Opposite Membrane Potential Changes Induced by Glucose Deprivation in Striatal Spiny Neurons and in Large Aspiny Interneurons

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Volume 17, Number 6, Issue of March 15, 1997 pp. 1940-1949
Copyright ©1997 Society for Neuroscience

Opposite Membrane Potential Changes Induced by Glucose Deprivation in Striatal Spiny Neurons and in Large Aspiny Interneurons

Paolo Calabresi¹, Carlos Magarinos Ascone¹, Diego Centonze¹, Antonio Pisani¹^,², Giuseppe Sancesario¹, Vincenza D'Angelo¹, and Giorgio Bernardi¹^,²
¹ Clinica Neurologica, Dip. Sanitá, Universitá di Roma Tor Vergata, 00173 Rome, Italy, and ² IRCCS Ospedale S. Lucia, Via Ardeatina, Rome, Italy

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

We have studied the electrophysiological effects of glucose deprivation on morphologically identified striatal neurons recordedfrom a corticostriatal slice preparation. The large majority ofthe recorded cells were spiny neurons and responded to aglycemiawith a slow membrane depolarization coupled with a reduction ofthe input resistance. In voltage-clamp experiments aglycemia causedan inward current. This current was associated with a conductanceincrease and reversed at $-$ 40 mV. The aglycemia-induced membranedepolarization was not affected by tetrodotoxin (TTX) or 6-cyano-7-nitroquinoxaline-2,3-dioneplus aminophosphonovalerate, antagonists acting respectively onAMPA and NMDA glutamate receptors. Also, the intracellular injectionof bis(2-aminophenoxy)ethane-N,N,N $'$ ,N $'$ -tetra-acetic acid, a calcium(Ca²⁺) chelator, and low Ca²⁺/high Mg²⁺-containing solutions failed to reduce this phenomenon. Conversely,it was reduced by lowering external sodium (Na⁺) concentration.
A minority of the recorded cells had the morphological characteristics of large aspiny interneurons and the electrophysiologicalproperties of "long-lasting afterhyperpolarization (LA) cells."These cells responded to aglycemia with a membrane hyperpolarization/outwardcurrent that was coupled with an increased conductance. This currentwas not altered by TTX, blockers of ATP-dependent potassium (K⁺) channels, and adenosine A1 receptor antagonists, whereas itwas reduced by solutions containing low Ca²⁺/high Mg²⁺. This current reversed at $-$ 105 mV and was blocked by barium,suggesting the involvement of a K⁺ conductance. We suggest that the opposite membrane responsesof striatal neuronal subtypes to glucose deprivation might accountfor their differential neuronal vulnerability to aglycemia andischemia.
Key words: aglycemia; ischemia; excitatory amino acids; neuronal death; striatum; interneurons

INTRODUCTION

In comparison with the cellular responses reported after anoxia in the CNS, the effects of glucose deprivation on single neuronalpopulations have been investigated less extensively. It is knownthat aglycemia hyperpolarizes hippocampal cells (Spuler et al.,1988) and neurons recorded from dorsolateral septal nucleus (Shoji,1992). Aglycemia-activated K⁺ channels are present on hippocampal neurons (Tromba et al., 1992);these channels are blocked by the sulfonylurea glibenclamide.In contrast, in human cortical neurons, intracellularly recordedin vitro postsynaptic changes were not observed for periods ofglucose depletion of <1 hr (Jiang and Haddad, 1992). Developmentaland regional differences in the vulnerability of rat hippocampalslices to lack of glucose have been reported (Crepel et al., 1992).

In the present study we have analyzed the effects produced by glucose deprivation on the membrane properties of striatal neuronsintracellularly recorded in a corticostriatal slice preparation.Most of these neurons have been morphologically identified. Moreover,we have investigated the possible involvement of excitatory aminoacids in the effects of glucose deprivation and the ionic mechanismsunderlying the membrane potential changes induced by aglycemia.We have been encouraged to examine this issue for three main reasons.First, striatum belongs to the selective vulnerable brain regionsthat are prone to develop neuronal damage in clinical and experimentalaglycemia (Auer et al., 1984; Auer and Siesjo, 1988; Kristianet al., 1995; Nakao et al., 1995) and ischemia (Brierley, 1976;Pulsinelli et al., 1982; Hawker and Lang, 1990). Second, subpopulationsof striatal neurons show a differential sensitivity to energydeprivation (Beal, 1992). In fact, although spiny neurons arevulnerable to ischemia (Brierley, 1976; Pulsinelli, 1985; Xu,1995) and excitatory amino acid agonists (Beal et al., 1986; Calabresiet al., 1990a, 1995a), striatal interneurons are more resistantto ischemia (Francis and Pulsinelli, 1982) and excitotoxicity(Koh and Choi, 1988). Third, different subtypes of striatal interneuronshave been identified recently on the basis of differential electrophysiological,morphological, and histochemical properties (Wilson et al., 1990;Kawaguchi, 1993; Kawaguchi et al., 1995). Thus, it is of particularinterest to investigate the membrane changes induced by aglycemiaon spiny neurons and to compare these responses with those observedin interneurons.

