Electrophysiological and Morphological Evidence for a GABAergic Nigrostriatal Pathway

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The Journal of Neuroscience, June 1, 1999, 19(11):4682-4694

Electrophysiological and Morphological Evidence for a GABAergic Nigrostriatal Pathway
Manuel Rodríguez¹ and Tomás González-Hernández²
Departments of ¹ Physiology and ² Anatomy, Faculty of Medicine, University of La Laguna, La Laguna, Tenerife, Canary Islands, Spain

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The electrophysiological and neurochemical characteristics of the nondopaminergic nigrostriatal (NO-DA) cells and their functionalresponse to the degeneration of dopaminergic nigrostriatal (DA)cells were studied. Three different criteria were used to identifyNO-DA cells: (1) antidromic response to striatal stimulation withan electrophysiological behavior (firing rate, interspike intervalvariability, and conduction velocity) different from that of DAcells; (2) retrograde labeling after striatal injection of HRPbut showing immunonegativity for DA cell markers (tyrosine hydroxylase,calretinin, calbindin-D28k, and cholecystokinin); and (3) resistanceto neurotoxic effect of 6-hydroxydomine (6-OHDA). Our resultsshowed that under normal conditions, 5-8% of nigrostriatal neuronsare immunoreactive for GABA, glutamic acid decarboxylase, andparvalbumin, markers of GABAergic neurons, a percentage that reached81-84% after 6-OHDA injection. Electrophysiologically, NO-DA cellsshowed a behavior similar to that found in other nigral GABAergic(nigrothalamic) cells. In addition, the 6-OHDA degeneration ofDA cells induced a modification of their electrophysiologicalpattern similar to that found in GABAergic nigrothalamic neurons.Taken together, the present data indicate the existence of a smallGABAergic nigrostriatal pathway and suggest their involvementin the pathophysiology of Parkinson'sdisease.

Key words: nigrostriatal pathway; dopaminergic cells; GABAergic cells; GABA; glutamic acid decarboxylase; parvalbumin; calretinin; calbindin-D28k; cholecystokinin; Parkinson's disease

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The substantia nigra (SN) is a major output center of the basal ganglia (DeLong, 1990; Gerfen et al., 1990; Graybiel, 1990;Obeso et al., 1997), participating in their sensory-motor functions(DeLong et al., 1983; Hikosaka and Wurtz, 1983a-c; Schwarz etal., 1984; Schultz, 1986). This, together with its direct implicationon the physiopathology of Parkinson's disease (Albin et al., 1989;DeLong, 1990; Graybiel, 1990; Obeso et al., 1997; Viteck et al.,1997), has increased the interest in studying this mesencephaliccenter. The SN is composed primarily of two projection neurons.Dopaminergic (DA) cells, located in the pars compacta (SNc) andpars reticulata (SNr) and projecting to the striatum, and GABAcells, located in the pars reticulata and projecting to the thalamus,superior colliculus, and pedunculopontine nucleus (Dahlströmand Fuxe 1964; Kilpatrick et al., 1980; Childs and Gale, 1983;Chiodo, 1988; Hedreen and DeLong, 1991; Parent and Hazrati, 1995;Hazrati, 1995a,b). Some preliminary evidence suggests that, besidesthe dopaminergic nigrostriatal system, there are nondopaminergicnigral cells projecting to the striatum. Thus, not all SN cellsprojecting to the striatum show catecholamine fluorescence (vander Kooy et al., 1981) or tyrosine hydroxylase immunoreactivity(Swanson, 1982; Gerfen et al., 1987). Early electrophysiologicalstudies classified nigrostriatal cells as belonging to slow conductionvelocity (0.5 m/sec) pars compacta neurons and higher conductionvelocity (1.7 m/sec) pars reticulata neurons (Deniau et al., 1978;Guyenet and Aghajanian, 1978). The slow conduction velocity neuronswere subsequently identified as dopaminergic (Grace and Bunney,1980, 1983a). Most studies have been focused on this neuron type(Grace and Bunney, 1980, 1983a-c, 1984a,b, 1985a,b; DeLong etal., 1983; Schwarz et al., 1984; Schultz, 1986; Chiodo, 1988;Schultz and Romo, 1990), because they are probably conditionedby their direct involvement in various neurological disorders,including Parkinson's disease (Ehringer and Hornykiewicz, 1960),whereas the higher conduction velocity neurons have remained practicallyunexplored.

