Ethanol-GABAA Receptor Interactions: A Comparison between Cell Lines and Cerebellar Purkinje Cells

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Vol. 284, Issue 2, 768-776, February 1998

Ethanol-GABA_A Receptor Interactions: A Comparison between Cell Lines and Cerebellar Purkinje Cells¹

Douglas W. Sapp and Hermes H. Yeh

Departments of Pharmacology (D.W.S., H.H.Y.), Neurology (H.H.Y.) and Program in Neuroscience (H.H.Y.), University of Connecticut Health Center, Farmington, Connecticut

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

This study compared the interaction between ethanol and $gamma$ -aminobutyric acid (GABA)-mediated current responses elicited inseveral immortalized cell lines and stably transfected cells,as well as in cultured and acutely dissociated rat cerebellarPurkinje cells. Only cell lines that were found previously topossess functional GABA_A receptors were examined in this study.Under identical recording conditions, ethanol (10-200 mM) exertedno effect on GABA-induced currents in any of the cell lines orstably transfected cells tested in this study. However, GABA responsesmonitored in both primary culture and acutely dissociated Purkinjecells were significantly potentiated by ethanol (25 and 50 mM).Mouse pancreatic cells (RINm5F) were insensitive to both diazepamand ethanol suggesting the expression of a GABA_A receptor isoformlacking a $gamma$ subunit. Immortalized neuroblastoma IMR-32 cells displayedGABA responses that could be distinguished based on differentialsensitivity to diazepam. However, none of the IMR-32 cells displayedGABA responses that were sensitive to modulation by ethanol. GABAresponses in the stably transfected cell lines, PA3 ( $alpha$ 1 $beta$ 1 $gamma$ 2_L)and WSS-1 ( $alpha$ 1 $beta$ 2 $gamma$ 2), were also unaffected by exposure to ethanol.In Purkinje cells acutely dissociated from the neonatal cerebellum,the ethanol-induced potentiation of GABA-induced current responsecould be observed before postnatal day 7, when only the $gamma$ 2_S butnot the $gamma$ 2_L splice variant is expressed. This indicates that the $gamma$ 2_L subunit is not necessary for an ethanol-induced potentiationof GABA_A receptor-mediated response to become manifest. In addition,the results point to inherent differences that should be takeninto account in interpreting comparative data between native andrecombinant GABA_A receptors.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Considerable experimental attention in research on the central effects of ethanol has been directed toward examining its modulatoryeffects on the GABA_A receptor complex. Early biochemical studiesdemonstrated an ethanol-induced potentiation of GABA-mediated³⁶Cl flux in synaptoneurosomes and microsacs derived from rat andmouse cerebral cortex (Allan and Harris, 1986; Mehta and Ticku,1988; Suzdak et al., 1986). This was largely corroborated by electrophysiologicalstudies indicating that physiologically-relevant concentrationsof ethanol potentiated GABA-mediated currents in cultured cerebralcortical and spinal cord neurons (Aguayo, 1990; Celentano et al.,1988; Nishio and Narahashi, 1990; Reynolds and Prasad, 1991).Other electrophysiological studies, however, failed to observemodulatory effects of ethanol on neuronal responses to GABA (Sigelet al., 1993; Siggins et al., 1987; White et al., 1990). One prevailingpostulate to reconcile the diverse and apparently conflictingresults related to sensitivity to modulation by ethanol takesinto account the diversity of the known GABA_A receptor subunits,of which 17 have been uncovered and classified into five families[reviewed in (Macdonald and Olsen, 1994; McKernan and Whiting,1996; Sieghart 1995; Tyndale et al., 1995; Yeh and Grigorenko,1995)]. The subunits display discrete yet overlapping patternsof distribution in the brain, and recombinant GABA_A receptorsof defined subunit combinations exhibit different yet predictablefunctional properties. These considerations, taken together, couldaccount in theory for the observed modulation of GABA_A receptorsby ethanol among different types of neurons and brain regions.

Several studies have attempted to define the subunit composition of GABA_A receptors sensitive to modulation by ethanol throughthe use of recombinant receptors assembled in a variety of expressionsystems. Thus, differences in sensitivity to ethanol have beenfound to depend on the $alpha$ subunit isomer, because recombinant GABA_Areceptors expressing either the $alpha$ 1 or $alpha$ 6 subunit differed in ratesof desensitization in response to co-application of GABA and ethanol(Marszalec et al., 1994). Zolpidem, aside from its demonstratedhigh-affinity binding to Benzodiazepine type I receptors, alsoappears to be selective for receptors which are sensitive to potentiationby ethanol (Criswell et al., 1993).

The $gamma$ 2 subunit exists as either a long or a short alternatively spliced variant ( $gamma$ 2_L or $gamma$ 2_S) (Whiting et al., 1990). The $gamma$ 2_Lsplice variant contains in the intracellular loop between transmembranedomains TM3 and TM4 an additional 8-amino acid mini-exon thatalso harbors a consensus sequence for phosphorylation by PKC.In a series of studies using $alpha$ 1/ $beta$ 2/ $gamma$ 2-containing recombinant GABA_Areceptors expressed in Xenopus oocytes, a dependence on subunitspecificity was demonstrated in that the ethanol-induced potentiationwas observed only when the GABA_A receptor assembly included the $gamma$ 2_L subunit (Wafford et al., 1991; Wafford and Whiting, 1992).However, a lack of effect by ethanol on either $gamma$ 2_L- or $gamma$ 2_S-containingrecombinant GABA_A has also been reported (Sigel et al., 1993),and the degree to which sensitivity to modulation by ethanol dependson the $gamma$ 2_L subunit remains an outstanding issue.

