Ethanol Dual Modulatory Actions on Spontaneous Postsynaptic Currents in Spinal Motoneurons

doi:10.1152/jn.00614.2002

Ethanol Dual Modulatory Actions on Spontaneous Postsynaptic Currents in Spinal Motoneurons

Lea Ziskind-Conhaim, Bao-Xi Gao, and Christopher Hinckley

Department of Physiology and Center for Neuroscience University of Wisconsin Medical School, Madison, Wisconsin 53706

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Ziskind-Conhaim, Lea, Bao-Xi Gao, and Christopher Hinckley. Ethanol Dual Modulatory Actions on Spontaneous Postsynaptic Currents in Spinal Motoneurons. J. Neurophysiol. 89: 806-813, 2003. Recently we have shown that acute ethanol (EtOH) exposure suppresses dorsal root-evoked synaptic potentials in spinal motoneurons.To examine the synaptic mechanisms underlying the reduced excitatoryactivity, EtOH actions on properties of action potential-independentminiature excitatory and inhibitory postsynaptic currents (mEPSCsand mIPSCs) were studied in spinal motoneurons of newborn rats.Properties of mEPSCs generated by activation of N-methyl-D-aspartatereceptors (NMDARs) and non-NMDA receptors and of mIPSCs mediatedby glycine and $gamma$ -aminobutyric acid-A receptors (GlyR and GABA_AR)were examined during acute exposure to 70 and 200 mM EtOH. Inthe presence of 70 mM EtOH, the frequency of NMDAR- and non-NMDAR-mediatedmEPSCs decreased to 53 ± 5 and 45 ± 7% (means ± SE) of controlvalues, respectively. In contrast, the frequency of GlyR- andGABA_AR-mediated mIPSCs increased to 138 ± 15 and 167 ± 23% ofcontrol, respectively. Based on the quantal theory of transmitterrelease, changes in the frequency of miniature currents are correlatedwith changes in transmitter release, suggesting that EtOH decreasedpresynaptic glutamate release and increased the release of bothglycine and GABA. EtOH did not change the amplitude or rise anddecay times of either mEPSCs or mIPSCs, indicating that the presynapticchanges were not associated with changes in the properties ofpostsynaptic receptors/channels. Acute exposure to 200 mM EtOHincreased mIPSC frequency two- to threefold, significantly higherthan the increase induced by 70 mM EtOH. However, the decreasein mEPSC frequency was similar to that observed in 70 mM EtOH.Those findings implied that the regulatory effect of EtOH on glycineand GABA release was dose-dependent. Exposure to the higher EtOHconcentration had opposite actions on mEPSC and mIPSC amplitudes:it attenuated the amplitude of NMDAR- and non-NMDAR-mediated mEPSCsto ~80% of control and increased GlyR- and GABA_AR-mediated mIPSCamplitude by ~20%. EtOH-induced changes in the amplitude of postsynapticcurrents were not associated with changes in their basic kineticproperties. Our data suggested that in spinal networks of newbornrats, EtOH was more effective in modulating the release of excitatoryand inhibitory neurotransmitters than changing the propertiesof their receptors/channels.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

EtOH, a potent modulator of synaptic transmission, affects neural network function by interacting with a spectrum of specificmembrane proteins that initiate cellular signal transduction processes(reviewed by Faingold et al. 1998; Weight 1992). In a varietyof neuronal preparations, it modulates both excitatory and inhibitorysynaptic transmission, reducing glutamate-mediated excitationand increasing GABA-, glycine-, and adenosine-mediated inhibition(reviewed by Crews et al. 1996; Narahashi et al. 2001; Peopleset al. 1996). Its dual modulatory action on nicotinic acetylcholinereceptors resulted in depressing or facilitating acetylcholine-mediatedcurrents depending on the composition of the receptor subunits(Aistrup et al. 1999).

