of excitatory transmission recorded from spiny neurons wasselectively induced by pharmacological inhibition of mitochondrialcomplex II activity or could also be achieved by the inhibitionof other mitochondrial complexes, we incubated the slices in thepresence of rotenone, a selective inhibitor of mitochondrial complexI (Betarbet et al., 2000; Luetjens et al., 2000). Bath application(20 min) of 1 µM rotenone failed to affect either the NMDA- orthe AMPA-mediated striatal EPSPs recorded from spiny neurons (n= 8 for both experimental conditions) (Fig. 1c). We also testedthe effects of a higher concentration of this toxin: 3 µM rotenoneproduced a slow and irreversible membrane depolarization of striatalspiny neurons, which was not coupled, however, to a significantincrease in NMDA-mediated EPSP amplitude (n = 5; data notshown).

Effects of intracellular BAPTA and nifedipine on 3-NP-LTP

The integrity of mitochondrial function is crucial for cytosolic calcium homeostasis (Berridge, 1998). Thus, disruption ofmitochondrial activity by SD inhibitors results in a disregulationof calcium buffering mechanisms (Murphy et al., 1999). To testwhether increased intracellular calcium is critical for 3-NP-LTP,as has been found for physiological striatal synaptic plasticity(Calabresi et al., 1993a), we used recording electrodes filledwith the calcium chelator BAPTA (100 mM). This treatment completelyprevented 3-NP-LTP (n = 10; p > 0.05) (Fig. 3b). To test the possibleinvolvement of high-voltage activated L-type calcium channels,which have been shown to contribute to the potentiation of NMDAresponses induced in spiny neurons by D1 receptor activation (Cepedaet al., 1998), we tested the ability of nifedipine (10 µM, 10min bath application; n = 6) to influence 3-NP-LTP. As shown inFigure 3b, this blocker failed to affect the amplitude and durationof this form of synaptic plasticity. Moreover, 10 µM nifedipinealso failed to alter the amplitude and duration of control striatalEPSPs (n = 6; data not shown). Conversely, this concentrationof nifedipine significantly reduced the duration of calcium-dependentplateau potentials recorded after blockade of potassium channelsfrom striatal spiny neurons (Stefani et al., 1995). We also testedthe possibility that acetylcholine, an endogenous neurotransmitterthat increases intracellular calcium via M1 muscarinic receptorsand favors striatal post-tetanic LTP (Calabresi et al., 1999),might also be involved in the formation of 3-NP-LTP. This possibilityis unlikely, because 100 nM pirenzepine, an M1-like receptor antagonist,failed to affect 3-NP-LTP (n = 4; p > 0.05) (Fig. 3b).

3-NP-LTP is expressed only when the neurons are in the "up" state

Membrane potential of striatal spiny neurons recorded in intact animals oscillates between a hyperpolarized "down" state anda more depolarized "up" state, the latter being determined byconverging excitatory synaptic inputs from the cortex (Stern etal., 1998). During the "up" state, the membrane potential of spinyneurons reaches a level (approximately $-$ 55 mV) capable of relievingthe voltage-dependent magnesium blockade of the NMDA receptorchannel. In the presence of a physiological concentration of magnesium(1.2 mM), membrane depolarization to $-$ 55 mV produced by intracellularinjection of positive current reveals a component of synapticpotential that undergoes a long-term enhancement after SD inhibition(n = 10) (Fig. 4a). In these experiments, 50 mM QX-314, a lidocainederivative that blocks voltage-dependent sodium channels withoutaffecting excitatory synaptic potentials (Calabresi et al., 1994),was used to block action potential discharge during current-inducedmembrane depolarization of the recorded neurons. APV (30 µM) significantlyreduced the duration of EPSPs recorded at $-$ 55 mV and fully preventedthe potentiation induced by 3-NP (n = 5) (Fig. 4b). Conversely,the EPSPs recorded in the same neurons at resting membrane potential(down state, $-$ 85 mV) did not show 3-NP-induced potentiation andwere insensitive to NMDA receptor antagonism. Thus, mitochondrialinhibition and prolonged cortical discharge, which lead to thegeneration of the up state of the neuron, may also cooperate toinduce 3-NP-LTP in vivo.