In this study we compared the effect of ethanol on whole-cell GABA-activated current responses under identical patch clampelectrophysiological recording conditions in two immortalizedcell lines expressing endogenous functional GABA_A receptors, twocell lines stably transfected with $alpha$ 1/ $beta$ x/ $gamma$ 2 GABA_A receptor subunitsand in cerebellar Purkinje cells either maintained in long-termprimary culture or after acute dissociation from the neonatalrat cerebellum. We chose to examine cerebellar Purkinje cellsbecause they express GABA_A receptor subunit profiles similar tothose of the stably transfected cell lines examined (Laurie etal., 1992). We report that ethanol potentiated GABA-mediated currentin Purkinje cells but had no effect on GABA responses recordedin any of the cell lines tested. Furthermore, an ethanol-inducedpotentiation of GABA responses in Purkinje cells could be observedat a time in development before the expression of the $gamma$ 2_L GABA_Areceptor subunit mRNA.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Maintenance of cell lines in culture. The RINm5F, IMR-32, WSS-1 and PA3/X25 cell lines were each maintained under conditions according to published reports (Hadinghamet al., 1992; Noble et al., 1993; Tyndale et al., 1994; Wong etal., 1992). The RINm5F cell line was maintained in RPMI medium,the IMR-32 cell line in $alpha$ -minimum essential medium, and the WSS-1cell line in DMEM. These media were supplemented with 10% fetalbovine serum and fungizone/penicillin/streptomycin. The PA3 andX25 cell lines were cultured on 0.01% poly-D-lysine coated platesand maintained in DMEM supplemented with 5% fetal calf serum.After 2 days in culture, 1 µM dexamethasone was added to the PA3and X25 cell cultures to induce GABA_A receptor expression andelectrophysiological recordings were conducted 3 to 5 days thereafter.

Preparation of primary and acutely dissociated cerebellar cells. Primary cultures of cerebellar neurons were derived from cerebella of PD 0 Sprague-Dawley rats. Cerebella were removed, mincedand then incubated in Ca⁺⁺-Mg⁺⁺-free phosphate-buffered saline containing 0.1% DNase and 0.25%trypsin for 15 min at 37°C. The tissue was then gently trituratedin medium containing DMEM, 10% heat-inactivated fetal bovine serum,2 mM glutamine and fungizone/penicillin/streptomycin. Dissociatedcells in suspension were added at a density of 3 × 10⁴ cells/cm² to glass coverslips coated with 0.01% poly-D-lysine and placedin an incubator for 1 hr to allow the cells to adhere. Beforethe seeding of cells, silicone droplets were attached to the peripheryof each cover slip. Once the cells have adhered, the coverslipswere placed inverted in 35-mm culture dishes containing a bedof cerebellar glial cells. Then 48 hr after plating, the serum-containingmedium was replaced with a DMEM-based serum-free growth mediumsupplemented with B-27 nutrient mixture. The cultures were maintainedin humidified 95% oxygen/5% carbon dioxide at 37°C and replenishedwith serum-free growth medium every 2 days. On selected days afterplating, cerebellar cultures were fixed and processed immunohistochemicallyaccording to previously established procedures (Cheun and Yeh,1992) to reveal calbindin-like immunoreactive cells. In vivo,only Purkinje cells express calbindin-like immunoreactivity inthe cerebellum (Sequier et al., 1990). Calbindin-like immunoreactivityhas also been used to identify Purkinje cells in culture (Brorsonet al., 1991). Thus, calbindin-like immunoreactivity and cellmorphology was used to identify Purkinje cells in culture forelectrophysiological recording (see fig. 5A).

Acutely dissociated Purkinje cells were obtained from cerebella of PD-0 to -10 Sprague-Dawley rat pups as previously described(Cheun and Yeh, 1992

). Briefly, rat pups were decapitated, thecerebellum was quickly removed, freed of the overlying dura, mincedinto approximately 1 mm³ pieces and incubated at 34°C in Earle's balanced salt solutioncontaining papain (15 U/ml; Worthington, Freehold, NJ) for 60min. The tissue was then treated with horse serum or ovomucoidto inactivate protease activity and washed several times withthe bath solution used for electrophysiological recording. Gentleone-pass trituration of the tissue yielded a suspension of singlecells that was then transferred to a 35-mm plastic Petri dish.The cells were allowed to adhere to the bottom of the dish, andacutely dissociated Purkinje cells were identified based on theirmorphology (Cheun and Yeh, 1992

). All recordings were performedwithin 3 hr after acute dissociation.

Electrophysiology. Unless stated otherwise, whole-cell patch clamp recording of GABA-activated current responses were performed at room temperaturein a bath solution containing (in mM): 140 NaCl, 5.4 KCl, 1.8CaCl₂, 1 MgCl₂, 5 HEPES, (pH 7.4). Some experiments involvingPA3 and X25 cells employed bath solution consisting of (in mM):130 NaCl, 5 KCl, 2 CaCl₂, 1 MgCl₂, 5 HEPES, 11 D-glucose, 13 sucrose(pH 7.2) in accordance with a previously published protocol (Harriset al., 1995a). Recording pipets were fire-polished to an inputresistance of 5 to 10 M $Omega$ . Seal formation and recordings were conductedusing conventional whole-cell patch clamp recording procedures(Hamill et al., 1981) using an EPC-7 amplifier (Darmstadt, Germany).The recording solution contained (in mM): 140 KCl, 1.8 CaCl₂,1 MgCl₂, 5 HEPES, 3 Mg⁺⁺-ATP, 0.1 leupeptin (pH 7.4). Leupeptin was included to inhibitproteolysis and Mg⁺⁺-ATP was included to prevent possible rundown of the GABA-activatedresponse (Chen et al., 1990). Membrane currents were amplifiedand filtered through a 4-pole Bessel filter. The analog signalswere also monitored throughout the experiments using a Gould Brush260 chart-recorder. GABA-activated currents were filtered, digitizedand analyzed off-line using a data acquisition and analysis program(DATAQ/DATANAL, JPM Programming). Data were analyzed as previouslydescribed (Yeh and Kolb, 1997). Ethanol was determined to havea potentiating effect when there was a $>=$ 20% increase in the GABA-ethanolresponse amplitude over mean peak control response.