Glutamate receptors, the major excitatory receptors in the CNS, consist of three ionotropic receptor subtypes: N-methyl-D-aspartate(NMDA), $alpha$ -amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid (AMPA),and kainate receptors. Until recently the general consensus wasthat NMDA receptors (NMDAR) are the primary targets of EtOH becauseat relatively low concentrations, it antagonizes NMDAR-mediatedresponses in a diverse populations of neurons (Lima-Lindman andAlbuquerque 1989; Lovinger et al. 1990; Morrisett and Swartzwelder1993; reviewed by Faingold et al. 1998; Li et al. 2002; Tabakoffand Hoffman 1996; Woodward 2000). NMDA receptor sensitivity toEtOH is regulated by its subunit composition, but factors suchas phosphorylation also play important role in modulating EtOHsensitivity (reviewed by Woodward 2000). The effect of EtOH onnon-NMDA receptors is somewhat controversial (Crews et al. 1996;Lovinger 1997), but in spinal and cortical neurons, NMDAR- andnon-NMDAR-mediated synaptic events are similarly affected by EtOHinhibitory actions (Wang et al. 1999, Wirkner et al. 2000).

Numerous studies have demonstrated that EtOH-induced intoxication is correlated with its interaction with $gamma$ -aminobutyric acid-A(GABA_A) receptors (reviewed by Crews et al. 1996). In isolatedbrain preparations and cultured neurons, EtOH increases GABA_Areceptor-mediated Cl conductance (Aguayo 1990; Celentano et al. 1988; Nestores 1980;Reynolds and Prasad 1991), and similarly it potentiates glycine-mediatedCl flux in synaptoneurosomes (Engblom and Åkerman 1991) and enhancesglycine currents generated in hippocampal neurons (Aguayo andPancetti 1994). A comparison between EtOH actions on glycine-and GABA-mediated Cl currents in dissociated spinal neurons indicated that glycinereceptors are more sensitive to EtOH than GABA receptors (Celentanoet al.1988). It has been proposed that GABA_A and glycine receptorsensitivity to EtOH depends primarily on the expression of the $alpha$ 1 receptor subunit (Eggers et al. 2000; Mascia et al. 1996).

In addition to EtOH opposite actions on excitatory and inhibitory neurotransmitter receptors, its dual effects on presynapticrelease of excitatory and inhibitory neurotransmitters have alsobeen documented. EtOH inhibits NMDAR-mediated glutamate releasein the rat striatum (Carboni et al. 1993), and in the hippocampus,it suppresses high-K⁺-evoked release of endogenous glutamate, aspartate, and GABA (Martinand Swartzwelder 1992). In contrast, EtOH increases the frequencyof action potential-independent glycinergic currents in hypoglossalmotoneurons, implying that it increases presynaptic glycine release(Eggers et al. 2000).

We have demonstrated that EtOH suppresses motoneuron electrical activity by reducing motoneuron excitability, decreasing theamplitude of dorsal root-evoked excitatory postsynaptic potentialsand decreasing the frequency of spontaneous excitatory postsynapticcurrents, while increasing the frequency of inhibitory postsynapticcurrents (Cheng et al. 1999). In that study, spontaneous excitatoryand inhibitory currents were recorded concurrently; thereforeit is conceivable that EtOH action partly resulted from modifyingthe synaptic interaction between those currents rather than directlyinfluencing excitatory and inhibitory synaptic transmission (Marszalecet al. 1998). In this study, properties of pharmacologically isolatedaction potential-independent postsynaptic currents were examinedto determine EtOH effects on action potential-independent presynapticrelease of glutamate, glycine, and GABA and its modulatory actionson postsynaptic NMDA, non-NMDA, glycine, and GABA_A receptors/channels.

A preliminary report of this study was published in an abstract form (Gao and Ziskind-Conhaim 2000).

	METHODS

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Spinal cord preparation

Lumbar spinal cords were isolated from 1- to 4-day old postnatal Sprague-Dawley rats (P1-4). The procedure for spinal corddissection was similar to that described previously (Gao and Ziskind-Conhaim1998; Ziskind-Conhaim 1990). Postnatal rats were anesthetizedby hypothermia. The lumbar region of the spinal cord was removedand placed in oxygenated cold dissection solution. The dissectionsolution contained (in mM): 113 NaCl, 3 KCl, 1 CaCl₂, 6 MgCl₂,25 NaHCO₃, 1 NaH₂PO₄, and 11 glucose (pH 7.2-7.4). The isolatedspinal cord was embedded in agar (2% in extracellular solution).Transverse slices, 350 µm thick, were cut using a Vibratome (TechnicalProducts International). Prior to whole cell recordings, sliceswere incubated in extracellular solution at room temperature for30-60 min. The extracellular solution contained (in mM): 113 NaCl,3 KCl, 2 CaCl₂, 1 MgCl₂, 25 NaHCO₃, 1 NaH₂PO₄, and 11 glucose.The solution was equilibrated with 95% O₂-5% CO₂ (pH 7.2 at 20-22°C).