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Figure 4. 3-NP-LTP is expressed when striatal neurons are in the up state. In the presence of physiological concentrations of external magnesium, 3-NP enhanced EPSPs recorded from neurons depolarized to $-$ 55 mV by intracellular injection of positive current ("up" state), but not EPSPs recorded at resting membrane potentials ( $-$ 85 mV; "down" state) (a). Note that the data represented in a were obtained by shifting the membrane potential of each single neuron from the up to the down state and vice versa throughout the duration of 10 electrophysiological experiments. This experimental protocol was followed to test whether the induction of 3-NP-LTP on the up state EPSP also influenced the AMPA component of the EPSP as detected in the down state. The NMDA receptor antagonist APV fully prevented the formation of 3-NP-LTP observed in the up state (b). Traces in the bottom part represent examples of EPSPs recorded from two different spiny neurons in the absence (a) and presence (b) of APV at different membrane potential levels.

Effects of 3-NP and MMA on postsynaptic responses induced by application of AMPA and NMDA

We also investigated whether application of SD inhibitors could affect postsynaptic responses induced by application of AMPAand NMDA in spiny neurons and cholinergic interneurons. As shownpreviously (Calabresi et al., 1998), brief (20-60 sec) bath applicationsof these agonists induced inward currents in both of these neuronalsubtypes. In the presence of 1 µM TTX, bath application of either3-NP (30 µM; n = 9) or MMA (300 µM; n = 8) enhanced the inwardcurrents induced by NMDA (p < 0.001) but not those caused by AMPA(p > 0.05) in spiny neurons (Fig. 5a,b). Conversely, 3-NP (n =6; p > 0.05) (Fig. 5c) and MMA (n = 6; p > 0.05; data not shown)failed to alter agonist-induced inward currents recorded fromstriatal cholinergic interneurons.

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Figure 5. SD inhibitors enhance inward currents induced by bath application of NMDA in striatal spiny neurons but not in cholinergic interneurons. In spiny neurons, bath application of 3-NP significantly enhanced the inward current evoked by application of NMDA but not of AMPA (a). A single experiment obtained from a striatal spiny neuron voltage clamped at $-$ 80 mV is shown (b). The effect of 3-NP was mimicked by MMA (c). Application of 3-NP failed to affect NMDA- and AMPA-mediated currents in striatal cholinergic interneurons (d).

Microfluorimetric measurements of intracellular calcium changes after 3-NP

In the presence of TTX (1 µM), under the control condition, bath application of NMDA (30 µM, 1 min) elicited a membrane depolarizationcoupled to a transient and reversible elevation in intracellularcalcium (Fig. 6). After pretreatment with 100 µM 3-NP (20 min),no significant change in resting membrane potential was observed,whereas the intracellular calcium level was moderately but significantlyincreased (n = 7; p < 0.05) (Fig. 6). In these conditions, NMDAevoked a marked membrane depolarization up to threefold higherthan in controls that slowly returned to resting values. Afterthe onset of this depolarization, intracellular calcium concentrationsincreased steadily, reaching a peak at the washout of NMDA (n= 7; p < 0.001). After a rapid decrease from this peak, however,the intracellular calcium level remained elevated and generallyreturned to basal levels only 10-15 min after the wash of theagonist (Fig. 6).

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Figure 6. 3-NP enhances basal and NMDA-induced intracellular calcium concentration in striatal spiny neurons. The histogram shows the mean percentage of increase ± SEM of intracellular calcium (expressed as ratio values) in response to NMDA, 3-NP alone, and NMDA in the presence of 3-NP (a). The traces in the top panel show the membrane depolarization induced by NMDA (30 µM) in the control condition (left) and after 20 min of 3-NP treatment (right). The bottom panel shows the simultaneous measurements of intracellular calcium levels in the same neuron (b). Resting membrane potential = $-$ 84 mV. *p < 0.05; **p < 0.01; ***p < 0.001 (Student's t test for paired observations).