The main aim of this study was the electrophysiological and neurochemical characterization of nondopaminergic nigroestriatal(NO-DA) cells. Before analyzing their electrophysiological behavior,SN cells were classified as nigrostriatal or nigrothalamic accordingto their antidromic response (Guyenet and Aghajanian, 1978; Graceand Bunney, 1980, 1983a-c; Ruffieux and Schultz, 1980; Sandersonet al., 1986; Chiodo, 1988; MacLeod et al., 1990; Castellano andRodríguez, 1991; Castellano et al., 1993). In the neurochemicalstudy, nigrostriatal neurons were first identified by the retrogradetransport of horseradish peroxidase (HRP) from the striatum. Thenthey were classified as DA or GABA cells using different neurochemicalmarkers. For DA cells, besides tyrosine hydroxylase (TH, the rate-limitingenzyme in the DA synthesis), we used the peptide cholecystokinin(CCK; Hökfelt et al., 1980, 1985; Chiodo, 1988; Freeman and Chiodo,1988) and the calcium-binding proteins calretinin (CR) and calbindin(CB; Goodman et al., 1979; Rogers, 1987; Yamada et al., 1990;Heizmann and Hunziker, 1991; Iacopino et al., 1994; Liang et al.,1996), three substances contained in DA neurons (Résibois andRogers, 1992; Liang et al., 1996; McRitchie et al., 1996). ForGABA cells, besides GABA and glutamic acid decarboxylase (GAD,the synthesizing enzyme for GABA), we used parvalbumin (PV), acalcium-binding protein that, in the SN, is expressed by and restrictedto GABAergic neurons (Reiner and Anderson, 1993; Rajakumar etal., 1994).

In addition, taking into account experimental (Arbuthnott, 1974; Ruffieux and Schultz, 1980; Sanderson et al., 1986; Mitchellel al., 1989; DeLong, 1990; MacLeod et al., 1990; Robledo andFéger, 1992; Herrero et al., 1993; Burbaud et al., 1995) andclinical (Bernheimer et al., 1973; Condé, 1992) data suggestingthat some Parkinsonian motor disturbances, acquired after thedestruction of DA cells, are induced by a functional modificationin SN GABAergic cells projecting to the thalamus, we have alsostudied the effect of experimentally produced degeneration ofDA cells on the electrophysiological behavior of NO-DAcells.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals. Experiments were performed on male Sprague Dawley rats (300-350 gm; Panlab, Barcelona, Spain). Animals were housedat 22°C, two per cage, under normal laboratory conditions on astandard 12 hr light/dark schedule (with lights on from 3 A.M.to 3 P.M.) and with free access to food and water. Experimentalprotocols were in accordance with the European Community CouncilDirective of November 24, 1986 (86/609/EEC) regarding the careand use of animals for experimental procedures. Adequate measureswere also taken to minimize pain anddiscomfort.

A group of animals were lesioned using a procedure that induces a marked and selective destruction of DA neurons (Hökfeltand Ungerstedt, 1973; Castro et al., 1985). Under anesthesia (80mg/kg ketamine plus 12 mg/kg xylazine, i.p.), rats received adouble unilateral injection of 6-hydroxydopamine hydrochloride(6-OHDA; Sigma, St. Louis, MO; 8 µg in 4 µl of a 0.9% saline solutionwith 0.3 µg/µl ascorbic acid/injection; 1 µl/min) or vehicle inthe medial forebrain bundle (Castro et al., 1985; Burunat et al.,1988; Barroso and Rodríguez, 1996), according to the stereotaxiccoordinates of Paxinos and Watson (1988): 4.0 mm anterior to $lambda$ ,1.6 mm to the right of the midline, and 8 mm below the dura (firstinjection); and 4.6 mm anterior to $lambda$ , 1.4 mm to the right of themidline, and 8 mm below the dura (second injection). The behavioralevaluation of lesion degree (Castro et al., 1985) was performed2-3 weeks later. Animals showing more than eight turns per minutein response to apomorphine hydrochloride (1 mg/kg, i.p.; Sigma)were included in thestudy.

Electrophysiological studies. Unlesioned, sham-lesioned, and 6-OHDA lesioned (4-6 weeks after lesion) rats were anesthetizedwith chloral hydrate (400 mg/kg, i.p.), and the extracellularactivity of SN neurons was monitored according to the procedureof Castellano and Rodríguez (1991). Recordings (2.8-3.4 mm anteriorto $lambda$ , 1.8-2.4 mm lateral to the midline, and 7-8.5 mm below thecortical surface) were obtained from rats kept between 36.5 and37.0°C by using electrodes (glass tubing filled with 2 M NaClcontaining 2% Pontamine Sky Blue; BDH Chemicals, Poole, England)with a 6-9 m $Omega$ impedance (at 1000 Hz). The signal was amplified(3000×) and filtered (200-5000 Hz) in a high input impedance differentialamplifier (CAN96T; Telcan, Tenerife,Spain).

To identify nigrostriatal and nigrothalamic cells (Castellano et al., 1993; Rodríguez and Barroso, 1996), stimulating electrodeswere placed in the head of the caudate nucleus (0.0 mm anteriorto bregma, 3.2 mm to the right of the midline, and 5 mm ventralto the brain surface) and in the ventral thalamus (2.5 mm posteriorto bregma, 1.5 mm to the right of the midline, and 6.5-7 mm ventralto the brain surface). The collision test was applied to determinethe antidromic activation from these nuclei, using a Grass (WestWarwick, RI) S-8800 and a bipolar stimulating electrode made withstainless steel rods (250 µm diameter; A-M Systems, Everet, WA).Two rods were electroetched with a 60 Hz alternating current [1:1(v/v) 96% sulfuric acid/85% phosphoric acid] and insulated withSylgar 184 (Dow Corning, Wiesbaden, Germany), and their conductivetips (0.5 mm) were placed 500 µm apart. Neurons were consideredantidromically activated (0.5 mA/0.3 msec square pulse) when theyshowed (1) an antidromic spike per stimulus and a fixed latencyfrom the stimulus artifact (<0.05 msec) during high-rate stimulation(50 Hz) and (2) a collision between the spontaneously occurringaction potentials and the stimulation-elicited spikes. DA neuronswere identified by a 2-5 msec triphasic extracellular wave form(with a positive first phase), often displaying a prominent notch(initial segment-somatodendritic break) in the initial positiverising, a spontaneous activity <10 spikes/sec, and a long-latencyantidromic response (conduction velocity of ~0.5 m/sec) to striatalstimulation, mostly consisting of the initial segment componentof the action potential. GABAergic nigrothalamic neurons wereidentified by their biphasic extracellular wave form (often showinga duration of <1 msec) and a short-latency antidromic response(a conduction velocity of >1 m/sec) evoked from the ventromedialnucleus of thethalamus.