MATERIALS AND METHODS
Preparation and maintenance of the slices. Wistar rats (150-250 gm) were used. The preparation and maintenance of coronalslices have been described previously (Calabresi et al., 1990a,b,c,1991). Briefly, corticostriatal coronal slices (200-300 µm) wereprepared from tissue blocks of the brain with the use of a vibratome.A single slice was transferred to a recording chamber and submergedin a continuously flowing Krebs solution (35°C, 2-3 ml/min) gassedwith 95% O₂/5% CO₂. To study glucose metabolism in striatal neurons,we deprived slices of glucose by removing glucose totally fromthe perfusate and by adding saccharose to balance the osmolarity.In some experiments the osmolarity was balanced by increasingthe NaCl concentration (Jiang and Haddad, 1992). Because experimentsperformed by using these different procedures to replace glucosegave similar results, all the data were pooled. Aglycemic solutionsentered the recording chamber no later then 20 sec after a three-waytap was turned. Complete replacement of the medium in the chambertook ~90 sec, as determined by the speed of diffusion of a coloredsolution. The composition of the control solution was (in mM):126 NaCl, 2.5 KCl, 1.2 MgCl₂, 1.2 NaH₂PO₄, 2.4 CaCl₂, 11 glucose,25 NaHCO₃. In some experiments, choline chloride was used to replaceNa⁺ chloride. In these experiments, Na⁺ chloride was reduced to 30% (38 mM). In other experiments, lowCa²⁺ (0.5 mM)/high Mg²⁺ (10 mM) solutions were used.

Recording technique. In most of the experiments, the intracellular recording electrodes were filled with 2 M KCl (30-60 M $Omega$ ).In some experiments, the pipettes were filled with 2 M potassiumacetate. In other experiments, 200 mM BAPTA was added to the solutionof the intracellular pipette. An Axoclamp 2A amplifier was usedfor recordings in either current-clamp or voltage-clamp mode.In the single-electrode voltage-clamp mode, the switching frequencywas 3 kHz. The headstage signal was monitored continuously ona separate oscilloscope. Traces were displayed on an oscilloscopeand stored on a digital system. For synaptic stimulation, bipolarelectrodes were used. These stimulating electrodes were locatedeither in the cortical areas close to the recording electrodeor in the white matter between the cortex and the striatum toactivate corticostriatal fibers.

In some experiments, biocytin (Sigma, St. Louis, MO) was used in the intracellular electrode to stain the neurons. In thesecases, biocytin at a concentration of 2-4% was added to a 0.5M KCl pipette solution. Slices containing neurons stained withbiocytin were fixed in paraformaldehyde (in 0.1 M phosphate bufferat pH 7.4) overnight and processed according to published protocols(Horikawa and Armstrong, 1988).

In other experiments, the tip of microelectrodes was filled with a solution containing 2 mM fura-2 pentapotassium salt (MolecularProbes, Eugene, OR) and 100 mM KCl, and the shank was filled with1 M KCl. After intracellular injection of the dye with negativecurrent (0.1-0.5 nA), fluorescence was elicited by epi-illuminationwith a Xenon arc lamp. Excitation light was filtered at both 340and 380 nm. Fluorescent emission light was filtered through along-pass barrier filter and detected by a CCD camera controlledby software (ImproVision) running on Power Macintosh 8100. Videoimages (see Fig. 1b) are 380 nm images (each of which representsthe average of 256 frames).
Fig. 1. Morphological identification of striatal neurons. The figure represents two striatal neuronal subtypes: a biocytin-injectedspiny striatal neuron (a) and a large LA interneuron filled withthe dye fura-2 (b) (380 nm image, average of 256 frames) (fordetails, see Materials and Methods). Scale bar (shown in b): a,70 µm; b, 30 µm.
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Data analysis and drug applications. Values given in the text and in the figures are mean ± SEM of changes in the respectivecell populations. Student's t test (for paired and unpaired observations)was used to compare the means. The characteristics of action potentialsand of current-voltage curves (I-V) in different experimentalconditions were studied by using a fast chart recorder and a digitalsystem (Nicolet System 400: Benchtop Waveform Acquisition System).Drugs were applied by dissolving them to the desired final concentrationin the saline and by switching the perfusion from control salineto drug-containing saline. 6-Cyano-7-nitroquinoxaline-2,3-dione(CNQX) was from Tocris. D-2-amino-5-phosphonovalerate (APV), BAPTA,and tetrodotoxin (TTX) were from Sigma. 8-Cyclopentyl-1,3-dimethylxanthine(CPT) and 1,3-dipropyl-8-cyclopentylxanthine (CPX) were from RBI(Natick, MA). Tolbutamide and glipizide were a gift from Dr. N.B. Mercuri.