Role of endogenous dopamine

The pathologic alterations found in HD, as well as those induced by inhibitors of SD, are selective for the striatum (Ferranteet al., 1985). The reason for this regional specificity is unknown.A unique feature of the striatum, compared with other brain areas,is the massive dopaminergic innervation arising from the substantianigra (Graybiel, 1995). Endogenous DA and energy metabolism impairmentcaused by mitochondrial alteration might cooperatively producethe neuronal damage induced by 3-NP in the striatum by favoring3-NP-LTP induction. Accordingly, we found that 3-NP-LTP was absentin slices obtained from rats in which the striatum was DA-depletedby homolateral nigral injection of 6-OHDA (n = 15). Conversely,slices obtained from the contralateral intact side expressed 3-NP-LTP(Fig. 7a) (n = 11). In DA-denervated slices, 3-NP-LTP was restoredby previous application (15 min) of 3 µM quinpirole (n = 8), aD2-like DA receptor agonist, but not by 10 µM SKF 38393 (n = 9),a D1-like DA receptor agonist (Fig. 7b). These results suggestedthat activation of D2- but not D1-like DA receptors is requiredfor the induction of 3-NP-LTP. It is worth noting that DA denervationdid not affect the resting membrane potential ( $-$ 86 ± 5 mV; n =12) and the input resistance (38 ± 8 M $Omega$ ; n = 12) of striatal spinyneurons.

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Figure 7. Endogenous DA controls the formation of 3-NP-LTP through the activation of D2 DA receptors. 3-NP-LTP was abolished in slices obtained from DA-depleted striata, whereas it was normally expressed in tissue obtained from intact contralateral striata (a). Quinpirole, a D2-like DA receptor agonist, but not SKF 38393, a D1-like DA receptor agonist, restored 3-NP-LTP in DA-denervated neurons (b). 3-NP-LTP was blocked by L-sulpiride, a D2-like DA receptor antagonist, but not by SCH 23390, a D1-like DA receptor antagonist (c). 3-NP-LTP was also prevented by forskolin, an adenylyl cyclase activator, and by SKF 38393, a D1-like DA receptor agonist (d). Intracellular application of the PKA inhibitor H89 partially prevented the inhibitory effects of L-sulpiride and forskolin on 3-NP-LTP formation (e). 3-NP-LTP was absent in striatal neurons recorded from mice lacking D2 receptors but not in WT animals. Intracellular injection of H89 partially restored 3-NP-LTP in mice lacking D2 (f). Note that in this latter graph data obtained from WT mice were significantly different from both D2 knock-out (KO) mice (p < 0.01) and D2 KO mice plus H89 (p < 0.001). Moreover, a statistical significance (p < 0.001) was detected between D2 KO mice and D2 KO mice plus intracellular H89.

To further evaluate the potential roles of D1- and D2-like receptors in 3-NP-LTP induction, slices prepared from control ratswere incubated in 1 µM L-sulpiride (n = 27; p > 0.05), a D2-likeDA receptor antagonist, or 10 µM SCH 23390 (n = 25; p < 0.001),a D1-like DA receptor antagonist. L-sulpiride, but not SCH 23390,fully prevented 3-NP-LTP (Fig. 7c). Notably, L-sulpiride was unableto block 3-NP-LTP when applied after its induction (n = 8; p <0.001), demonstrating that striatal DA is required for the inductionbut not for the maintenance of this phenomenon (data not shown).In the presence of endogenous DA, the blockade of D2-like DA receptorsresults in an increased activity of adenylyl cyclase. A similareffect is achieved by the stimulation of D1-like receptors byexogenous agonists (Jaber et al., 1996; Vallone et al., 2000).Accordingly, the inhibitory effect of L-sulpiride on 3-NP-LTPformation was mimicked by incubation of the slices in 30 µM forskolin(n = 14), an activator of adenylyl cyclase, or 10 µM SKF 38393(n = 12) (Fig. 7d), indicating that high cAMP levels prevent inductionof 3-NP-LTP and that the stimulation of D1-like receptors providesa negative modulation of the D2-like receptor-mediated 3-NP-LTPformation. Neither forskolin (n = 3) nor SKF 38393 (n = 4) affected3-NP-LTP when applied after its induction (data not shown). Becausethe available pharmacological tools do not distinguish betweenthe subtypes composing the D2-like DA receptor family (D2, D3,and D4), we used mice lacking D2 DA receptors (Baik et al., 1995).Corticostriatal slices prepared from these mice failed to show3-NP-LTP (n = 6), whereas slices from WT animals showed 3-NP-LTP(n = 7) (Fig. 7f), thereby confirming an essential role for D2receptors in this process. When protein kinase A (PKA) activitywas blocked with H89 by previous intracellular (100 µM; n = 5)(Fig. 7e) or bath application (10 µM; n = 5) (data not shown),L-sulpiride, forskolin (n = 8) (Fig. 7e), or D2 receptor disruption(n = 5) (Fig. 7f) only partially prevented 3-NP-induced 3-NP-LTP.Thus 3-NP-LTP induction apparently requires the D2-receptor-mediatedinhibition of PKA at the postsynapticsite.