The basal activity of neurons was recorded 10 min after their antidromic identification. Extracellular signals were simultaneouslydigitized on a Pentium-based computer by using a 16 bit analog-to-digitalconverter (LTI-C30; Madrid, Spain), recorded on magnetic tapefor off-line analysis, and displayed on a storage oscilloscope.Only recordings with single-unit activity were used. Action potentialswere considered as displayed by the same neuron when the spikeshape, analyzed with both hardware (SD1 spike discriminator; Tucker-DavisTechnologies, Gainesville, Florida) and software (hybrid multilayerartificial neural network; Garcia et al., 1998) procedures, didnot change during the recording session. The firing rate (numberof spikes per second) and variation coefficient of interspikeintervals (VC; SD of interspike intervals/mean of interspike intervals)were computed for a recording time of at least 4min.

At the end of each experiment, the recording sites were marked by iontophoretic injection of Pontamine Sky Blue ( $-$ 20 µA, 30min), and the stimulus sites were marked by means of an iron depositedby passing a current of 10 µA for 30 sec. Rats were perfused with0.9% saline and 1% potassium ferricyanide in 10% formaldehyde.Brains were post-fixed in the same solution for 6-10 hr and cryoprotectedovernight in 30% sucrose at 4°C. Serial sections (50 µm thick)were obtained with a freezing microtome and stained with formalthionine.

Morphological studies. These studies were performed by combining retrograde transport of HRP and immunocytochemistry for differentmarkers of nigral neurons. Under anesthesia (80 mg/kg ketamineand 12 mg/kg xylazine, i.p.) and aseptic conditions, rats receiveda single injection of 0.2-0.4 µl of 40% HRP (Boehringer Mannheim,Mannheim, Germany) in the striatum 42-68 hr before killing. Giventhat under normal conditions the soma concentrations of some neuropeptides(i.e., CCK) and enzymes (i.e., GAD) are so low that they are difficultto detect with immunocytochemistry, a group of rats were injectedin the lateral ventricle (ipsilateral to the HRP injection) with10 µl of colchicine (10 mg/ml, Sigma) dissolved in saline 24 hrbefore killing. This is a successful procedure to block the axonaltransport, increasing the immunoreactivity in somata (Fallon etal., 1983; Seroogy et al., 1989; Campbell et al., 1991). Ratswere heavily anesthetized and transcardially perfused with 0.9%saline and a fixative solution of 1% paraformaldehyde and 1.25%glutaraldehyde in 0.1 M phosphate buffer, pH 7.4. Brains wereremoved and stored in the same fixative at 4°C for 4-12 hr. Midbrainswere initially obtained by using a brain blocker (ActivationalSystem, Warren, MI) and then cut at 30 µm with a vibratome. Sectionswere collected in parallel series, treated for inhibition of endogenousperoxidase with 3% H₂O₂, and processed for double labeling. First,they were processed for histochemical localization of HRP by using3,3'-diaminobenzidine (DAB, Sigma) intensified by cobalt chloride(Sigma; Adams, 1977) or nickel amonium sulfate (Serva, Heidelberg,Germany; Adams, 1981) as chromogen, which produces a black granularreaction product, and thereafter for immunocytochemical detectionof distinct markers (one series per marker) using nonintensifiedDAB, which produces a brown diffuse reactionproduct.

As primary antibodies we used a mouse anti-TH monoclonal antibody (1:8000, Sigma), a mouse anti-GABA monoclonal antibody (1:12,000;Matute and Streit, 1986), a rabbit anti-GAD polyclonal antibody(1:2000; Chemicon, Temecula, CA), a rabbit anti-CCK-8 polyclonalantibody (1:12000, Sigma), a mouse anti-CB monoclonal antibody(1:1000, Sigma), a rabbit anti-CR polyclonal antibody (1:5000,Chemicon), and a mouse anti-PV monoclonal antibody (1:6000, Sigma).After HRP histochemistry, sections were washed in 0.1 M PBS, pH7.4, and immersed for 60 min in the preincubation solution (PIS):3% normal goat serum (NGS; Vector Laboratories, Burlingame, CA)for GAD, CCK, and CR, or 3% normal horse serum (NHS, Vector Laboratories)for TH, GABA, CB, and PV; and 0.5% BSA (Serva) and 0.1% TritonX-100 (TX-100, Sigma) in PBS. Sections were then incubated overnightin the primary antibody dissolved in PIS. In GAD and GABA immunocytochemistryTX-100 was omitted. Sections were washed several times in PBSand incubated for 60 min in 1:200 biotinylated goat anti-rabbitantiserum (for GAD, CCK, and CR; Vector Laboratories) or 1:200biotinylated horse anti-mouse antiserum (for TH, GABA, CB, andPV; Vector Laboratories) and either 1:200 NGS or 1:200 NHS inPBS. Immunoreactions were visualized by incubation for 2 hr inExtrAvidin (1:5000, Sigma) in PBS and for 10 min in 0.005% DAB(Sigma) and 0.001% H₂O₂ in cacodylate buffer. After several rinsesin PBS, sections were mounted on gelatinized slides, dehydrated,cleared in xylene, and coverslipped with DPX (BDH). Control experimentsto demonstrate the specificity of the immunolabeling were performedby removing the primary or secondary antibodies, resulting innegativestaining.