RESULTS

Physiological and morphological properties of spiny neurons
We recorded from 197 spiny striatal neurons. In 91 of 197 recorded spiny neurons, the electrophysiological identificationwas confirmed by a morphological analysis obtained by using biocytinstaining (Fig. 1a). These cells had a small soma (10-18 µm) andan extensive dendritic tree studded densely with spines. Thesecells had high resting-membrane potential ( $-$ 84 ± 5 mV), relativelylow apparent input resistance (38 ± 8 M $Omega$ ) when measured at theresting potentials from the amplitude of small (<10 mV) hyperpolarizingelectrotonic potentials, action potentials of short duration (1.1± 0.3 msec), and high amplitude (102 ± 4 mV). These cells weresilent at rest and showed membrane rectification and tonic firingactivity during depolarizing current pulses (Fig. 2C). All ofthe 40 cells studied with voltage-clamp showed prominent inwardrectification in the steady-state I-V relation. When the currentswere evoked by hyperpolarizing command steps, there was no detectabletime-dependent component. Some of these properties have been describedpreviously both in vivo (Preston et al., 1979; Wilson and Groves,1980; Calabresi et al., 1990c; Onn et al., 1994a; Xu, 1995) andin vitro (Kita et al., 1984; Calabresi et al., 1990b, 1991, 1995b;Jiang and North, 1991; Cepeda et al., 1994) and resemble thosereported for intracellularly stained spiny striatal neurons (Prestonet al., 1979; Cepeda et al., 1994; Onn et al., 1994b; Calabresiet al., 1995a).
Fig. 2. Aglycemia depolarizes striatal spiny neurons and decreases their membrane input resistance. A, The top part represents selectedchart records of the membrane potential changes caused by glucosedeprivation. The black arrows indicate the onset of hypoglycemia(a), 15 min of aglycemia (b), the onset of the washout (c), and10 min of washout (d). Interruptions of the traces between twoopen arrows represent different periods of recording: 13 min betweena and b, 13 min between b and c, and 6 min between c and d. Thebottom part shows the current trace monitored during the recording.The downward voltage deflections are induced by negative currentsteps. B, Single sweeps recorded at higher speed at the same timesas those indicated in A. Current and voltage calibrations in Aapply also for B. In Bc, the dotted line indicates the originalresting membrane potential (RMP = $-$ 85 mV). C, The tonic firingdischarge (a) induced by a depolarizing pulse (b) in a striatalspiny cell (RMP= $-$ 86 mV).
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Effects of glucose deprivation on spiny neurons
As shown in Figure 2, periods of glucose deprivation >10 min induced a progressive, slow membrane depolarization. The amplitudeof this depolarization was dependent on the duration of aglycemia(Fig. 3). The aglycemia-induced membrane depolarization was coupledwith a decrease of the apparent input resistance (Fig. 2A,B).At 25 min from the onset of the aglycemic solution the input resistancewas 55 ± 5% (n = 15) of the control value. This effect persistedalso when the membrane was manually clamped to the resting level(n = 7; data not shown). Brief periods (5-10 min) of glucose deprivationdid not cause significant changes of membrane potential and inputresistance. We also studied the effects of aglycemia in single-microelectrodevoltage-clamp experiments. Periods of glucose deprivation >10min induced inward currents associated with an increase in membraneconductance (Figs. 4, 5A,B). These events had a time course similarto that observed in current-clamp experiments. In most of theexperiments, we used a period of glucose deprivation lasting 25min, which produced reversible membrane depolarization/inwardcurrent. In several experiments, a transient overshoot of ~10mV was observed (Fig. 2) on restoration of normal glucose concentration.In six experiments, we also studied effects produced by 40 minof aglycemia. This period of glucose deprivation induced irreversibledeterioration of the membrane properties in all of the recordedneurons (six of six cells; data not shown). As shown in Figure5C, the extrapolated reversal potential for the aglycemia-inducedinward current was $-$ 40 ± 4 mV (n = 7) by using K⁺ chloride-filled electrodes. This value was obtained in voltage-clampexperiments by applying voltage steps (1-3 sec duration) in bothdepolarizing and hyperpolarizing directions. In four experimentsthe intracellular pipette was filled with K⁺ acetate, and the extrapolated reversal potential for the inwardcurrent induced by hypoglycemia was $-$ 41 ± 5 mV (data not shown).