Whole cell recording

Slices were transferred into a recording chamber, which was mounted on the stage of an upright microscope and were superfusedwith aerated extracellular solution at room temperature (20-22°C).Large neurons in the medial and lateral ventral horn were visualizedusing infrared DIC optics, and those were assumed to be motoneurons.Whole cell patch-clamp recordings in motoneurons were performedusing patch electrodes pulled to tip resistances of 3-5 M $Omega$ usinga multi-stage puller (Sutter Instruments). Electrodes were filledwith solution containing (in mM): 149 CsCl, 10 HEPES, 0.2 EGTA,1 Mg-ATP, and 0.1 GTP. The solution was adjusted to pH 7.2 usingCsOH, and the osmolarity was 290 mosM. Typically, the series resistancewas two- to threefold higher than the pipette resistance. Experimentswere rejected if the series resistance changed >15%.

Action potential-independent miniature excitatory and inhibitory postsynaptic currents (mEPSCs and mIPSCs) were recorded inthe presence of TTX (1 µM). At P1-4, mEPSC and mIPSC frequencieswere 0.5 and 0.3 Hz, respectively (Gao et al. 1998), and the frequenciesof pharmacologically isolated NMDAR- and non-NMDAR-mediated mEPSCsand GlyR- and GABA_AR-mediated mIPSCs were ~50% lower. Thereforeto acquire a large sample of mEPSCs and mIPSCs for statisticalanalysis, experiments were performed in high extracellular K⁺ (18 mM, Gao et al. 1998, 2001). Synaptic currents were recordedusing an Axopatch 200A amplifier (Axon Instruments). Currentswere filtered at 1 kHz, digitized at 5 kHz, and stored on a diskfor later analysis. In most motoneurons, continuous recordingswere carried out until >100 events wererecorded.

Data analysis

The threshold for detection of miniature currents was set at 2 pA above the background noise. The average noise SD was 1.7pA at -60 mV (see also Gao et al. 2001), not significantly differentfrom the 1.9 pA measured at +40 mV. mEPSCs and mIPSCs were measuredusing Mini Analysis software (Synaptosoft). Kinetic analysis wasperformed on averaged miniature currents, which were obtainedby lining up the rising phase of single currents. In most motoneurons,>100 events were averaged. Kinetic analysis included: peak amplitude,rise time from 10 to 90% peak amplitude and decay time constant(decay $tau$ ). Typically, the time course of decay of mEPSCs and mIPSCswas best fitted with the sum of two exponentials. Data are presentedas means ± SE. Student's t-test was used to determine the statisticalsignificance (P < 0.05).

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

EtOH modulation of mEPSC and mIPSC properties was examined in spinal motoneurons of P1-4 rats. Acute EtOH exposure does notsignificantly change the properties of dorsal root-evoked potentialsat concentrations <70 mM (Cheng et al. 1999). To determine whetherlower EtOH concentration altered the properties of action potential-independentminiature synaptic currents, mEPSC and mIPSC frequencies and amplitudeswere examined during a 10- to 15-min exposure to 30 mM EtOH (n= 4). At that concentration, EtOH did not alter mEPSC and mIPSCfrequencies (not shown), confirming our previous findings thathigher EtOH concentrations were required to significantly reduceexcitatory synaptic transmission and motoneuron excitability innewly formed spinal networks (Cheng et al. 1999). Therefore inthis study, EtOH actions on pharmacologically isolated miniaturesynaptic currents were examined only at higher concentrationsof 70 and 200mM.

EtOH decreased mEPSC frequency and increased mIPSC frequency

Glutamate-mediated mEPSCs were recorded in the presence of strychnine (0.5 µM) and bicuculline (5 µM), glycine, and GABA_Areceptor antagonists, respectively. mEPSCs were recorded at aholding potential (HP) of +40 mV to remove the voltage-dependentMg²⁺ block of NMDA channels. Some experiments were initially carriedout at a HP of -60 mV, and Mg²⁺ was omitted from the extracellular solution (see following text).However, because of the possibility that Mg²⁺ modulated presynaptic release, mEPSC properties were analyzedonly when recorded at +40mV.