The percentage of nigrostriatal neurons that were immunostained for the different markers was computed by counting the numberof double-labeled neurons in a total of 900 HRP-positive cellsper series in each unlesioned rat [700 in SN, 160 in ventral tegmentalarea (VTA), and 40 in retrorubral field (RRF)] and 70 HRP-positivecells per series in each lesioned rat (all then in SN). In eachseries, HRP-positive neurons were randomly elected in 10 sectionsseparated by a distance of 210 µm from each other and taken fromrostral SN to caudal RRF. The quantitative study was performedwith the aid of a Magiscan image analysis system using the Geniasprogram (Joyce-Loebl) and dividing the SN, VTA, and RRF into fieldsof 400 × 400 µm at a magnification of 200×. Taking into accountthat antisera only penetrate 8-10 µm from the surface, whereasHRP-positive neurons are evident at all depths of the section,we have only counted those single- and double-labeled neuronsexposed on the surface of sections, excluding diffusely HRP-labeledcells.

Statistical comparisons. The statistical analyses were performed using a one-way ANOVA followed by appropriate post hoc tests(Statistica; Statsoft, Tulsa, OK). In all cases, a level of p< 0.05 was considered critical for assigning statisticalsignificance.

Experiment 1: electrophysiological identification of nondopaminergic nigrostriatal cells. The extracellular electrophysiologicalactivity of 374 nigral cells was recorded in 33 unlesioned rats.Electrical stimulation of the head of the caudate nucleus andventral thalamus was used for identifying the target of recordedneurons. Multiunitary recordings were excluded, and only cellsshowing antidromic response to striatal (n = 142) or thalamic(n = 62) stimulation were finallyincluded.

Experiment 2: morphological and neurochemical identification of nondopaminergic nigrostriatal cells. To identify cells projectingto the striatum, 12 rats were injected in the caudate nucleuswith HRP. Two days later, 6 of them were injected in the lateralventricle with colchicine. After 2 d in the case of the colchicine-untreatedrats and 3 d in the case of colchicine-treated rats, they wereheavily anesthetized, perfused, and processed for the histochemicaland immunocytochemicalstudies.

Experiment 3: effect of dopaminergic nigrostriatal cells degeneration on nondopaminergic nigrostriatal neurons. Forty-fourrats were used to evaluate the effects of DA cell degenerationon nondopaminergic nigrostriatal and nigrothalamic neurons. Twoto 3 weeks after 6-OHDA (n = 22) or vehicle (n = 22) injections,rats were behaviorally tested to determine the lesion degree.Twenty to 40 d later they were anesthetized for the electrophysiological(16 sham and 16 6-OHDA-injected rats) or neurochemical (6 shamand 6 6-OHDA-injected rats) studies, following the same protocolsused in experiments 1 and 2, but in this experiment colchicinewas notused.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experiment 1: electrophysiological identification of nondopaminergic nigrostriatal cells

During this experiment 123 DA cells, 19 NO-DA cells, and 62 nigrothalamic cells were recorded. DA cells showed the characteristictriphasic action potential with the first phase being positive(often displaying a notch on the initial rising) and a durationof 2-6 msec (Fig. 1c). The DA cells showed a stable antidromiclatency (oscillations <0.05 msec) and were identified as nigrostriatalneurons by the collision test (Fig. 1f). The conduction velocitywas 0.52 ± 0.023 m/sec (mean ± SE; Fig. 1h) with an antidromiclatency of 7-20 msec (Fig. 1g). NO-DA cells showed a biphasicshort-duration (often <1 msec) spike with a positive first phase(Fig. 1a) and an antidromic response to striatal stimulation witha positive collision test (Fig. 1d). The conduction velocity was3.48 ± 1.80 m/sec (Fig. 1h) with an antidromic latency of 0.5-5msec (Fig. 1g). Nigrothalamic neurons displayed a characteristicbiphasic action potential with a positive first phase and a durationof <1 msec (data not shown). The thalamic stimulation induceda stable antidromic response with a positive collision test (Fig.1e) and a conduction velocity of 1.65 ± 1.03 m/sec (Fig. 1h).Thus, the conduction velocity was different in the three cellgroups (ANOVA, F = 42.19; p < 0.0001), with the nigrothalamicneurons showing values lower than those of NO-DA cells (p < 0.0001)and higher than those of DA neurons (p < 0.0001).