Preparation and delivery of drugs. GABA, bicuculline methiodide and ethanol were dissolved bath solution. Diazepam was first dissolved in DMSO and then seriallydiluted in bath solution so that the final concentration of DMSOwas <0.01%. Drugs were loaded into separate barrels of a multi-barrelpipet assembly and delivered by brief pulses of regulated pressure( $<=$ 2 PSI). The drug pipet assembly was mounted onto a micromanipulatorso that it could be navigated under visual control to within 10µm of the cell under study. This method facilitated brief focalapplications of multiple test substances. One of the drug pipetswithin the multibarrel pipet assembly was routinely filled withbath solution that was applied continuously between epochs ofdrug application to clear drugs from the immediate vicinity ofthe cell and to control for possible mechanical artifacts dueto bulk flow.

RT-PCR-based profiling of GABA_A receptor subunit mRNAs. Candidate GABA_A receptor mRNA profiles were obtained from the different cell line cultures as well as from selected singlecells by means of an RT-PCR-based protocol (Yeh et al., 1996).For cultures, RNA was extracted with TRI reagent (Molecular ResearchCenter), solubilized in RNase-free water and cDNA was synthesizedby the addition of AMV reverse transcriptase (10 U) (Seikagaku,Ijamsville, MD), 1X first strand buffer, 2.5 mM dNTPs (Promega,Madison, WI), 10 ng oligo (dT) (Genosys, Woodlands, TX), RNasininhibitor (20 U) and 10 mM dithiothreitol, incubated for 1 hrat 42°C. For single cells, first-strand cDNA was synthesized asabove except that the oligonucleotide contained an oligo-dT regionand the T7 RNA polymerase promotor. This facilitated one roundof aRNA amplification using the T7 RNA polymerase before amplicationby PCR (Eberwine et al., 1992). PCR amplification of the reversedtranscribed cDNA template derived from either cultures or singlecells was then performed in a solution containing thermal buffer,2.5 mM MgCl₂, 0.25 mM dNTPs, 2 U of Taq DNA polymerase (Promega),50 pmol of primers, and 1 µl cDNA in a final volume of 20 µl.Samples were amplified for 30 or 40 cycles at 94°C for 45 sec,60°C for 45 sec, 72°C for 1 min and a final extension was appliedat 72°C for 7 min using a programmable thermocycler (Perkin-ElmerCetus, Cupertino, CA). The amplified products were separated ona 2% agarose gel and visualized under UV illumination after stainingwith ethidium bromide. Whole-brain rat cDNA was used as positivecontrol. Samples of reversed transcribed template to which noRNA was added served as negative control. Southern blot analysis,such as that illustrated in figure 6C, was performed as describedpreviously (Yeh et al., 1996) using cDNA probes specific for the $gamma$ 2_S and $gamma$ 2_L GABA_A receptor subunits.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

IMR-32

IMR-32 (human neuroblastoma) cells possess functional GABA_A receptors, as revealed by TBPS binding autoradiography and GABA-stimulatedchloride flux assays (Anderson et al., 1993). Western blot analysisdemonstrated the presence of at least the $alpha$ 3 subunit (Noble etal., 1993), but the full complement of GABA_A receptor subunitshas yet to be characterized. In our study, we profiled the expressionof GABA_A receptor subunit mRNAs in cultured IMR-32 cells. An exampleof such an expression profile is illustrated in figure 1A. Inaddition to mRNA encoding the $alpha$ 3 subunit, $alpha$ 1, $alpha$ 4, $beta$ 1, $beta$ 3, $gamma$ 2 and $delta$ subunit mRNAs were also detected. Thus, numerous GABA_A receptorsubunit transcripts were found to be expressed by IMR-32 cells.However, pharmacological characterization of GABA-activated currentresponse properties of individual IMR-32 cells suggests that notall IMR-32 cells express the full profile of subunits (D.W. Sappand H.H. Yeh, manuscript in preparation). For example, individualIMR-32 cells could be shown to display GABA responses that wereeither sensitive or insensitive to potentiation by diazepam (fig.2, A and B).

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Fig. 1. IMR-32 cells express functional GABA_A receptors. A, Ethidium bromide-stained agarose gel showing PCR-amplified products generatedin the presence of GABA_A receptor subunit-specific primers andcorresponding to the $alpha$ 1, $alpha$ 3, $alpha$ 4, $beta$ 1, $beta$ 3, $gamma$ 2 and $delta$ subunits. ThecDNA template used for PCR was reverse transcribed from mRNA isolatedfrom IMR-32 cells that had been grown to confluence in two 60-mmPetri dishes. $beta$ -actin ( $beta$ A) was routinely included as a positivecontrol. B, The penwriter record (upper panel) shows that theGABA-activated current response is markedly reduced in the presenceof bicuculline (100 µM). Digitized and averaged traces correspondingto GABA responses before (control), during and after (recovery)exposure to bicuculline are superimposed to facilitate quantitativeanalysis; bicuculline reduced the GABA response by 91%. C, PeakGABA response current-voltage relationship obtained from an IMR-32cell. The inset illustrates a set of superimposed current tracesobtained at various holding potentials, as indicated, and thiswas used to determine the peak amplitude of the GABA responseat a given holding potential.