Fig. 3. Time course of the membrane depolarization induced by aglycemia in normal medium and in different experimental conditions.The graphs show the amplitude of the membrane depolarization inducedby 25 min of glucose deprivation in control medium (filled circles),in 1 µM TTX (open circles), in 10 µM CNQX plus 50 µM APV (openrhombs), in low Na⁺ (38 mM, filled rhombs), in the presence of BAPTA-filled electrodes(open squares), in the presence of low calcium (0.5 mM)/high magnesium(10 mM) solutions (filled squares), and in the presence of theadenosine A1 receptor antagonist CPX (300 nM; filled triangles).Each data point represents the mean of at least four single observations.Asterisks indicate significant difference from control values(p < 0.01).
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Fig. 4. Aglycemia induces an inward current and increases the membrane conductance in spiny neurons. A, During a single-microelectrodevoltage-clamp experiment, the voltage was monitored (see top part).The glucose deprivation induced an inward current. The black arrowsindicate the onset of aglycemia (a), 15 min of aglycemia (b),the onset of the washout after 25 min of aglycemia (c), and 10min of washout (d). Interruptions of the traces between two openarrows represent different periods of recording: 14 min betweena and b, 7 min between b and c, and 8 min between c and d. Thedownward deflections are induced by negative current steps. B,This part of the figure shows single sweeps recorded at higherspeed at the same times as those indicated in A. Current and voltagecalibrations in A apply also for B. The holding potential duringthe experiment was $-$ 85 mV.
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Fig. 5. Characteristics of the inward current induced by aglycemia in spiny neurons. A, The graph shows the time course of the inwardcurrent induced by 25 min of glucose deprivation. B, The graphindicates the relative membrane conductance changes caused by25 min of aglycemia. C, I-V relationship showing the extrapolatedreversal potential ( $-$ 40 mV, arrow) of the aglycemia-induced inwardcurrent. Long-lasting (1-3 sec) voltage steps were applied inboth negative and positive directions before (filled circles)and during (open circles) aglycemia. The holding potential was $-$ 80 mV. Each data point represents the mean of at least four singleobservations.
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TTX, low Ca²⁺/high Mg²⁺ medium, and glutamate receptor antagonists on aglycemia-induced depolarization in spiny neurons
To analyze whether the aglycemia-induced membrane depolarization observed in spiny cells was caused by a presynaptic mechanisminvolving an enhanced release of excitatory transmitters, we testedthe effect of the preincubation (10 min before the onset of theglucose deprivation) of the slices in 1 µM TTX. As shown in Figure3, this Na⁺ channel blocker did not affect the membrane depolarization inducedby aglycemia (p > 0.05). To investigate the possible involvementof a TTX-resistant release of excitatory neurotransmitters, westudied the effect of low Ca²⁺ (0.5 mM)/high Mg²⁺ (10 mM) medium on the membrane depolarization induced by aglycemia.Incubation of the slices in low Ca²⁺/high Mg²⁺ solutions did not reduce the aglycemia-induced membrane depolarization(p > 0.05) (Fig. 3). We also tested whether the direct blockadeof postsynaptic glutamate receptors could affect the aglycemia-inducedmembrane depolarization. We incubated (10 min before the onsetof aglycemia) the slices in 10 µM CNQX, an antagonist of AMPAglutamate receptors, plus 50 µM APV, an antagonist of NMDA glutamatereceptor. Even in this experimental condition, aglycemia causedmembrane depolarizations whose amplitude and duration were similarto those observed in control medium (p > 0.05) (Fig. 3). Theseconcentrations of antagonists fully blocked excitatory postsynapticpotentials evoked by activation of glutamatergic corticostriatalfibers in brain slice preparations (Calabresi et al., 1995b, 1996).CPT (1 µM, data not shown; n = 5) and CPX (300 nM; n = 6) (Fig.3), antagonists of A1 adenosine receptors, did not affect themembrane depolarization caused by glucose deprivation (p > 0.05).