At +40 mV, mEPSCs were recorded as outward currents (Fig. 1), and consisted of a mixed population of fast-rising, fast-decayingnon-NMDAR-mediated mEPSCs and slow-rising, slow-decaying NMDAR-mediatedmEPSCs. A third subpopulation of dual-component mixed fast- andslow-decaying mEPSCs was also apparent, and it was assumed thatthose were generated by co-activation of NMDA and non-NMDA receptors.Pharmacologically isolated non-NMDAR-mediated mEPSCs were recordedin the presence of D-2-amino-5-phosphonovaleric acid (D-APV, 20µM), a NMDA receptor antagonist (Fig. 2). NMDAR-mediated mEPSCswere recorded in the presence of 6-cyano-7-nitroquinoxaline-2,3-dione(CNQX, 5-10 µM), an AMPA/kainate receptors antagonist (Fig. 3).

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Fig. 1. Ethanol, EtOH reversibly suppressed the frequency of miniature excitatory postsynaptic currents (mEPSCs) in a P4 motoneuron. A: traces of continuously recorded mEPSCs before (control), during EtOH exposure (EtOH) and after the removal of EtOH from the extracellular solution (wash). mEPSC frequency decreased from 3.7 Hz before EtOH application to 3.0 Hz in its presence. mEPSC frequency of 3.2 Hz was recorded 20 min after EtOH removal. B: mEPSC frequency and amplitude during EtOH exposure (% of control) and after its removal. EtOH significantly suppressed mEPSC frequency to 84 ± 6% of control (P < 0.04), and the frequency increased to 91 ± 6% of control 20 min after EtOH removal. The averaged amplitude did not significantly change, decreasing to 86 ± 4% of the control value (P < 0.07) in the presence of EtOH and increasing to 101 ± 8% after its removal. Values are means ± SE of 6 motoneurons.

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Fig. 2. EtOH significantly reduced the frequency of fast-decaying nonN-methyl-D-aspartate receptor (non-NMDAR)-mediated mEPSCs, without changing mEPSC amplitudes and basic kinetic properties. Top: traces of continuously recorded mEPSCs in a P4 motoneuron before and during a brief exposure to 70 mM EtOH. Bottom left: amplitude distributions of non-NMDAR-mediated mEPSCs recorded in control and EtOH-containing solution. mEPSC amplitudes >45 pA are not shown. Mean peak amplitudes were 16.5 (control) and 15.0 pA (EtOH). mEPSC frequency decreased from 0.6 Hz before EtOH application to 0.2 Hz in its presence. Bottom right: averaged non-NMDAR-mediated mEPSCs before and during EtOH exposure (control mEPSCs, n = 373; EtOH mEPSCs, n = 134). Overlapping currents were not averaged.

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Fig. 3. EtOH significantly reduced the frequency of slow-decaying NMDAR-mediated mEPSCs but did not change mEPSC amplitudes and basic kinetic properties. Top: traces of continuously recorded mEPSCs in a P3 motoneuron before EtOH application and in its presence (70 mM). Bottom left: amplitude distributions of NMDAR-mediated mEPSCs before and during EtOH exposure. mEPSC amplitudes >25 pA are not shown. Mean peak amplitudes were 10.6 and 10.7 pA before and after EtOH exposure, respectively. mEPSC frequency was reduced from 0.4 Hz (control) to 0.2 Hz (EtOH). Bottom right: averaged NMDAR-mediated mEPSCs before and during EtOH exposure (control mEPSCs, n = 192; EtOH mEPSCs, n = 79).

mIPSCs were recorded in the presence of D-APV (20 µM) and CNQX (5-10 µM), and at a HP of -60 mV they appeared as inward currents(Cl equilibrium potential was approximately $-$ 5 mV). Based on theirkinetic properties, mIPSC population consisted of three groups:fast-decaying glycinergic mIPSCs, slow-decaying GABAergic mIPSCs,and dual-component, fast-slow-decaying mixed glycine-GABA-mediatedmIPSCs (Gao et al. 2001). Pharmacologically isolated GlyR-mediatedmIPSCs were recorded in the presence of bicuculline (5 µM, Fig.4), and GABA_AR-mediated mIPSCs were recorded in the presence ofstrychnine (0.5 µM, Fig. 5).