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Fig. 2. Effect of ethanol on GABA-activated current response in IMR-32 cells. A, Continuous penwriter record (A1) and averaged digitizedtraces corresponding to periods before (control), during and after(recovery) application of ethanol (100 mM; A2) or diazepam (0.5µM; A3). This cell was insensitive to ethanol but was sensitiveto positive modulation by diazepam. B, Continuous penwriter record(B1) and averaged digitized traces from another IMR-32 cell thatwas insensitive to modulation by either ethanol (100 mM; B2) ordiazepam (0.5 µM; B3). C, Summary of data from all IMR-32 cells(n = 31) in which interaction between GABA and ethanol (10-200mM; open bars) as well as diazepam (shaded bars) were tested inthe same cell. For this and all subsequent figures, the numbersincluded in the bar graphs reflect the number of cells testedin the corresponding experiments.

GABA (100 µM) delivered by regulated pressure induced whole-cell inward currents in IMR-32 cells held near their resting membranepotential. The GABA-activated current was blocked by 100 µM bicucullinemethiodide (fig. 1B) and reversed at approximately 0 mV with equimolar[Cl]_in and [Cl]_out (fig. 1C). GABA was applied for variable lengths of timein order to derive an operationally defined range of responseamplitudes that would be suitable for testing the effect of ethanol(fig. 1D, inset). With a 5-sec application of 100 µM GABA, themaximal response (I_max) typically ranged between 200 to 300 pA(274 ± 31 pA, mean ± S.E.M.; n = 42). Figure 1D also illustratesdata obtained from an IMR-32 cell in which amplitudes of the peakcurrent response to GABA were plotted as a function of durationof agonist application. A "duration-response" relationship couldbe readily established. For each cell tested, the duration ofagonist application was thus adjusted so as to produce currentresponses of constant amplitude approximately 20% of the I_maxin response to 100 µM GABA, and this was subsequently used toassess the modulatory effect of ethanol and diazepam on the samecell. As determined by data obtained from the 31 IMR-32 cellsincluded in this study, the duration of GABA application rangedbetween 40 and 200 msec.

Ethanol at any concentration examined in this study (10-200 mM) had no effect on the GABA-mediated current responses in IMRcells (fig. 2C). In figure 2A1 (top panel), the continuous penwriterrecord shows GABA-activated current responses monitored on-linebefore, during and after exposure to ethanol (100 mM) and diazepam(0.5 µM). The averaged digitized traces (fig. 2, A1 and A2) indicatethat, although exposure to ethanol did not affect the amplitudeof the GABA-activated current response, exposure to diazepam resultedin a reversible 81% potentiation of the GABA response in the samecell. Overall, in IMR-32 cells (n = 10) that could be shown tobe sensitive to diazepam, the benzodiazepine-induced potentiationaveraged 59 ± 16%, although ethanol exerted no effect in any ofthese cells. IMR-32 cells displaying GABA responses that wereinsensitive to modulation by diazepam were also encountered inthis study (fig. 2B). Ethanol also did not affect the GABA responsesin such cells (n = 21). The data obtained from diazepam-sensitiveand -insensitive cells were pooled and are graphically summarizedin figure 2C.

RINm5F

RINm5F cells display GABA-activated current responses that are blocked by bicuculline and zinc but are insensitive to modulationby the benzodiazepines, suggesting the predominant expressionof a GABA_A receptor that lacks a $gamma$ subunit (Hales and Tyndale,1994). Pressure application of 100 µM GABA ( $>=$ 1 sec in duration)produced an I_max of 64 ± 9 pA (mean ± S.E.M.; n = 8), similarto those reported previously (Hales and Tyndale, 1994). To assessthe effect of ethanol, the duration of GABA application was adjustedfor each cell so as to produce an approximately half-maximal levelof the GABA-activated current response. The protocol for testingthe effect of ethanol or diazepam on RINm5F responses to GABAwas identical to that described above for testing IMR-32 cells.Neither a low (10 mM) nor a higher (100 mM) concentration of ethanolmodulated the GABA-activated currents (fig. 3). The GABA-activatedcurrent responses monitored in RINm5F cells were also insensitiveto potentiation by diazepam (fig. 3).

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Fig. 3. Effect of ethanol and diazepam on GABA responses elicited in RINm5F cells. This bar graph summarizes data obtained from RINm5Fcells that were tested for both diazepam-GABA and ethanol (10or 100 mM)-GABA interactions. Error bars reflect the S.E.M.

PA-3, X-25 and WSS-1. The PA-3 and X-25 cells are derived from a mouse fibroblast cell line that had been stably transfected with the $alpha$ 1/ $beta$ 1/ $gamma$ 2_Land $alpha$ 1/ $beta$ 1 combinations of GABA_A receptor subunits, respectively(Hadingham et al., 1992). In both ³⁶Cl flux assays and electrophysiological studies (Harris et al.,1995a), GABA-mediated responses of PA3 cells, but not those ofX-25 cells, were potentiated by 10 mM ethanol. In PA-3 cells maintainedon a poly-L-lysine substrate, the ethanol effect was observedat low GABA concentrations (3 and 10 µM). In our study, the interactionbetween ethanol and GABA-activated current responses was examinedin PA-3 cells and X-25 cells under similar conditions using GABAat a concentration of 10 µM (fig. 4A). As was observed in everyPA-3 cell tested (n = 28), a robust and readily reversible potentiationof the GABA response could be elicited upon exposure to diazepambut not to ethanol. In contrast, X-25 cells (12 of 12) were neithersensitive to modulation by diazepam nor ethanol. Ethanol testedat a range from low to high concentrations (10, 30 and 100 mM)yielded the same results (fig. 4A).