External low Na⁺ and intracellular BAPTA on aglycemia-induced membrane depolarization in spiny neurons
To test the possible involvement of a TTX-resistant Na⁺ influx in the membrane depolarization/inward current observed in spinyneurons after glucose deprivation, we studied the effects of aglycemiain low Na⁺-containing solutions (38 mM; see Materials and Methods). Thelowering of the extracellular Na⁺ concentration significantly reduced the aglycemia-induced membranedepolarizations (p < 0.01; n = 6) (Fig. 3) and inward currents(n = 3;, data not shown). In low Na⁺-containing solutions, the reversal potential for the aglycemia-inducedinward current was $-$ 68 mV ± 4 (n = 3).

The dependence of the aglycemia-induced membrane depolarization/inward current on intracellular Ca²⁺ was studied with microelectrodes filled with the Ca²⁺ chelating agent BAPTA (200 mM). As reported previously (Calabresiet al., 1994), 20 min after the intracellular BAPTA injection(performed by applying negative pulses 1 nA in amplitude, 1 secin duration, 0.3 Hz) the long-term depression (LTD) of excitatorysynaptic transmission observed after tetanic stimulation of thecorticostriatal fibers was blocked. This test was performed beforethe glucose deprivation to confirm that the injection of intracellularBAPTA had prevented the rise in internal Ca²⁺ required to trigger the LTD. In fact, striatal spiny neuronshave neither prominent slow afterhyperpolarization nor firingaccommodation (Calabresi et al., 1990b,c); thus the blockade ofthese events by BAPTA could not be used to detect the efficacyof this Ca²⁺ chelator. In BAPTA-injected neurons the aglycemia-induced membranedepolarization was not altered (p > 0.05; n = 6) (Fig. 3). Moreover,in the presence of intracellular BAPTA the inward current inducedby glucose deprivation was unaffected (p > 0.05; n = 3; data notshown).

Physiological and morphological properties of large aspiny interneurons
Twenty-nine recorded cells had electrophysiological characteristics different from those described for spiny neurons and showedproperties that have been attributed previously to large aspinyinterneurons (Wilson et al., 1990; Jiang and North, 1991; Kawaguchi,1992, 1993; Kawaguchi et al., 1995). In 11 of these 29 LA interneuronsthe electrophysiological identification was confirmed by a morphologicalanalysis. This analysis was performed by using either biocytinor fura-2 staining (Fig. 1b). The soma of LA neurons was larger(range, 25-49 µm) than those of spiny cells. The LA interneuronshad polygonal or fusiform cell bodies, and their dendrites didnot show spines. These cells had low membrane potential ( $-$ 60 ±3 mV) and high input resistance (195 ± 55 M $Omega$ ). Spontaneous firingoccurred in 5 of these 29 cells. As shown in Figure 6C, in theseneurons depolarizing current pulses of small amplitude (200-400pA) and short duration (5-30 msec) elicited a single action potentialfollowed by a long-lasting afterhyperpolarization (amplitude 8.9± 9 mV, duration 350 ± 130 msec). The amplitude of the actionpotential was 70.5 ± 3 mV, and the duration of spike at half-amplitudewas 0.71 ± 0.05 msec. The hyperpolarizing electrotonic potentialdeclined after about the first 100 msec (Fig. 6). For this reason,the input resistance values were calculated either from the peakamplitude of the electrotonic potential evoked by a 300-400 pAcurrent pulse or at the steady-state. The decline in the electrotonichyperpolarizing potential was blocked by 2 mM cesium in the externalmedium (n = 4; data not shown). This finding suggests that itmight be attributed to the activation of an I_h current, as hasbeen suggested previously (Jiang and North, 1991).
Fig. 6. Aglycemia hyperpolarizes LA striatal interneurons and decreases their membrane input resistance. A, The top part representsselected chart records of the membrane potential changes causedby glucose deprivation. The black arrows indicate the onset ofaglycemia (a), 10 min of aglycemia (b), the onset of the washout(c), and 10 min of washout (d). Interruptions of the traces betweentwo open arrows represent different periods of recording: 8 minbetween a and b, 3 min between b and c, and 7 min between c andd. The bottom part shows the current trace monitored during therecording. The downward voltage deflections are induced by negativecurrent steps. B, Single sweeps recorded at higher speed at thesame times as indicated in A. In Ac and Bc, the dotted line indicatesthe original resting membrane potential ( $-$ 59 mV). C, A singleaction potential followed by a long-lasting hyperpolarization(a) is induced by a depolarizing current pulse (b) in an LA striatalinterneuron. The dotted line represents the resting membrane potentialof the neuron ( $-$ 59 mV).
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Effects of aglycemia on large aspiny interneurons
Unlike spiny neurons, the large aspiny interneurons (LA cells) were hyperpolarized by glucose deprivation (n = 22) (Fig. 6).This hyperpolarization started about 10 min after the onset ofthe glucose-free solution, and it reversed completely after 10-15min of washout. As shown in Figure 6, the aglycemia-induced hyperpolarizationwas coupled with a reduction of the apparent input resistanceas detected by the decreased amplitude of long-hyperpolarizingpulses. After 25 min of aglycemia the input resistance measuredat the steady-state was 59 ± 5% (n = 9) of the control value.In nine LA interneurons the effect of glucose deprivation wasalso measured by using the single microelectrode voltage-clamptechnique. Under this experimental condition aglycemia producedan outward current associated with an increase of the membraneconductance (Fig. 7). The hyperpolarization generated by glucosedeprivation in LA interneurons was blocked by 300 µM barium (p< 0.001; n = 4) but not by 1 mM tolbutamide (p > 0.05; n = 3)or 100 nM glipizide (p > 0.05; n = 3), blockers of ATP-dependentK⁺ channels (Fig. 8A). TTX (1 µM) did not alter the membrane hyperpolarization(p > 0.05; n = 4; data not shown) or the outward current inducedby aglycemia in large aspiny neurons (p > 0.05; n = 4; data notshown). Incubation of the slices in low Ca²⁺ (0.5 mM)/high Mg²⁺ (10 mM)-containing solutions significantly attenuated the aglycemia-inducedmembrane hyperpolarization but did not block this phenomenon (p< 0.01; n = 4) (Fig. 8). We also evaluated the possible effectof CPT and CPX, antagonists of adenosine A1 receptors, on themembrane hyperpolarization caused by glucose deprivation. NeitherCPT (p > 0.05; n = 3; data not shown) nor CPX (p > 0.05; n = 4)(Fig. 8A) altered the time course of the aglycemia-induced membranehyperpolarization; however, these antagonists blocked the membranehyperpolarization induced by exogenous adenosine (30 µM; n = 3)in a reversible manner (Fig. 8C). The reversal potential of theaglycemia-induced outward current was $-$ 105 ± 5 mV (n = 4) (Fig.8B). This value was calculated by measuring the steady-state currentsgenerated by long-lasting (1-3 sec) voltage steps of progressivelyincreasing amplitude delivered from the resting membrane potentialin hyperpolarizing direction before and during the applicationof glucose-free medium.
Fig. 7. Aglycemia induces an outward current and increases the membrane conductance in LA striatal interneurons. A, During a single-microelectrodevoltage-clamp experiment, aglycemia caused an outward current(top part); during the experiment the voltage was monitored (seebottom part). The black arrows indicate the onset of aglycemia(a), the onset of the washout after 15 min of aglycemia (b), and10 min after the washout (c). The interruption of the traces betweentwo open arrows represents a period of recording of 12 min. Thedownward deflections are induced by negative current steps. B,Single sweeps recorded at higher speed at the same times as indicatedin A. The holding potential during the experiment was $-$ 60 mV.
[View Larger Version of this Image (34K GIF file)]