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Fig. 4. EtOH significantly increased the frequency of fast-decaying glycine receptor (GlyR)-mediated miniature inhibitory postsynaptic currents (mIPSCs), without changing mIPSC basic kinetic properties. Top: traces of continuously recorded mIPSCs in a P4 motoneuron before and during exposure to 70 mM EtOH. Bottom left: amplitude distributions of GlyR-mediated mIPSCs in control and EtOH-containing solution. mIPSC frequency increased from 0.6 Hz (control) to 0.9 Hz (EtOH). mIPSC amplitudes >65 pA are not shown. Mean peak amplitudes were 18.3 (control) and 25.1 pA (EtOH), the largest amplitude increase induced by 70 mM EtOH. Bottom right: averaged GlyR-mediated mIPSCs before and during EtOH exposure (control mIPSCs, n = 194; EtOH mIPSCs, n = 253). The large EtOH-induced increase in the amplitude of GlyR-mediated mIPSCs was not associated with changes in their rise time and decay time constants.

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Fig. 5. EtOH significantly increased the frequency of slow-decaying GABA_AR-mediated mIPSCs but did not change mIPSC amplitudes and basic kinetic properties. Top: traces of continuously recorded mIPSCs in a P3 motoneuron before EtOH application and in its presence (70 mM). Bottom left: amplitude distributions of GABA_AR-mediated mIPSCs before and during EtOH exposure. mIPSC amplitudes larger than 130 pA are not shown. Mean peak amplitude increased from 35.5 (control) to 36.5 pA (EtOH). mIPSC frequency increased from 0.2 Hz (control) to 0.6 Hz (EtOH), with a significant number of overlapping currents. Bottom right: averaged GABA_AR-mediated mIPSCs before and during EtOH exposure (control mIPSCs, n = 111; EtOH mIPSCs, n = 161).

A brief (10-15 min) exposure to 70 mM EtOH reversibly suppressed mEPSC frequency to ~50% of control (Figs. 1-3). The frequencyof non-NMDAR-mediated mEPSCs was significantly reduced from 0.64± 0.16 Hz (SE, n = 8) before EtOH exposure to 0.29 ± 0.11 Hz inits presence and that of NMDAR-mediated mEPSCs decreased from0.51 ± 0.13 Hz (n = 11) to 0.27 ± 0.09 Hz (Fig. 6). Opposite modulatoryaction was apparent on mIPSC frequency, significantly increasingthe frequency of GlyR- and GABA_AR-mediated mIPSCs to 138 ± 15%(n = 8) and 167 ± 23% (n = 9) of control, respectively (Fig. 6).Although we cannot rule it out, it is unlikely that the apparentreduction in mEPSC frequency reflected a failure to detect currentsthat decreased in amplitude during EtOH exposure. EtOH did notsignificantly change mEPSC amplitude distributions (Figs. 2 and3), and small mEPSCs (2.5-6 pA) constituted only a small fractionof mEPSC population. Therefore even if EtOH acted on postsynapticglutamatergic receptors to reduce the amplitude of the small currentsbelow the level of detection, it could not have accounted forthe 50% reduction in mEPSC frequency.

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Fig. 6. The frequency of non-NMDAR- and NMDAR-mediated mEPSCs significantly decreased and the frequency of GlyR- and GABA_AR-mediated mIPSCs significantly increased during EtOH exposure (70 mM). At this concentration, EtOH did not significantly alter mEPSC and mIPSC amplitudes. Averages ± SE of 8 and 11 motoneurons for non-NMDAR- and NMDAR-mediated mEPSCs, respectively, and 8 and 9 motoneurons for GlyR- and GABA_AR-mediated mIPSCs.