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Figure 1. Electrophysiological identification of NO-DA, DA, and nigrothalamic cells. An example of the spike shape (a-c) and collision test (d-f) in NO-DA, nigrothalamic, and DA cells, respectively, is shown. The antidromic response consisted of the full spike in NO-DA cells (d) and nigrothalamic cells (e) and the initial segment in DA cells (f). Because the antidromic stimulation of DA cells often displays the initial segment but not the somatodendritic component of the spike (spike dissociation), the antidromic spike shown at the top of f is clearly different (somatodendritic component virtually absent) from the spontaneous spike showed at the bottom of f. g, Antidromic latency histogram of nigrostriatal cells. Values are expressed as a percentage of the total number of NO-DA (n = 19) or DA (n = 123) recorded neurons. h, Basal activity and conduction velocity of DA and NO-DA nigrostriatal (NS) and nigrothalamic (NT) cells. *p < 0.0001 versus NS DA cells; **p < 0.01 versus NS DA cells. °p < 0.0001 versus NT cells. Arrows in c and d indicate the initial part of the striatal stimulus artifact. Values represent the mean ± SE.

Statistical differences were also found for firing rate and VC (Fig. 1h). Both NO-DA (p < 0.0001) and nigrothalamic (p < 0.0001)cells showed a firing rate higher than that found in DA cells(ANOVA, F = 67.42; p < 0.0001), with no difference between NO-DAand nigrothalamic neurons (p = 0.43). VC also showed higher valuesin NO-DA (p < 0.01) and nigrothalamic (p < 0.0001) cells thanin DA cells (ANOVA, F, = 15.34; p < 0.0001), with no statisticaldifference between NO-DA and nigrothalamic cells (p = 0.51). Whereasa group of DA and nigrothalamic neurons showed a bursting activity,most NO-DA cells presented a regular tonic discharge, and onlya few of them displayed irregulardischarges.

Experiment 2: morphological and neurochemical identification of nondopaminergic nigrostriatal cells

Although as expected, after HRP injection in the striatum, most HRP-positive neurons in the basal midbrain were immunopositivefor TH, a significant number of them were TH-negative (15.3%).They were preferentially located in the SNr (Figs. 2, 3), in alower proportion in VTA, and only a few of them in RRF (Fig. 3).

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Figure 2. HRP-TH double labeling after HRP injection in the striatum of unlesioned rats. a, Rostrolateral region of the SN; b, boxed area in a; c, caudomedial region of the SN. Arrows in b and c indicate single HRP-stained neurons in focus with double-labeled neurons (arrowheads). Scale bars: a, 200 µm; b, c, 50 µm.

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Figure 3. Mesencephalic distribution of cells projecting to the striatum according to their tyrosine hydroxylase immunoreactivity (n = 10,800 HRP cells). TH (+), Tyrosine hydroxylase-immunopositive cells; TH ( $-$ ), tyrosine hydroxylase-immunonegative cells.

As mentioned above, to identify these nigrostriatal neurons neurochemically, alternate sections were immunostained with differentnigral neuron markers. In this experiment, we focused on GABAergicneuron markers, using GAD, GABA, and PV immunocytochemistry inboth colchicine-treated and untreatedrats.

Double-labeled neurons were found in both colchine-treated and untreated rats (Fig. 4). The number of the GAD-HRP-positivecells (Fig. 4a-c) was slightly higher in the colchicine-treatedrats, in which they reached levels of 5.2% of the total numberof HRP-positive cells. In untreated rats, this proportion was3.8%. The number of GABA-HRP-positive neurons (Fig. 4d,e) was1.5% of the total number of HRP neurons. PV-HRP-positive neurons(Fig. 4f) displayed the largest proportion of double-labeled neurons(7.7%). The percentage of GABA-HRP- and PV-HRP-labeled cells didnot change after colchicine injection.

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Figure 4. Double-labeled neurons for HRP and GAD (a-c), HRP and GABA (d, e), and HRP and PV (f) in the SNr (a, b, d-f) and VTA (c) of unlesioned rats. The arrow in a indicates the neuron shown in b. In c, d, and f, arrows indicate double-labeled neurons; arrowheads indicate single immunostained neurons. Scale bars: a, 200 µm; b, f, 20 µm; c-e, 30 µm.

The distribution pattern of double-labeled neurons was very similar to that of single HRP-stained neurons in material processedfor TH with the largest number of GABA-projecting (77.8%), GAD-projecting(74.3%), and PV-projecting (80.2%) neurons localized in the SNr(Fig. 4a,b,d,e,f), only a few of them in VTA (Fig. 4c), and nonein the SNc and RRF. Morphologically, they constitute a polymorphicpopulation of elongated and round cells, with their largest diameterranging between 15 and 23 µm. Although the aim of this study wasnot to investigate the topography of this projection, we observedthat the localization of double-labeled cells in the SNr varieddepending on the injection site in striatum. As shown in Figure5, neurons projecting to the medial part of striatum localizein medial regions of the SNr, and those projecting to the lateralpart of striatum localize in the lateral part of the SNr. In therostrocaudal axis, this topographic relation was not as evidentas in the mediolateral one, because after injection in any placein the striatum, double-labeled cells were present at any rostrocaudallevel of the SNr. However, after rostral injections, the largestnumber of double-labeled cells was in the rostral half of theSNr, and after caudal injections, they localize perferentiallyin caudal regions of the SNr.