Fig. 8. The aglycemia-induced hyperpolarization/outward current in LA interneurons is mediated by a K⁺ conductance. A, Time course of the membrane changes induced by25 min of glucose deprivation in different experimental conditions:control (n = 9; filled circles), 300 µM barium (n = 4; open circles),1 mM tolbutamide (n = 3; open rhombs), 100 nM glipizide (n = 3;filled squares), 300 nM CPX (n = 4; open squares), and low calcium(0.5 mM)/high magnesium (10 mM) solutions (n = 4; filled rhombs).Asterisks indicate significant difference from control values(p < 0.01). B, In an LA interneuron, bath application of 30 µMadenosine induced a membrane hyperpolarization (a); this membranehyperpolarization was fully blocked by 300 nM CPX, an adenosineA1 receptor antagonist (b); after the washout of this antagonist,the hyperpolarizing action of adenosine was restored (c). C, Thereversal potential of the aglycemia-induced outward current isindicated by the arrow ( $-$ 105 mV; n = 4). This value was calculatedby measuring the steady-state currents generated by long-lasting(1-3 sec) voltage steps of progressively increasing amplitudefrom the holding potential ( $-$ 60 mV; n = 4) before (filled circles)and during glucose deprivation (25 min, open circles).
[View Larger Version of this Image (25K GIF file)]

DISCUSSION
The main finding of the present study is that glucose deprivation causes opposite membrane potential changes in striatal spinyneurons and in large aspiny interneurons. Spiny neurons are depolarizedby aglycemia, whereas large aspiny interneurons are hyperpolarizedby glucose deprivation. These different electrophysiological responsesmay account for the differential neuronal vulnerability observedin these neuronal subtypes after aglycemia and ischemia.