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Fig. 4. Effect of ethanol and diazepam on GABA-activated current responses in cell lines expressing recombinant $alpha$ 1 $beta$ 2 $gamma$ 2_S (WSS1 cells), $alpha$ 1 $beta$ 1 $gamma$ 2_L (PA3 cells) and $alpha$ 1 $beta$ 1 (X25 cells) GABA_A receptors. A, Dataobtained from each cell tested were normalized such that the averagedamplitudes of GABA (10 µM) responses recorded during exposureto ethanol (10, 30, 100 mM) or diazepam (0.5 µM) were expressedas a percentage change from those obtained during control (pre-ethanolor -diazepam exposure) periods. Inset, Examples of averaged, superimposedcurrent traces taken from a PA3 cell (left panel) and an X25 cell(right panel) showing positive modulation by and no effect ofdiazepam, respectively. B, RT-PCR profiling of $gamma$ 2_L and $gamma$ 2_S mRNAexpression in single IMR-32, PA3, X25 and WSS-1 cells. Each cellillustrated had been recorded electrophysiologically, and thedata were incorporated into the summary graphs shown in figure2C (IMR-32 cell) and figure 4A (WSS-1, PA3, X25 cells).

Ethanol also did not modulate GABA responses monitored in the WSS-1 cell line that stably expresses functional $alpha$ 1/ $beta$ 2/ $gamma$ 2 recombinantGABA_A receptors (Wong et al., 1992

). An interaction between ethanoland GABA (10 µM) was tested in a total of 32 WSS-1 cells in thepresence of ethanol at 10 mM (n = 9), 30 mM (n = 11) and 100 mM(n = 12). In 14 of the 32 cases, the effects of ethanol and diazepamon GABA-activated current responses were examined in the samecell. In each case, diazepam, but not ethanol, potentiated GABAresponses (192 ± 18% potentiation, n = 14; fig 4A). This is consistentwith results obtained using the PA-3 cell line. Whether the longor short variant of $gamma$ 2 subunit was used for transfecting WSS-1cells was not specified in the original study (Wong et al., 1992

The results of our RT/PCR-based mRNA profiling (fig. 4B) suggest the expression of the $gamma$ 2_S transcript in WSS-1 cells, thatof the $gamma$ 2_L in PA-3 cells, both $gamma$ 2_S and $gamma$ 2_L mRNAs in IMR-32 cells,and an absence of any $gamma$ 2 splice variant messages altogether inX-25 cells.

Cerebellar Purkinje cells

Cultured Purkinje cells. The outcome of an interaction between ethanol and GABA (25 µM) was examined in cultured Purkinje cells, identified based onsize and morphology of calbindin-immunopositive profiles in long-termprimary cultures derived from postnatal day 0 rat cerebellum (fig.5A). The electrophysiological recordings were performed between2 and 10 days in culture. In sharp contrast to the consistentlack of an effect in cell lines, ethanol (25 mM) potentiated theamplitude of the GABA-activated current responses elicited incultured Purkinje cells. An ethanol-induced potentiation (34 ±7%, mean ± S.E.M.; range = 20-42%) was seen in 10 of 14 cases(71%). In figure 5B, data derived from the 14 cells tested aresummarized in the form of a scattergram and an example taken froman individual Purkinje cell is given in the inset.

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Fig. 5. Ethanol-induced potentiation of GABA-activated current response in cultured cerebellar Purkinje cells. A, Calbindin-like immunoreactivityin cerebellar neurons in vivo (A1) and maintained 4 days in aculture derived from PD 0 rat (A2). Calbindin-like immunoreactiveprofiles (solid arrow), presumably Purkinje cells, display a largesoma and dendritic branching that is more elaborate than the smallercells (open arrow) displaying background level of staining. Bars= 50 µm. B, "Scattergram" summarizing data derived from 14 culturedPurkinje cells tested for ethanol-GABA interaction. Each datapoint represents the mean peak amplitude of the GABA (25 µM) responseduring exposure to 25 mM ethanol plotted as a function of thatmonitored during the control (pre-ethanol exposure) period. Theshaded area on either side of the 45° "equivalence" line (Yehand Kolb, 1997

) predicts no significant change due to ethanolexposure using 20% as an operationally defined level of significancefor ethanol potentiation of GABA-mediated currents. Of the 14cells, data points derived from 10 cells lie above this area,indicating potentiation of the GABA response in the presence ofethanol.

Acutely dissociated Purkinje cells. The ethanol-induced potentiation of GABA responses observed under long-term culture conditions was also found in Purkinjeneurons acutely dissociated from neonatal cerebella (fig. 6A).Data from a total of 18 Purkinje cells, acutely dissociated fromPD-3 (n = 4), PD-5 (n = 6), PD-7 (n = 6) and PD-10 (n = 2) ratcerebella, were included for analysis in this study (fig. 6B).The degree of potentiation induced by ethanol was highly variableand, given the limited sampling size for each postnatal age, itwas not possible to attribute this variability to the age of thecerebellum from which the acutely dissociated Purkinje cells werederived. Acute exposure to ethanol resulted in a $>=$ 20% increasein the GABA (10 µM) response amplitude in 83% (15/18) of the cellstested, reflecting a 39.0 ± 5.2% (mean ± S.E.M.) augmentationof the control GABA response.