Role of MAP kinase ERK

D2 receptors and intracellular calcium interact to regulate the mitogen-activated protein kinase ERK in slices (Yan et al.,1999). All of these factors also participate in the generationof 3-NP-LTP. In addition, like 3-NP-LTP induction, ERK activityis controlled by glutamate acting through NMDA but not AMPA receptors(Kurino et al., 1995). ERK is an important intermediate in physiologicalsynaptic plasticity (Kornhauser and Greenberg, 1997; Robersonet al., 1999) and excitotoxicity (Xia et al., 1996). We thereforeevaluated the possibility that ERK might be involved in mediatingthe effect of D2 agonists in 3-NP-LTP. Indeed, treatment of corticostriatalslices with 3-NP induced ERK phosphorylation, a measure of itsactivation (Fig. 8a). This was fully abolished by preincubationwith 10 µM PD 98059, an inhibitor of the ERK-activating kinaseMEK. Using the same conditions, this pharmacological agent alsoprevented the induction of 3-NP-LTP (n = 15; p > 0.05) (Fig. 8b),thereby implicating the ERK cascade in this phenomenon. Accordingly,similar results were obtained by incubating the slices in thepresence of 30 µM of UO126 (n = 5; data not shown), another specificinhibitor of MEK. Furthermore, we found that doses of L-sulpirideable to block 3-NP-LTP (1 µM) significantly reduced the phosphorylationof ERK produced by 3-NP treatment (Fig. 8a).

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Figure 8. 3-NP-LTP induction is blocked by the ERK cascade inhibitor PD98059. Corticostriatal slices were treated with 100 µM 3-NP, with 3-NP plus MEK inhibitor PD 98059 (PD; 10 µM), or 3-NP together with 1 µM L-sulpiride as indicated in Materials and Methods. After protein extraction, ERK activation was analyzed by immunoblotting with antibodies specific for phosphorylated, activated ERKs 1 and 2. Equal levels of ERK were confirmed by immunoblotting with anti-ERK1/2 (a). Inhibition of MAP kinase activity by 10 µM PD 98059 prevented 3-NP-induced 3-NP-LTP (b).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

General findings

The present study provides two major novel findings. First, inhibition of mitochondrial complex II but not mitochondrial complexI activity results in a selective long-term enhancement of NMDA-mediatedsynaptic transmission in striatal spiny neurons. Second, endogenousDA is required for this form of synaptic plasticity via the activationof D2 DAreceptors.

Interestingly, the non-NMDA-mediated component of glutamatergic EPSPs is not affected by SD inhibitors. This observation indicatesthat 3-NP-LTP is expressed at the postsynaptic site. In fact,a presynaptic site of expression of this phenomenon (i.e., anincreased glutamate release after SD inhibition) would be detectedas an increase of both NMDA and non-NMDA components of striatalEPSPs. Accordingly, we found that in spiny neurons, but not incholinergic interneurons, both SD inhibitors selectively enhancedinward currents induced by application of NMDA, whereas responsesinduced by AMPA were unchanged. Because these experiments wereperformed in the presence of TTX, we assume that the facilitatoryeffect of NMDA responses caused by SD inhibitors is exerted ata postsynaptic site of action. However, a definitive demonstrationthat 3-NP does not influence excitatory transmission by enhancingglutamate release will require the analysis of spontaneous miniaturepotentials.

We have also evaluated the sensitivity to 3-NP of frontal and prefrontal pyramidal cortical neurons. These neurons have beenshown to be sensitive to mitochondrial activity inhibition (Ohgohet al., 2000), but at least in our experimental conditions, theydid not show significant electrophysiological changes after applicationof 3-NP. It is possible that higher concentrations, or longerperiods of exposure, or both, are required to affect the electrophysiologicalparameters in these neuronalsubtypes.