Spiny neurons are depolarized by glucose deprivation
The large majority of striatal neurons is represented by spiny projecting cells whose anatomical, physiological, and pharmacologicalproperties have been widely characterized (Graybiel, 1990; Smithand Bolam, 1990; Surmeier and Kitai, 1994; Calabresi et al., 1996).These small GABAergic cells are highly vulnerable to transientforebrain ischemia (Brierley, 1976; Pulsinelli et al., 1982; Xu,1995), energy metabolism failure (Beal, 1992, 1995), and aglycemiccoma (Auer et al., 1984; Kristian et al., 1995). Accordingly wehave found that glucose deprivation depolarizes spiny neurons.Periods of aglycemia <30 min cause reversible membrane potentialchanges; however, when aglycemia lasts >30 min, the membrane depolarizationis irreversible. The aglycemia-induced membrane depolarizationis coupled with a decreased input resistance. In voltage-clampmode, aglycemia generates an inward current associated with anincreased conductance. TTX does not alter the amplitude or thetime course of the aglycemia-induced depolarization. Low-Na⁺-containing solutions significantly reduce the amplitude of thedepolarization caused by glucose deprivation. A TTX-resistantCa²⁺-activated nonspecific cationic current has been reported to actas a depolarizing driving force in neurons of invertebrates (Hofmeierand Lux, 1981) and in rat hippocampal neurons (Crepel et al.,1994). The finding that the aglycemia-induced depolarization isnot altered by the intracellular injection of BAPTA, however,does not support the involvement of a Ca²⁺-activated conductance in the aglycemia-induced effects. Thereseems to be a discrepancy between the equilibrium potential forNa⁺ ions and the reversal potential of the aglycemia-induced inwardcurrent in spiny neurons that is inconsistent with the involvementof a conductance generated exclusively by Na⁺ ions. On the basis of an extrapolated I-V plot (Fig. 5C), thiscurrent apparently reverses at approximately $-$ 40 mV. Given theionic composition of the medium, the equilibrium potential forNa⁺ ions should be approximately +50 mV, whereas the equilibriumpotential for K⁺ ions should be approximately $-$ 105 mV (assuming [K]i = 160 mM).Therefore, a reversal potential of approximately $-$ 40 mV mightindicate a nonselective cation conductance or the combinationof independent Na⁺ and K⁺ conductance. In either case, the reduction of the extracellularNa⁺ concentration to 38 mM (30% of the control) will reduce the equilibriumpotential for Na⁺ ions to approximately +34 mV and thereby change the reversalpotential of a mixed cation conductance to approximately $-$ 70 mV.This potential is very close to the value that we obtained inour experiments by using low Na⁺-containing medium ( $-$ 68 mV). It has to be stressed that on therestoration of normal glucose concentration a transient membranepotential overshoot of ~10 mV was observed. This phenomenon mayreveal that several compensatory currents are at play that havedifferent rates of recovery. This evidence might also supportthe idea that the inconsistency between the reversal potentialof the aglycemia-induced current and the equilibrium potentialfor Na⁺ ions is explained by a second, opposing K⁺ current. Interestingly, an increase of the extracellular K⁺ concentration associated with a decreased intracellular concentrationof this ion has been reported in some neuronal subtypes duringenergy deprivation (Jiang and Haddad, 1991; for review, see Martinet al., 1994). Conversely, the participation of chloride ionsin the aglycemia-induced inward current is ruled out, becausethe reversal potential of this current is not changed by usingmicroelectrodes filled with K⁺ acetate instead of K⁺ chloride.

The evidence that low Ca²⁺/high Mg²⁺ solutions did not reduce the aglycemia-induced membrane depolarization rules out the possibleinvolvement of presynaptic mechanisms in this electrophysiologicalphenomenon. Moreover, our experiments showing the lack of effectof CNQX and APV on the aglycemia-induced electrophysiologicalactions clearly indicate that activation of ionotropic glutamatereceptors is not involved in the aglycemia-induced depolarization/inwardcurrent. It has already been shown that glutamate receptor antagonistsfail to alter anoxia-induced membrane depolarization in striatalspiny neurons (Calabresi et al., 1995b) and in brainstem neurons(Haddad and Jiang, 1993). It is possible, however, that althoughexcitatory amino acids are not involved in the "acute" effectsof glucose deprivation, they may play a role in the "delayed neuronaldeath" (Choi, 1990; Choi and Rothmann, 1990). Accordingly, lesionsof the glutamatergic corticostriatal projections in the rat ameliorateaglycemic brain damage in the striatum (Wieloch et al., 1985),and the blockade of NMDA receptors prevents the aglycemia-inducedneuronal damage (Wieloch, 1985).

We have observed recently that brief periods (5-10 min) of aglycemia cause presynaptic inhibition at corticostriatal synapses.This effect is mediated by the release of endogenous adenosineacting on A1 receptors located on corticostriatal glutamatergicterminals (our unpublished observations). Endogenous adenosine,however, does not seem to be involved in the postsynaptic changesobserved in spiny neurons during aglycemia, because A1 receptorantagonists affected neither the amplitude nor the time courseof the membrane depolarization caused by glucose deprivation.