At this concentration, EtOH did not significantly alter the amplitude or rise and decay times of either mEPSCs or mIPSCs.The mean amplitude of non-NMDAR-mediated mEPSCs was 18.3 ± 1.1pA before EtOH application and 16.7 ± 1.2 pA in its presence andthat of NMDAR-mediated mEPSCs changed from 11.2 ± 1.8 to 11.8± 1.8 pA (Fig. 6). It is conceivable that small mEPSCs were notdetected at a HP of +40 mV because of a potential leak, whichcould have masked changes in mEPSC amplitudes during EtOH exposure.However, at a HP of -60 mV (extracellular Mg²⁺ was omitted), the mean amplitude of non-NMDAR-mediated mEPSCswas 18.9 ± 2.1 pA (n = 5) and that of NMDAR-mediated mEPSCs was11.6 ± 1.6 (n = 4), not significantly different from those recordedat +40 mV. Therefore it is unlikely that the failure to detectchanges in mEPSC amplitudes resulted from the inability to recordsmall currents at a HP of +40mV.

The amplitude of GlyR- and GABA_AR-mediated mIPSCs increased ~10% during EtOH exposure. Our recent study has demonstrated thatEtOH does not significantly change motoneuron membrane resistance(Cheng et al. 1999), therefore it is unlikely the inability todetect changes in mEPSC and mIPSC amplitudes resulted from a decreasein membrane resistance during EtOHexposure.

Our findings that EtOH changed the frequency but not amplitude of mEPSCs and mIPSCs implied that acute exposure to 70 mM EtOHmodulated presynaptic release of glutamate, glycine, and GABAwithout changing the properties of their postsynaptic receptors/channels.

High EtOH concentration reduced mEPSC amplitude and increased mIPSC amplitude

To determine whether the amplitude and basic kinetic properties of mEPSCs and mIPSCs were modulated by high EtOH concentration,current properties were examined in the presence of 200 mM EtOH.The ~30% decrease in mEPSC frequency (Table 1) was similar tothe reduction induced by 70 mM EtOH, indicating that the lowerconcentration produced a maximal inhibitory effect on mEPSC frequency.At that concentration, the decrease in mEPSC frequency was associatedwith a significant decrease in mEPSC amplitude, with a reductionof ~20% in the amplitude of both NMDAR- and non-NMDAR-mediatedmEPSCs (Table 1). EtOH-induced amplitude attenuation was notassociated with changes in basic kinetic properties of glutamate-mediatedmEPSCs.

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Table 1. Acute exposure to 200 mM EtOH significantly decreased the frequency and amplitude of non-NMDAR- and NMDAR-mediated mEPSCs

mIPSC frequency increased two- to threefold during the exposure to 200 mM EtOH (Table 2), significantly higher than the increaseinduced during the exposure to 70 mM EtOH. This effect was reversibleon removal of EtOH from the extracellular solution (Fig. 7). Thesedata demonstrated that unlike its inhibitory action on mEPSC frequency,EtOH facilitatory action on mIPSC frequency was dose-dependent.At the higher concentration EtOH induced an ~20% increase in theamplitude of both GlyR- and GABA_AR-mediated mIPSCs, but it didnot affect mIPSC basic kinetic properties (Table 2).

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Table 2. Changes in mIPSC properties during acute exposure to 200 mM EtOH

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Fig. 7. mIPSC frequency and amplitude significantly increased during acute exposure to 200 mM EtOH. A: continuously recorded mIPSCs in a P3 motoneuron before (control), in the presence of EtOH (EtOH) and after its removal (wash). mIPSC frequency was 1.4 Hz and the mean amplitude was 94.7 pA before EtOH application and 4.6 Hz and 136 pA in its presence. EtOH effects were partially reversible and the frequency and amplitude decreased to 0.9 Hz and 45.4 pA after its removal. B: mIPSC frequency and amplitude during EtOH exposure (% of control) and after its removal. EtOH significantly increased mIPSC frequency to 295 ± 73% of control (P < 0.01), and the frequency decreased to 70 ± 18% of control 20 min after EtOH removal. The averaged amplitude increased to 142 ± 29% of control in the presence of EtOH and decreased to 80 ± 20% after its removal. Values are means ± SE of 4 motoneurons.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