Moreover, we have also tested whether the inhibition of mitochondrial complex I by rotenone, which has been reported to interferewith dopamine cell survival (Betarbet et al., 2000), could alsomimic the 3-NP-LTP in striatal spiny neurons. We found that concentrationsof rotenone able to inhibit mitochondrial complex I activity invitro (Luetjens et al., 2000) do not induce potentiation of NMDA-mediatedresponses in striatal spiny neurons. This lack of effect of rotenonesuggests that the enhancement of NMDA-mediated neurotransmissionin the striatum is a pathophysiological response selectively triggeredby inhibition of SDactivity.

Role of intracellular calcium and glutamate receptors

An augmentation of postsynaptic intracellular calcium is a critical requirement for 3-NP-LTP, as demonstrated by the factthat blockade of this form of synaptic plasticity was achievedby buffering intracellular calcium. This observation is in agreementwith the view that intact mitochondrial activity is of crucialimportance for the maintenance of intracellular calcium homeostasis(Greene and Greenamyre, 1996; Murphy et al., 1999). Moreover,the capability of intracellular BAPTA to block 3-NP-LTP furthersupports the concept that, at least in the induction phase, 3-NP-LTPrequires postsynaptic changes in striatal spinyneurons.

In the present study, by using combined electrophysiological recordings and microfluorimetric measurements of intracellularcalcium from the same single striatal spiny neuron, we obtainedtwo major results. First, although 3-NP did not alter somaticmembrane potential of spiny neurons, it significantly enhancedbasal intracellular calcium levels. Second, a dramatic and long-lastingenhancement of intracellular calcium levels was triggered by NMDAapplication in the presence of 3-NP. This large, lasting increasein intracellular calcium levels after combined inhibition of mitochondrialcomplex II and activation of NMDA receptors might initiate thecascade of metabolic events leading to selective neuronal deathin thestriatum.

It has recently been reported that transgenic mice expressing an HD mutation are resistant to quinolinic acid-induced striatalexcitotoxicity (Hansson et al., 1999). This observation is incontrast to the excitotoxic hypothesis of HD pathology that ourdata support. Interestingly, in agreement with our findings, Levineet al. (1999) recently found an enhanced sensitivity to NMDA receptoractivation in two animal models ofHD.

Another novel finding of the present study is that SD inhibitors generate 3-NP-LTP only when the spiny neurons are in theup state. This experimental evidence could have profound pathophysiologicalimplications, because it suggests that any event leading to continuousmembrane depolarization, such as repetitive cortical activation,ischemia, or additional mitochondrial impairment, might facilitate3-NP-LTP induction via the generation of a vicious cycle of continualreinforcement.

Our understanding of the genetics of HD has advanced substantially in recent years (Reddy et al., 1999; Yamamoto et al., 2000).The discovery of the link between an expanded polyglutamine repeatin the IT15 gene and the synthesis of an altered huntingtin proteinrepresented a key step toward the definition of the molecularmechanisms underlying the pathogenesis of this disorder. Huntingtinis diffusely expressed in the brain and inhibits glyceraldehyde-3-phosphatedehydrogenase, a key enzyme in energy metabolism (Burke et al.,1996). Accordingly, brains of HD patients show decreased striatalglucose metabolism, abnormalities in mitochondrial electron transportchain, and increased concentrations of lactate (Gu et al., 1996;Browne et al., 1997). Nevertheless, it remained unclear how theinhibition of mitochondrial activity that affects the whole brainleads to the regional and cell type-specific vulnerability inHD. Our experiments provide novel insights into thisprocess.

Is endogenous dopamine involved in striatal neurodegeneration and 3-NP-LTP?

Oxidative stress impairs DA uptake (Berman et al., 1996), which can account for increased levels of DA in the cerebrospinalfluid of HD patients (Garrett and Soares-da-Silva, 1992). Thus,elevated concentrations of endogenous DA, combined with mitochondrialimpairment, might lead to increased sensitivity to excitotoxicity,resulting in preferential cell death in the striatum. It is alsopossible that DA metabolites, rather than DA itself, might contributeto cell death in animal models of HD. DA uptake is reduced instriatal synaptosomes exposed to mitochondrial poisons, and striatalDA levels are increased in rodents during infusion of the SD inhibitormalonate. Furthermore, animals treated with 3-NP for 5 d showedelevated levels of DOPAC but not DA, suggesting increased turnoverof DA by monoamino-oxidases (for review, see Jakel and Maragos,2000).