Large aspiny interneurons are hyperpolarized by glucose deprivation
The development of cytochemical approaches to identification and classification of interneurons has recently been combinedwith the physiological analysis of the basic cellular propertiesof the various subtypes of interneurons (for review, see Kawaguchiet al., 1995). We have studied the membrane responses to glucosedeprivation of large aspiny interneurons that have the electrophysiologicalproperties of LA cells (Jiang and North, 1991; Kawaguchi, 1992,1993). These cells are considered cholinergic interneurons. Theyreceive glutamatergic and dopaminergic inputs and provide an intrinsiccholinergic innervation to spiny neurons. The response of LA interneuronsto glucose deprivation is qualitatively different from the effectsobserved in spiny neurons. In fact, LA cells respond to aglycemiawith a membrane hyperpolarization coupled with a decrease of theinput resistance. The voltage-clamp analysis has revealed thatthe hyperpolarization induced by glucose deprivation in thesecells is caused by an outward current that reversed at the K⁺ equilibrium potential. The finding that this outward currentis blocked by barium suggests further that it is caused by theactivation of a K⁺-mediated conductance. Moreover, the lack of effect of TTX onthe membrane hyperpolarization/outward current-generated aglycemiasuggests that this electrophysiological effect is not dependenton a TTX-sensitive release of transmitters. We found that lowCa²⁺/high Mg²⁺-containing solutions significantly reduced but did not blockthe aglycemia-induced membrane hyperpolarization. This findingmight have two possible explanations. 1) A component of the K⁺ conductance generating the aglycemia-induced membrane hyperpolarizationis Ca²⁺-dependent, and 2) a Ca²⁺-dependent, TTX-insensitive release of transmitters plays a rolein this membrane hyperpolarization. This observation, however,demonstrates clearly that at least part of the aglycemia-inducedmembrane hyperpolarization is postsynaptically mediated. Interestingly,tolbutamide and glipizide fail to block the membrane hyperpolarization/outwardcurrent induced by glucose deprivation in LA cells, suggestingthat at least in our experimental condition the activation ofATP-sensitive K⁺ channels does not play a prominent role in the electrophysiologicaleffects induced by glucose deprivation. Membrane potential changesobserved in LA interneurons strongly resemble those observed indorsolateral septal nucleus neurons during aglycemia (Shoji, 1992),in which glucose deprivation causes K⁺-dependent membrane hyperpolarizations that are not affected byinhibitors of ATP-dependent K⁺ channels.

Extracellular levels of adenosine increase during energy deprivation caused by either anoxia or aglycemia (Martin et al.,1994). Because adenosine has been reported to hyperpolarize variousneuronal subtypes by activating K⁺ channels (Greene and Haas, 1991), we have studied the possibleinvolvement of endogenous adenosine in the aglycemia-induced membranehyperpolarization. Antagonists of adenosine A1 receptors fullyblocked the membrane hyperpolarization induced by exogenous adenosine,but they failed to affect the hyperpolarizing action of aglycemia,suggesting that endogenous adenosine does not play a prominentrole in the membrane potential changes observed during glucosedeprivation.

The membrane hyperpolarization observed during glucose deprivation in large LA interneurons might represent a protective mechanismactivated when energy metabolism fails. This hypothesis can alsoexplain previous morphological results showing that although spinyneurons are highly vulnerable to transient forebrain ischemia(Brierley, 1976; Pulsinelli et al., 1982), energy metabolism failure(Beal, 1992, 1995), and aglycemic coma (Auer et al., 1984; Kristianet al., 1995), large cholinergic interneurons are spared duringthese pathological events (Francis and Pulsinelli, 1982; Pulsinelli,1985; Chesselet et al., 1990). Our observation, however, doesnot exclude the possibility that a reduced expression of excitatoryamino acid receptor subtypes or an enhanced activity of protectivetrophic factors or both might also account for the relative viabilityof large cholinergic interneurons to hypoxic-ischemic insults(Burke and Kenyon, 1991; Nakao et al., 1995).

FOOTNOTES

Received Oct. 21, 1996; revised Jan. 2, 1997; accepted Jan. 7, 1997.

This work was supported by Consiglio Nazionale delle Ricerche grants to P.C. and G.B. We thank G. Gattoni and M. Tolu forexcellent technical assistance.

Correspondence should be addressed to Paolo Calabresi, Clinica Neurologica, Dip. Sanitá, Universitá di Roma Tor Vergata,Via O. Raimondo 8, 00173 Rome, Italy.

Dr. C. Magarinos Ascone's present address: Hopital Ramon Y Cajal, Servicio de Neurologia Experimental, Madrid, Spain.

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Volume 17, Number 6, Issue of March 15, 1997 pp. 1940-1949 Copyright ©1997 Society for Neuroscience

Opposite Membrane Potential Changes Induced by Glucose Deprivation in Striatal Spiny Neurons and in Large Aspiny Interneurons

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Volume 17, Number 6, Issue of March 15, 1997 pp. 1940-1949
Copyright ©1997 Society for Neuroscience