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Fig. 6. Ethanol potentiates GABA-activated current responses in acutely dissociated rat cerebellar Purkinje cells. A, Continuous penwriterrecord (top) and digitized current traces (bottom) illustratecurrent transients in response to GABA (10 µM) monitored correspondingto periods before (control), during and after (recovery) exposureto 50 mM ethanol. The 200-msec pressure pulses of GABA were appliedevery 30 sec. The bar above the penwriter record indicates an18-sec period of continuous application of ethanol. During thecontrol and recovery periods, bath solution was applied from aseparate drug pipet in lieu of ethanol. B, Agarose gel and correspondingSouthern blot of PCR-amplified products derived from individualelectrophysiologically-studied Purkinje cells indicate that the $gamma$ 2_L subunit mRNA is not detected on PD-5 but is present by PD-7although the $gamma$ 2_S subunit transcript can be detected on both PD-5and PD-7.

An issue addressed was whether the expression of the $gamma$ 2_L subunit and its inclusion in the assembly of the GABA_A receptor complexwas required for conferring the ethanol-induced potentiation ofthe GABA response. Adult cerebellar Purkinje cells uniformly expressboth long and short variants of the $gamma$ 2 GABA_A receptor subunitmRNAs, in addition to those encoding the $alpha$ 1, $beta$ 2, and $beta$ 3 subunits(Gutierrez et al., 1994

; Laurie et al., 1992

). The presence ofthe $gamma$ 2 subunit mRNAs was confirmed in our study, insofar as combinedpatch clamp/RT-PCR in individual neurons revealed that Purkinjecells acutely dissociated from PD-7 or older cerebella with demonstratedsensitivity to GABA modulation by ethanol also expressed boththe $gamma$ 2_L and $gamma$ 2_S subunit transcripts (fig. 6C). However, a strikingand unexpected finding was that, although an ethanol-induced enhancementof GABA response could be observed in Purkinje cells before PD-7,the individual electrophysiologically-recorded cells expressedthe $gamma$ 2_S but not the $gamma$ 2_L mRNA (fig. 6C).

Figure 6C focuses on the expression of the $gamma$ 2_S and/or $gamma$ 2_L messages in 3 PD-5 and 1 PD-7 acutely dissociated Purkinje cells,all of which had been verified electrophysiologically to displayGABA responses that were sensitive to modulation by ethanol. Theagarose gel (top panel) and Southern blot of the same gel probedwith $gamma$ 2_S- and $gamma$ 2_L-specific oligonucleotides (lower panel) indicatethat, while the $gamma$ 2_S transcript could be readily detected in everyPurkinje cell, that of the $gamma$ 2_L was evident on PD-7 but not onPD-5. Thus, sensitivity to modulation by ethanol could be demonstratedin Purkinje cells that do not express the $gamma$ 2_L mRNA.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

This study addresses two fundamental issues related to the relationship between GABA_A receptor subunit combination and sensitivityto modulation by ethanol. The first issue relates to the discrepantresults in the literature on ethanol-recombinant GABA_A receptorinteractions that have often been attributed to differences inexperimental techniques and methods of analysis. To this end,ethanol-GABA_A receptor interaction was examined under identicalrecording conditions in several cell lines and in cerebellar Purkinjecells. The second issue relates to whether there is a specificrequirement of the $gamma$ 2_L subunit in conferring ethanol sensitivityto native GABA_A receptors, as has been reported for recombinantGABA_A receptors, and this was examined in primary rat cerebellarcell cultures and in acutely-dissociated Purkinje cells.

Subunit combination alone does not determine sensitivity to GABA_A receptor modulation by ethanol. Taking the view that subunit composition is a critical determinant in the neuroactive nature of ethanol on the native GABA_Areceptor, sensitivity to modulation by ethanol can be expectedto vary, depending on the GABA_A receptor isoform. Given the diversityof GABA_A receptor subunits that can assemble to form functionallydistinct receptor complexes, an intuitively logical approach towardresolving the issue of whether sensitivity to ethanol may dependon subunit composition has been to examine recombinant GABA_A receptorsof defined heterologous subunit combinations in expression systems.However, although several studies have reported subunit-specificdependence of the ethanol effect (Wafford et al., 1991), othershave not (Marszalec et al., 1994; Korpi et al., 1995), and thesediscrepant outcomes have been commonly attributed to differencesin the electrophysiological methods employed by individual laboratories.In this study, identical patch clamp recording conditions wereemployed to compare the effect of ethanol on GABA-mediated currentresponses in immortalized cells, stably transfected cells andrat cerebellar Purkinje cells either maintained in primary cultureor isolated after acute dissociation. The PA-3 and WSS-1 celllines express $alpha$ 1/ $beta$ 1/ $gamma$ 2 and $alpha$ 1/ $beta$ 2/ $gamma$ 2 recombinant GABA_A receptors,respectively, similar to that expected to be expressed in cerebellarPurkinje cells because they express a limited set of $alpha$ 1/ $beta$ 2/ $beta$ 3/ $gamma$ 2transcripts (Hadingham et al., 1992). Our results clearly indicatethat ethanol had no effect on GABA-mediated currents elicitedin either the PA-3 or WSS-1 cell line, but potentiated GABA responseselicited in Purkinje cells. A systematic analysis of sensitivityto ethanol under varying concentrations of GABA was not performedin this study. Nonetheless, aside from this consideration, ourresults rule out differences in other electrophysiological recordingconditions as confounding factors. Thus, we are led to concludethat subunit combination alone cannot account for sensitivityto modulation by ethanol.