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Figure 5. Distribution of GAD-IR nigrostriatal neurons. a, Example of HRP injection in the striatum. b, Schematic drawing showing the localization of the HRP injection in some representative cases. c, Distribution of GAD-HRP neurons in the SN in two cases. Solid circles indicate the localization of double-labeled neurons after injection in the lateral half of striatum (shown in a, black area in b). Open circles indicate the localization of double-labeled neurons after injection in the medial half of striatum (shadowed area in b). Each circle corresponds to three neurons. Modified drawing from Paxinos and Watson (1988). The distance of each section to the interaural line is shown in millimeters. ac, Anterior commissure; cc, corpus callosum; f, fornix; GP, globus pallidus; ic, internal capsule; lv, lateral ventricle; MT, medial terminal nucleus of the accessory optical tract; S, septum; SNl, substantia nigra pars lateralis; St, striatum. Scale bar, 1 mm.

Experiment 3: effect of dopaminergic nigrostriatal cells degeneration on nondopaminergic nigrostriatal neurons

The injection of 6-OHDA into the very center of the medial forebrain bundle led to the degeneration of practically all nigralDA-neurons ipsilateral to injection (Figs. 6a,b, 8), affectingtheir different neurochemical subpopulations in the same way,as demonstrated by CCK (see Fig. 8), CR (Figs. 6e,f, 8) and CB(Figs. 6g,h, 8) immunocytochemistry. By comparing the number ofdouble labeled neurons in sham and lesioned rats (Fig. 7), wefound that after lesion, the percentage of HRP cells showing immunoreactivityfor TH decreased from 82.3 to 1.2%, for CCK from 61.4 to 0.9%,for CB from 21.1 to 1.6%, and for CR from 86.1 to 1.6%.

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Figure 6. TH (a-d), CR (e, f), and CB (g, h) immunocytochemistry after 6-OHDA injection in the right medial forebrain bundle and HRP injection in the ipsilateral striatum. a, e, g, Lesioned side; b, f, h, unlesioned side. c, d, Boxed areas in a; arrows indicate single HRP-stained neurons. Scale bars: a, b, e-h, 150 µm; c, d, 35 µm.

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Figure 7. Double-labeled neurons for HRP and GAD (a), HRP and GABA (b), and HRP and PV (c, d) in SNr of 6-OHDA lesioned rats. d, Boxed area in c; arrows in b and d indicate double-labeled neurons; arrowhead in d indicates a single PV-immunostained neuron. Scale bars: a, b, 20 µm; c, 200 µm; d, 30 µm.

Despite the massive degeneration of DA cells, a number of retrogradely labeled neurons survived the neurotoxic effect of 6-OHDA(Fig. 6a,c,d), most of them showing immunoreactivity for differentGABA cell markers (Figs. 7, 8). Thus, when compared with the shamgroup, the percentage of HRP cells showing immunoreactivity forGABA (Fig. 7b) increased from 1.2 to 84.3%, those showing immunoreactivityfor GAD (Fig. 7a) increased from 4.9 to 81.3%, and those showingimmunoreactivity for PV (Fig. 7c,d) increased from 8.3 to 83.0%.

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Figure 8. Percentage of nigrostriatal cells showing TH, CCK, CB, CR, GABA, GAD, and PV immunoreactivity in sham (n = 4200 HRP cells per series) and 6-OHDA-injected (n = 420 HRP cells per series) rats.

The electrophysiological study showed a functional modification of NO-DA and nigrothalamic cells after the 6-OHDA degenerationof DA neurons (Fig. 9). Although no statistical differences werefound in the firing rate (p = 0.64) and conduction velocity (p= 0.45), NO-DA cells showed a higher VC in the 6-OHDA lesionedthan in the sham-lesioned rats (p < 0.05). This effect was similarto that found in the nigrothalamic GABAergic neurons, with nomodification in the firing rate (p = 0.45) and conduction velocity(p = 0.22) but with an increase in the VC (p < 0.05).

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Figure 9. Functional effect of DA cell degeneration on NO-DA and nigrothalamic (NT) cells. *p < 0.05 versus sham-lesioned rats. Values represent the mean ± SE.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study we present evidence supporting the existence of GABAergic nigrostriatal cells with electrophysiological andneurochemical characteristics similar to those of GABAergic nigrothalamiccells but different from DA nigrostriatal neurons. After 6-OHDAinjection, which produced the disappearance of the DA neurons,these cells remained intact, showing a change in the electrophysiologicalbehavior similar to that found in nigrothalamic cells. Taken together,present findings indicate the existence of a GABAergic nigrostriatalpathway and suggest its involvement in the pathophysiology ofParkinson'sdisease.