Our data suggest that the striatum is selectively vulnerable in HD because this structure is the main recipient of fibersreleasing DA, a neurotransmitter that is critical for the formationof 3-NP-LTP. In support of this possibility, DA antagonists andDA denervation limit striatal damage after chronic administrationof 3-NP and MMA (Maragos et al., 1998; Reynolds et al., 1998;Jakel and Maragos, 2000).

We found that D1 and D2 classes of DA receptors, which act in opposition to each other, are involved in the generation andmodulation of 3-NP-LTP. Several experimental findings supportthis hypothesis. First, 3-NP-LTP was absent in 6-OHDA-treatedrats and was restored by the administration of a D2 but not aD1 DA receptor agonist. Second, blockade of D2 but not of D1 DAreceptors prevented the expression of 3-NP-LTP. Interestingly,3-NP-LTP could also be inhibited by forskolin, an activator ofadenylyl cyclase, or by the D1 receptor agonist SKF 38393, suggestingthat inactivation of PKA is a crucial requirement for the generationof this form of synaptic plasticity. Accordingly, intracellularand bath application of H89, a PKA inhibitor, reverses the inhibitionof 3-NP-LTP induced by L-sulpiride, SKF 38393, and forskolin.Third, 3-NP-LTP was absent in mice lacking D2 DA receptors, confirmingthat D2 rather than other D2-like DA receptor subfamilies (D3and D4) are involved in this form ofplasticity.

The exact mechanism by which D2 receptor activation produces 3-NP-LTP is still an open question. In Figure 9, we propose apossible model to explain the interaction between intracellularcalcium, D2 DA receptors, PKA, and ERK (see below) in the generationof the 3-NP-LTP. It is possible that D2 receptors may favor releaseof calcium from intracellular stores (Vallar et al., 1990; Nemethyet al., 1998). Accordingly, it has recently been shown that activationof D2 DA receptors is able, via a phospholipase C-dependent mechanism,to mobilize intracellular calcium stores also in striatal spinyneurons (Hernandez-Lopez et al., 2000). This observation mightwell explain previous findings showing that activation of D2 receptorsincreases striatal calcineurin and ERK activity via calcium-dependentmechanisms (Nishi et al., 1997, Yan et al., 1999). Interestingly,the activation of this novel phospholipase C-dependent intracellularpathway by D2 receptors leads to a reduction of L-type calciumcurrents (Hernandez-Lopez et al., 2000). These data agree withour observation that D2- and calcium-dependent 3-NP-LTP are independentof L-type calcium channel activation. The D2-mediated mobilizationof intracellular calcium might further amplify the augmented calciumlevels induced by 3-NP-induced impairment of mitochondrial activityand NMDA receptor activation. Moreover, in this scenario, D2 receptoractivation blocks PKA activity and thereby might suppress PKA-dependentinhibition of Raf-1, leading to activation of the MAP/ERK cascade.It should be stressed, however, that the interaction between PKAand the ERK pathway is complex and remains controversial (forreview, see Sweatt, 2001). Thus, it is possible that an alternativepathway, not examined in this study, might account for ERK activationin 3-NP-LTP. Nevertheless, the intracellular cascade underlying3-NP-LTP seems to be specific for DA via D2 receptor activation.In fact, the blockade of M1-like muscarinic receptors, which alsoincreases intracellular calcium and favors striatal post-tetanicLTP (Calabresi et al., 1999), fails to alter 3-NP-LTP.

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Figure 9. Hypothetical model to account for the receptor and post-receptor mechanisms underlying 3-NP-LTP in striatal spiny neurons. D2 and D1 receptors exert opposing actions on adenylyl cyclase (AC) activity. The D2 receptor-mediated reduction of cAMP levels leads to the inhibition of protein kinase A (PKA) activity. This suppresses PKA-dependent inhibition of Raf-1 and consequently activates the MEK/ERK cascade. MEK activity is also stimulated by increased intracellular calcium levels ([Ca²⁺]_i). The increase in [Ca²⁺]_i is secondary to NMDA receptor stimulation, impairment of mitochondrial buffering properties caused by SD inhibition, and D2 receptor-mediated stimulation of phospholipase C (PLC). The final result of this cascade of biochemical events is the ERK-dependent induction of nuclear events leading to protein synthesis and altered NMDA receptor-channel complex function.