The cell lines used in this study included immortalized cells that endogenously express functional GABA_A receptors (RINm5F,IMR-32) as well as stably transfected cell lines that expressrecombinant GABA_A receptors of defined subunit combinations (PA3,X25 and WSS-1). Ethanol exerted no modulatory effect on GABA-activatedcurrent responses monitored in RINm5F, IMR-32, PA3, X25 and WSS-1cells. However, Diazepam markedly potentiated GABA responses elicitedin the same PA3, WSS-1 and some of the IMR-32 cells that lackedsensitivity to ethanol, but did not modulate responses of eitherRINm5F or X25 cells to GABA. These results are consistent with $gamma$ subunit-containing GABA_A receptors being sensitive to potentiationby diazepam (Knoflach et al., 1991

; Pritchett et al., 1989

; Ymeret al., 1990

), but not necessarily by ethanol.

Two of the cell lines, IMR-32 and PA-3, were found to express mRNA transcripts encoding the $alpha$ 1 and $gamma$ 2_L subunits. It was thusreasoned that the PA-3 and IMR-32 cell lines would be useful foraddressing issues related to ethanol- and diazepam-GABA interactions.In agreement with a previous report employing [³⁵S]TBPS binding and Cl uptake assays (Anderson et al., 1993

), we found that the majorityof IMR-32 cells displayed GABA responses that were insensitiveto diazepam. However, a minor subpopulation of IMR-32 cells weresensitive to modulation by diazepam, suggesting that IMR-32 cellscan express functional GABA_A receptor isoforms that either containor lack the $gamma$ 2_L subunit. Whether the individual IMR-32 cells examinedelectrophysiologically expressed exclusively either one of thetwo GABA_A receptor isoforms, or both isoforms but to varying levels,could not be addressed in our study.

Previous Western blot characterization of the IMR-32 cell line revealed the presence of only the $alpha$ ₃ subunit protein; otherGABA_A receptor subunit proteins, including those for the $alpha$ 1 and $gamma$ 2 subunits, were either not detected or not examined (Noble etal., 1993

). It may be that the $alpha$ 1 and $gamma$ 2_L subunit proteins areexpressed in a relatively small subpopulation of diazepam-sensitiveIMR-32 cells that could be revealed by electrophysiological recordingof individual cells but that their levels of expression are belowthe sensitivity of detection by Western blot analysis. In addition,the expression of the $alpha$ 3 subunit may predominate over that of $alpha$ 1, and IMR-32 cells may thus express primarily $alpha$ 3 $beta$ x $gamma$ 2_L/S GABA_Areceptors. In light of the potentiation of $alpha$ 1-containing GABA_Areceptors by zolpidem and its postulated link to ethanol (Criswellet al., 1993

), $alpha$ 3-containing GABA_A receptor isoforms may not beexpected to be sensitive to potentiation by ethanol yet wouldbe sensitive to diazepam. This could explain the lack of ethanolsensitivity in IMR-32 cells but falls short of explaining thesame lack of ethanol sensitivity in PA-3 which stably expressthe $alpha$ 1/ $beta$ 1/ $gamma$ 2_L subunit combination (Hadingham et al., 1992

Ethanol modulation of native GABA_A receptor function is independent of the expression of the $gamma$ 2_L subunit. In this study ethanol-induced potentiation of GABA-mediated responses was manifest in acutely dissociated immature Purkinjecells prior to the detection of $gamma$ 2_L mRNA expression, indicatinga lack of stringency for the expression of this subunit and thedevelopment of sensitivity to GABA_A receptor modulation by ethanol.Consistent with this finding, ethanol potentiated GABA-mediatedresponses in cultured Purkinje cells as early as 2 days in vitro,well before the onset of $gamma$ 2_L expression (H.H. Yeh, unpublishedobservation).

In the adult state, cerebellar Purkinje cells express a relatively simple combination of $alpha$ 1, $beta$ 2, $beta$ 3 and $gamma$ 2 receptor subunitsas determined by in situ hybridization (Laurie et al., 1992

) andimmunocytochemistry (Gutierrez et al., 1994

). Both long and shortsplice variants of the $gamma$ 2 subunit are present in approximatelyequal levels in the adult but, before postnatal day 7 during development,only the expression of the $gamma$ 2_S subunit is detected (Bovolin etal., 1992

; Wang and Burt, 1991

). Although the presence of a givenGABA_A receptor subunit mRNA transcript does not necessarily implytranslation and functional assembly of the encoded subunit protein,the absence of a given subunit mRNA transcript argues stronglyagainst the presence of the encoded protein. Thus, our observationthat ethanol potentiates GABA-activated current responses in immaturePurkinje cells, when only the $gamma$ 2_S subunit mRNA can be detected,provides compelling evidence against an absolute requirement ofthe $gamma$ 2_L subunit in conferring sensitivity to native GABA_A receptormodulation by ethanol. This information would not have been revealedwithout using the combination of patch clamp recording and singlecell RT-PCR. Indeed, other studies have failed to document thatethanol differentially modulates receptors containing either the $gamma$ 2_L or $gamma$ 2_S subunit. Sigel et al. (1993)

reported that recombinantGABA_A receptors expressed in Xenopus oocytes consisting of eitherthe $alpha$ 1 $beta$ 2 $gamma$ 2_L or $alpha$ 1 $beta$ 2 $gamma$ 2_S subunits were equally potentiated by ethanol.Ethanol also failed to differentiate [³⁵S]TBPS binding between $gamma$ 2_S- and $gamma$ 2_L-containing recombinant receptorscoexpressing either the $alpha$ 1 $beta$ 2 or $alpha$ 6 $beta$ 2 subunits (Korpi et al., 1995