Data supporting a nondopaminergic nigrostriatal pathway

Our morphological data show a subpopulation of SN neurons retrogradely labeled after HRP injection in the striatum that isnonimmunoreactive for TH, CCK, CR, or CB, proteins expressed byDA cells (Hökfelt et al., 1980, 1985; Résibois and Rogers, 1992;Liang et al., 1996; McRitchie et al., 1996). The fact that theseneurons do not degenerate after the injection of 6-OHDA, a neurotoxinselectively taken up by a transporter only contained in DA neurons(Hökfelt and Ungerstedt, 1973; Cohen and Heikkila, 1974; Walkinshawand Waters, 1994; Ciliax et al., 1995; Betarbet et al., 1997;Miller et al., 1997), also supports the existence of NO-DA cells.Present findings confirm previous morphological studies reportingnigrostriatal cells without catecholamine fluorescence (van derKooy et al., 1981) or TH immunoreactivity (Swanson, 1982; Gerfenet al., 1987) and provide further morphological evidence showingthat they are not immunoreactive for CR, CB, andCCK.

The electrophysiological studies also identified a group of nigrostriatal neurons with a conduction velocity several timeshigher than that found in the DA cells. Although this cell typewas mentioned in the early works of Deniau et al. (1978) and Guyenetand Aghajanian (1978), they were never systematically studied.As shown in Figure 1f, these cells displayed a higher basal firingrate and VC than those of DA neurons. In the 6-OHDA lesioned rats,surviving nigral neurons showing an antidromic response to striatalstimulation presented a conduction velocity and basal firing ratesimilar to those found for NO-DA cells in unlesioned rats. Thisfinding also indicates that 6-OHDA does not affect NO-DAcells.

Data supporting a GABAergic nigrostriatal pathway

Double labeling for HRP and GABA, GAD, or PV showed that 5-8% of nigrostriatal cells are GABAergic. This percentage reached81-84% of all retrogradely labeled neurons in 6-OHDA lesionedrats. The difference observed in the experiment 2, between thepercentage of nigrostriatal neurons showing TH immunonegativity(15%) and those showing GAD, GABA, and PV immunopositivity (5-8%),could suggest that not all NO-DA cells are GABAergic. The factthat after lesion (experiment 3) almost all TH, CCK, CR, and CBnigrostriatal neurons disappeared, whereas >80% of HRP neuronswere immunopositive for GAD, GABA, and PV, indicates that if asubpopulation of NO-DA cells is not GABAergic, this is quantitativelynegligible. It is possible that, despite our effort counting onlythose neurons lying in the surface of sections, and because ofthe limited penetration of antisera (8-10 µm) compared with thatof HRP (evident at all depths of the sections), the number ofsingle HRP-stained neurons was overestimated. So, we must be cautiouswhen interpreting our quantitativedata.

GABAergic nigrostriatal neurons are restricted to the SNr, and their distribution varies as a function of the injection sitein striatum. In the mediolateral axis, they follow a topographicpattern similar to that previously described for the dopaminergicnigrostriatal projection (Fallon and Moore, 1978) and for strionigraldescending fibers (Gerfen, 1985). In the rostrocaudal axis, thetopography of GABAergic nigrostriatal neurons is also biased accordingto the injection site, matching that of the dopaminergic ones(Fallon and Moore, 1978) but differing from that of descendingstrionigral fibers that, independently of the injection site,are distributed homogeneously throughout the rostrocaudal axisof the SNr (Gerfen, 1985). Although our material does not allowus to establish a precise spatial correspondence in the GABAergicnigrostrial pathway, we can suggest that this may be involvedin the modular organization of the nigro-strio-nigral loop (Deniauand Chevalier, 1992; Parent and Hazrati, 1995; Deniau and Thierry,1997).

A further support for the GABAergic nature of NO-DA cells comes from electrophysiological data. The firing rate and VC ofNO-DA cells were higher than those of DA cells (Grace and Bunney,1980, 1983a-c, 1984a,b, 1985a,b; DeLong et al., 1983; Schwarzet al., 1984; Schultz, 1986; Chiodo, 1988) but similar to thoseof other SN GABAergic neurons (Sanderson et al., 1986; Burbaudet al., 1995). Contrary to that reported in DA cells (Grace andBunney, 1984a,b; Overton and Clark, 1997), NO-DA cells showedno clear evidence of burst discharge. Most of them displayed tonicdischarges with different degrees of regularity, a pattern similarto that reported in two subgroups of nigrothalamic neurons: theregular tonic and the irregular tonic discharging groups (Sandersonet al., 1986; Burbaud et al., 1995). On the other hand, the conductionvelocity suggests that these GABAergic nigrostriatal cells areprobably composed of myelinated fibers of a relatively small diameter(3.48 ± 2.03 m/sec), in contrast to the unmyelinated axon of DAneurons (0.52 ± 0.02 m/sec).

It is known that, besides the dopaminergic nigrostriatal projection, there are DA cells projecting to the striatum from bothVTA and RRF (Parent et al., 1983; Charara and Parent, 1984; Lewisand Sesack, 1997). Along with these cells, we found nondopaminergiccells transporting HRP from the striatum to VTA and RRF. Recently,GABAergic cells have been reported in the VTA (Steffensen et al.,1998). Our data show that the striatum is one of the targets forthese cells, although the electrophysiological and neurochemicaldetails of this projection require furtherstudy.