This study demonstrated that EtOH shifted the balance between excitation and inhibition toward inhibition by modulating bothpre- and postsynaptic mechanisms underlying spontaneous synaptictransmission. EtOH dominant action was to increase high-K⁺-induced mIPSC frequency and depress mEPSC frequency, probablyreflecting an increase in glycine and GABA release and a suppressionof glutamate release. The dual presynaptic effects might contributeto EtOH-induced attenuation of dorsal root evoked potentials inspinal motoneurons (Cheng et al. 1999; Wang et al. 1999). At highconcentrations, presynaptic modulation was associated with oppositeactions on excitatory and inhibitory postsynaptic receptors/channelsas evident by the decrease in mEPSC amplitude and the increasein mIPSC amplitude. The concept of opposite EtOH actions on excitatoryand inhibitory synaptic transmission is not new, but this is thefirst study to show that during the period of spinal network formationin the rat (Seebach and Ziskind-Conhaim 1994), EtOH at the lowerconcentration (70 mM) was more effective in modulating presynapticrelease of excitatory and inhibitory neurotransmitters than changingthe properties of their postsynaptic receptors/channels. The findingthat relatively high EtOH concentrations were required to affectminiature current properties might be related to the age-dependentsensitivity to EtOH in the rat (Fang et al. 1997). It is conceivablethat lower EtOH concentrations would effectively modulate synapticcurrents in more maturerats.

Dual EtOH actions on neurotransmitter release

Our observations that EtOH depressed mEPSC frequency supported previous reports showing that it inhibited NMDA-mediated glutamaterelease in the rat striatum (Carboni et al. 1993) and suppressedhigh-K⁺-evoked release of endogenous glutamate and aspartate in the hippocampalslice (Martin and Swartzwelder 1992). The finding that EtOH increasedmIPSC frequency was similar to the increased frequency of glycinergicmIPSCs in postnatal hypoglossal motoneurons (Eggers et al. 2000)but contradicted its inhibitory effect on high-K⁺-evoked GABA release in the hippocampus (Martin and Swartzwelder1992). It should be noted that the decrease in endogenous GABArelease was measured in the whole tissue rather than its releaseat synaptic sites as reflected in ourstudy.

The mechanisms underlying EtOH-induced opposite actions on vesicular release of excitatory and inhibitory neurotransmittersare unknown. It is conceivable that different presynaptic receptorsthat influence intracellular calcium concentrations are expressedon terminals releasing glutamate, glycine and GABA. Dual EtOHactions on muscarine-stimulated release of norepinephrine (NE)have been demonstrated in PC12 cells (Rabe and Weight 1988). Ata concentration of 25 mM, EtOH inhibited both muscarine-inducedNE release and the increase in intracellular free Ca²⁺. However, at a concentration of 100 mM, it increased NE releaseand elevated intracellular Ca²⁺. Those findings implied that the dose-dependent dual EtOH actionswere associated with its opposite effects on intracellular Ca²⁺. Therefore it is possible that suppression of Ca²⁺ release from internal stores in glutamate containing nerve terminalscontributed to the reduced mEPSC frequency. It has been shownthat spontaneous transmitter release can result from spontaneousCa²⁺ release from internal stores in hippocampal synaptic boutons(Emptage et al. 2001), and in Purkinje cells, large mIPSCs aregenerated by multivesicular release mediated by Ca²⁺ release from presynaptic stores (Llano et al. 2000).

In our study, miniature postsynaptic currents were recorded in the presence of 18 mM extracellular K⁺ that produced ~20 mV depolarization, sufficient to reach thethreshold potential for Ca²⁺ current activation (Gao and Ziskind-Conhaim 1998). One of themost significant effects of EtOH on voltage-gated ion channelsis its inhibitory action on Ca²⁺ channels, in particular the L-type channel (reviewed by Crewset al. 1996). It is feasible that the decrease in mEPSC frequencyduring EtOH exposure resulted from its suppression of voltage-gatedCa²⁺ current. Our recent findings have indicated that EtOH reducedthe amplitude of Ca²⁺ current in spinal motoneurons of postnatal rats (Gao and Ziskind-Conhaim,unpublished data). That current was previously characterized asthe N-type current (Gao and Ziskind-Conhaim 1998), which appearedto regulate synaptic transmission in spinal cords of developingrodents (e.g., Gruner and Silva 1994; Xie and Ziskind-Conhaim1995).

It is conceivable that nerve terminals releasing glutamate have different components in the vesicular release sequence thanthose releasing glycine and GABA (Varoqueaux et al. 2002), resultingin different EtOH actions on the release of excitatory and inhibitoryneurotransmitters. The mechanisms underlying the increase in mIPSCfrequency are unknown, but it is possible that presynaptic facilitationvia ligand- or voltage-gated channels is responsible for the increasedmIPSCfrequency.