The WSS-1 cell line was generated by stably transfecting HEK-293 cells with the $alpha$ 1/ $beta$ 2/ $gamma$ 2 combination of GABA_A receptor subunits,although the spliced form of the $gamma$ 2 transcript used for transfectionwas not defined (Wong et al., 1992

). Our RT-PCR-based mRNA profilingof the electrophysiologically recorded WSS-1 cells revealed theexpression of the $gamma$ 2_S transcript. This GABA_A receptor subunitprofile thus resembles that found in immature Purkinje cells beforepostnatal day 7. However, it should be noted that tests of ethanol-GABAinteraction in WSS-1 and Purkinje cells yielded contrasting outcomes.

Overall, the results of this study demonstrate that there are important inherent differences between GABA_A receptors expressedin cell lines and those expressed in neurons, and that rules governingthe relationship between subunit specificity and ethanol sensitivityin recombinant receptors may not be directly pertinent to thosegoverning native GABA_A receptors. Indeed, it would not be surprisingif posttranslational processes involved in the assembly of GABA_Areceptor subunits differ among cell lines and neurons in cultureor in situ. As a specific example, the state of phosphorylationof the GABA_A receptor may be a critical factor in assessing theoutcome of an interaction with ethanol. Phosphorylation triggeredby the activation of second messenger cascades has been demonstratedto play a role in mediating ethanol-induced potentiation of GABAresponses in hippocampal (Weiner et al., 1997

) and cerebellarPurkinje cells (Freund and Palmer, 1997

). Also, a PKC-null mutantmouse line has been reported to exhibit decreased behavioral sensitivityto ethanol (Harris et al., 1995b

). GABA-mediated Cl uptake in synaptoneurosomes prepared from control mice but notfrom PKC-null mutant mice was potentiated by ethanol. Along thisline of thought, data derived from cell lines to determine thesubunit dependence or specificity underlying sensitivity to modulationby ethanol should be interpreted with caution in light of theirapplicability towards understanding interactions between ethanoland native GABA_A receptors.

	Acknowledgments

The authors thank Dr. Paul Whiting for the generous gift of the PA3 and X25 cell lines and Dr. E. V. Grigorenko for assistancein obtaining the data illustrated in figure 6.

	Footnotes

Accepted for publication October 28, 1997.

Received for publication August 12, 1997.

¹ This work was supported by PHS Grants AA09861 to HHY. D.W.S. was supported in part by ARC T32 AA07209.

Send reprint requests to: Douglas W. Sapp, Department of Pharmacology, MC6125, University of Connecticut Health Center, 263 Farmington Avenue, Farmington, CT 06030.

	Abbreviations

GABA, $gamma$ -aminobutyric acid; PKC, protein kinase C; DMEM, Dulbecco's modified eagle medium; PD, postnatal day; DMSO, dimethylsulfoxide; RT-PCR, reverse-transcriptase polymerase chain reaction; TBPS, t-butylbicylcophosphorothionate; I_max, maximal current; DZ, diazepam; EtOH, ethanol.

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				G. Akk and J. H. Steinbach Low doses of ethanol and a neuroactive steroid positively interact to modulate rat GABAA receptor function J. Physiol., February 1, 2003; 546(3): 641 - 646. [Abstract] [Full Text] [PDF]

				H. E. Criswell, Z. Ming, B. L. Griffith, and G. R. Breese Comparison of Effect of Ethanol on N-Methyl-D-aspartate- and GABA-Gated Currents from Acutely Dissociated Neurons: Absence of Regional Differences in Sensitivity to Ethanol J. Pharmacol. Exp. Ther., January 1, 2003; 304(1): 192 - 199. [Abstract] [Full Text] [PDF]

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				T. Narahashi Neuroreceptors and Ion Channels as the Basis for Drug Action: Past, Present, and Future J. Pharmacol. Exp. Ther., July 1, 2000; 294(1): 1 - 26. [Abstract] [Full Text]

				M. J. VanDoren, D. B. Matthews, G. C. Janis, A. C. Grobin, L. L. Devaud, and A. L. Morrow Neuroactive Steroid 3alpha -Hydroxy-5alpha -Pregnan-20-One Modulates Electrophysiological and Behavioral Actions of Ethanol J. Neurosci., March 1, 2000; 20(5): 1982 - 1989. [Abstract] [Full Text] [PDF]

				C. Ikonomidou, P. Bittigau, M. J. Ishimaru, D. F. Wozniak, C. Koch, K. Genz, M. T. Price, V. Stefovska, F. Hörster, T. Tenkova, et al. Ethanol-Induced Apoptotic Neurodegeneration and Fetal Alcohol Syndrome Science, February 11, 2000; 287(5455): 1056 - 1060. [Abstract] [Full Text]

				H. E. Criswell, T. J. McCown, Z. Ming, R. A. Mueller, and G. R. Breese Interactive Role for Neurosteroids in Ethanol Enhancement of gamma -Aminobutyric Acid-Gated Currents from Dissociated Substantia Nigra Reticulata Neurons J. Pharmacol. Exp. Ther., December 1, 1999; 291(3): 1054 - 1059. [Abstract] [Full Text]

Ethanol-GABAA Receptor Interactions: A Comparison between Cell Lines and Cerebellar Purkinje Cells1

Ethanol-GABA_A Receptor Interactions: A Comparison between Cell Lines and Cerebellar Purkinje Cells¹