GABAergic nigrostriatal pathway and dopaminergic cell degeneration

In the current model of the organization of basal ganglia, the symptoms of different diseases have been explained on the basisof modifications in the firing rate of specific cell groups (Albinet al., 1989; Alexander and Crutcher, 1990a,b; DeLong, 1990),disturbances that may be attenuated by new neurosurgical therapiesthat modify the balance between excitatory and inhibitory inputs(Marsden et al., 1997; Obeso et al., 1997; Pollak et al., 1997;Viteck et al., 1997). It has been suggested that a reduction ofstriatal dopamine leads to activation of the inhibitory GABAergicnigrothalamic input (Bernheimer et al., 1973; Mitchell et al.,1989; DeLong, 1990; MacLeod et al., 1990; Condé, 1992; Herreroet al., 1993; Burbaud et al., 1995), and a subsequent reductionof thalamo-cortical activation (DeLong, 1990; Obeso et al., 1997).The final result could be a cortical inhibition that may be directlyinvolved in different motor disturbances and especially in thehypokinesia often found in Parkinson's disease. This hypothesisis supported by previous experiments showing that the degenerationof dopaminergic nigrostriatal cells produces an increase of 2-deoxyglucoseuptake (Mitchell el al., 1989) and GAD mRNA levels (Herrero etal., 1993; Vila et al., 1996) in SNr cells. However, the overexpressionof GAD and GABA does not necessarily imply an increase of GABAergiccell activity or GABA release. Contradictory results have beenreported about the functional consequences of the DA cell degenerationon the GABA turnover (Tanaka et al., 1986; Lindgren, 1987; Samuelet al., 1988; Houssain and Weiner, 1995) and firing rate (Arbuthnott,1974; Ruffieux and Schultz, 1980; Sanderson et al., 1986; MacLeodet al., 1990; Robledo and Féger, 1992; Burbaud et al., 1995)of SNr cells. Our data show that the increase of GAD expressionpreviously reported by others in 6-OHDA lesioned rats is not associatedwith changes in the firing rate, at least in nigrothalamic andnigrostriatal GABAergic neurons. However, the VC increased inboth groups. Despite the fact that we did not block 6-OHDA uptakeinto noradrenergic fibers, the effect appears to be secondaryto the degeneration of DA neurons, because this was similar tothat consistently reported in previous studies for nigrothalamicneurons (Ruffieux and Schultz, 1980; Sanderson et al., 1986; MacLeodet al., 1990). It has been suggested that a firing pattern codecould be a more important feature than the mean firing rate forexplaining the basal ganglia activity (Chesslet and Delfs, 1996;Wichmann and DeLong, 1996; Parent and Ciccheti, 1998). However,the characteristics of this code remain unknown (Eggermont, 1990),and only indirect measurements of the information processing inthe basal ganglia can be taken. A suitable measure in this caseis the VC, an indicator of the interspike interval variabilitythat is invariant to the firing rate. From this point of view,the modification of VC observed in nigrothalamic and nigrostriatalGABAergic cells after 6-OHDA lesion suggests that DA cells modulatethe SNr cell activity in a complex manner and do not induce asimple modification of the firing rate. Previous evidence showedthat whereas the GABAergic neurons of SNr process and transmitinformation concerning different sensory or motor functions (DeLonget al., 1983; Hikosaka and Wurtz, 1983a-c; Schwarz et al., 1984;Joseph and Boussaoud, 1985; Schultz, 1986; Condé, 1992), theDA cells of SNc only have a role in maintaining stable levelsof dopamine in the striatum (Gonon and Buda, 1985; Gonon, 1988,1997; Levey et al., 1993; Overton and Clark, 1997), respondingin a similar and stereotyped manner to sensory stimuli and notencoding detailed movement parameters (DeLong and Georgopoulos,1979; Georgopoulos et al., 1983; Schultz et al., 1983; Schultzand Romo, 1990; Alexander and Crutcher, 1990a,b; Apicella et al.,1992; Schultz, 1998). Despite the fact that DA may not be directlyinvolved in the information processing, its presence is necessaryfor nigrothalamic cells to analyze and transmit information tothe thalamus on its return to the cerebral cortex (Penney andYoung, 1983; Alexander at el., 1986; DeLong, 1990; Gerfen et al.,1990; Graybiel, 1990). Present data show a new pathway that canbe used to reintroduce the information in the striatum, once ithas been processed in the SN. Because the 6-OHDA lesion inducesa similar modification in GABAergic cells projecting to the thalamus(a pathway extensively involved in the Parkinsonian symptoms)and striatum, present data suggest that GABAergic nigrostriatalneurons participate in the pathophysiology of this basal gangliadisorder.

  FOOTNOTES

Received Dec. 28, 1998; revised March 5, 1999; accepted March 24, 1999.

This work was supported by Ministerio de Sanidad y Consumo, FIS, Grant 98/1499) and Gobierno Autonomo de Canarias Grant PI1998/008,Spain.
Correspondence should be addressed to Manuel Rodríguez, Department of Physiology, Faculty of Medicine, University of La Laguna,La Laguna, Tenerife, Canary Islands,Spain.

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