Opposite EtOH actions on postsynaptic receptors

EtOH opposite actions on mEPSC and mIPSC amplitudes supported the general consensus that its interaction with glutamate receptors/channelsdepressed glutamatergic responses, while it increased glycine-and GABA-mediated Cl currents (reviewed by Faingold et al. 1998; Weight et al. 1992).It is thought that NMDAR-mediated synaptic transmission is especiallysensitive to acute EtOH exposure (Dildy-Mayfield et al. 1996;Lovinger et al. 1989; Morrisett and Swartzwelder 1993). However,our findings indicated that there was no differential sensitivityto EtOH of NMDA and non-NMDA receptors (see also Wang et al. 1999;Wrikner et al. 2000). NMDA receptor sensitivity to EtOH depends,at least in part, on the receptor subunit compositions (Lovinger1995; Masood et al. 1994; Yang et al. 1996; reviewed by Crewset al. 1996), and studies have suggested that EtOH has a moreprominent action on NMDAR-mediated currents in cells expressingthe NR1/NR2B combination than any other receptor subunit composition(Masood et al. 1994; Woodward 2000). Although we cannot rule itout, it is unlikely that the low sensitivity of the NMDA receptorto EtOH is related to its receptor subunit composition in developingspinal motoneurons, because NR1 and NR2B subunits are expressedin postnatal motoneurons (Stegenga and Kalb 2001). Moreover, EtOH(100 mM) has similar inhibitory action on both AMPAR- and NMDAR-mediatedsynaptic currents in motoneurons of 14- to 23-day-old rats (Wanget al. 1999), close to the time when adult-like NMDA receptorsubunit composition is expressed (Stegenga and Kalb 2001). Itis conceivable that other postsynaptic mechanisms, such as EtOHactions on pathways that regulate receptor phosphorylation (reviewedby Woodward 2000), mediate at least some of its effects on glutamate-mediatedsynaptictransmission.

Our observation that EtOH increased the amplitudes of GlyR- and GABA_AR-mediated mIPSCs supported previous reports showingan increase in GABA- and glycine-induced Cl flux during EtOH exposure (Aguayo 1990; Aguayo and Pancetti 1994;Celentano et al. 1988; Eggers et al. 2000; Nestores 1980; Reynoldsand Prasad 1991). EtOH had no differential actions on GlyR- andGABA_AR-mediated mIPSCs in postnatal motoneurons as reported indissociated spinal neurons in which EtOH induced larger increasein glycine- than GABA-induced current (Celentano et al. 1988).It is possible that EtOH significantly increased mIPSC amplitudeonly at a concentration of 200 mM because of the immature compositionof glycine and GABA receptor subunits. Expression of $alpha$ 1, $beta$ 2, and $gamma$ 2 GABA_A receptor subunits (Criswell et al. 1993; Duncan et al.1995; Wafford et al. 1991) and $alpha$ 1 glycine receptor domain (Eggerset al. 2000; Mascia et al. 1996) are correlated with high sensitivityto EtOH. In spinal sensory neurons, the switch in glycine receptorsubunits from the embryonic $alpha$ 2 to the adult $alpha$ 1 occurs betweenP8 to P16 (Takahashi et al. 1992), implying that motoneurons expressedprimarily the $alpha$ 2 subunit during the period examined in ourstudy.

Our data demonstrated that EtOH dual modulatory actions on excitatory and inhibitory synaptic currents resulted from its interactionswith both pre- and postsynaptic mechanisms that regulate synaptictransmission in the developing rat spinal cord. EtOH oppositeeffects on presynaptic release of excitatory and inhibitory neurotransmitterswere predominant in newly established spinalnetworks.

	ACKNOWLEDGMENTS

We thank Drs. Peter Lipton and Steve Redman for constructive comments on themanuscript.

This work was supported by National Institute of Neurological Disorders and Stroke Grant NS-23808 to L. Ziskind-Conhaim.

	FOOTNOTES

Address for reprint requests: L. Ziskind-Conhaim Dept. of Physiology, 129 SMI 1300 University Ave., University of Wisconsin,Medical School, Madison, WI 53706 (E-mail: lconhaim{at}physiology.wisc.edu).

REFERENCES

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

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