Is 3-NP-LTP a synaptic phenomenon specific for neurons vulnerable in HD?

The issue of cellular specificity is particularly important in HD. We have shown that 3-NP-LTP is expressed in spiny striatalneurons but not in cholinergic interneurons. Although this representsonly a partial step toward demonstrating true "striatal" specificity,we point out that in our experimental system, 3-NP failed to enhanceexcitatory transmission in frontal and prefrontal pyramidal corticalneurons.

It is well known that in HD the striatal enkephalinergic neurons of the "indirect" pathway are much more sensitive than arestriatal substance P neurons of the "direct" pathway (Antoniniet al., 1998; Mitchell et al., 1999). This corresponds to theirexpression of D2 and D1 receptors, respectively. In the currentview of striatal organization, the D2 receptor is expressed onlyin a part of spiny neurons. Nevertheless, it is worth noting thatstriatal neurons projecting to the internal segment of the globuspallidus and substantia nigra also can send axon collaterals tothe external segment of the globus pallidus, suggesting that directand indirect pathways are not truly segregated (Kawaguchi et al.,1990). In addition, although D1 and D2 receptors have been reportedto be largely segregated, single-cell RT-PCR experiments havealso demonstrated a substantial coexpression of these receptors(Surmeier et al., 1996; Nicola et al., 2000). Further supportof the hypothesis that D1 and D2 receptors are coexpressed instriatal spiny neurons arises from a recent anatomical and physiologicalstudy showing that both D1 and D2 receptors are coexpressed incultured striatal spiny neurons (Aizman et al., 2000). Thus, itis not surprising that we did not observe a heterogeneous responseof striatal spiny neurons to 3-NP. It is possible, in fact, thatalthough low levels of D2 receptors are not detectable by morphologicalanalysis, they could play a significant functionalrole.

Role of the MAP kinase ERK in 3-NP-LTP

Pathological events like energy metabolism impairment and excitotoxicity have been found to activate ERK in central neurons(Ghosh and Greenberg, 1995; Sugino et al., 2000). We found that3-NP induced a significant activation of ERK, as measured by itsphosphorylation, and that PD 98059 and UO126, two inhibitors ofthe ERK-activating kinase MEK, block 3-NP-LTP. One would expectthat the ERK cascade exerts its effect selectively on late phasesof synaptic plasticity by altering the pattern of gene expression.However, we found that the pharmacological inhibitors of the ERKcascade also blocked early stages of 3-NP-LTP, thereby suggestinga role early in this phenomenon. In agreement with this, PD 98059completely prevents LTP in the dentate gyrus and LTD in the prefrontalcortex, indicating that the activation of the MAP kinase ERK cascadecan play a role in the induction phases of different forms ofsynaptic plasticity in several brain areas (Coogan et al., 1999;Otani et al., 1999; Sweatt, 2001).

Conclusions

Future studies investigating the possible modulation of excitatory transmission in slices obtained from rats that have beenchronically intoxicated with systemic 3-NP injection should beperformed to compare the acute effects of this toxin with thoseproduced by the long-term inhibition of SDactivity.

Novel approaches in the therapy of HD have been proposed on the basis of mouse genetic models (Ona et al., 1999). Our datasuggest that drugs interfering with the mechanisms underlyingthe induction of 3-NP-LTP might represent an additional therapeuticstrategy to treat HD in its presymptomaticphase.

  FOOTNOTES

Received Nov. 27, 2000; revised March 23, 2001; accepted April 18, 2001.

This work was supported by the following grants: BIOMED Grant BMH4-97-2215 to P.C. and R.A.H.; Cofin-Ministero dell'Universitáe della Ricerca Scientifica e Tecnologica (MURST) and Telethon(Grant E.729) to P.C. and G.B.; MURST-Consiglio Nazionale delleRicerche (legge 95/95) to G.B.; and Grants MH-40899 and DA-10044to P.G. We thank Dr. Karima Chergui for helpful discussion andcritical reading of this manuscript. We also thank Massimo Tolufor technicalassistance.
Correspondence should be addressed to Prof. Paolo Calabresi, Clinica Neurologica, Dipartimento di Neuroscienze, Universitàdi Tor Vergata, Via di Tor Vergata 135, Rome 00133, Italy. E-mail:calabre{at}uniroma2.it.

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DISCUSSION
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