gamma -Hydroxybutyric Acid and Diazepam Antagonize a Rapid Increase in GABAA Receptors alpha 4 Subunit mRNA Abundance Induced by Ethanol Withdrawal in Cerebellar Granule Cells

doi:10.1124/mol.63.4.896

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Vol. 63, Issue 4, 896-907, April 2003

$gamma$ -Hydroxybutyric Acid and Diazepam Antagonize a Rapid Increase in GABA_A Receptors $alpha$ ₄ Subunit mRNA Abundance Induced by Ethanol Withdrawal in Cerebellar Granule Cells

Paolo Follesa, Luisa Mancuso, Francesca Biggio, Maria Cristina Mostallino, Annalisa Manca, Maria Paola Mascia, Fabio Busonero, Giuseppe Talani, Enrico Sanna, and Giovanni Biggio

Department of Experimental Biology "Bernardo Loddo", University of Cagliari, Cagliari, Italy (P.F., L.M., F.B., A.M., F.B., G.T., E.S., G.B.); CNR Institute of Neuroscience, Section of Neuropsychopharmacology, Cagliari, Italy (M.C.M., M.P.M., G.B.)

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

Both benzodiazepines and $gamma$ -hydroxybutyric acid (GHB) are used to treat alcohol withdrawal syndrome. The molecular basis forthis therapeutic efficacy was investigated with primary culturesof rat cerebellar granule cells. Long-term exposure of these cellsto ethanol (100 mM, 5 days) reduced the abundance of mRNAs encodingthe $gamma$ ₂L and $gamma$ ₂S subunits of the GABA type A receptor ( $-$ 32 and $-$ 23%, respectively) but failed to affect that of $alpha$ ₁, $alpha$ ₄, or $alpha$ ₆subunit mRNAs. Subsequent ethanol withdrawal resulted in decreasesin the amounts of $alpha$ ₁ ( $-$ 29%), $alpha$ ₆ ( $-$ 27%), $gamma$ ₂L ( $-$ 64%), and $gamma$ ₂S ( $-$ 76%),subunitmRNAs that were maximal after 6 to 12 h. In contrast, 3 h afterethanol withdrawal, the abundance of the $alpha$ ₄ subunit mRNA was increasedby 46%. Ethanol withdrawal did not affect neuronal morphologybut reduced cellular metabolic activity. The increase in $alpha$ ₄ subunitwas confirmed by functional studies showing a positive actionof flumazenil in patch clamp recordings of GABA-stimulated currentsafter ethanol withdrawal. Diazepam (10 µM) or GHB (100 mM) preventedthe increase in the amount of the $alpha$ ₄ subunit mRNA, the metabolicimpairment, and the positive action of flumazenil induced by ethanolwithdrawal but failed to restore the expression of the $alpha$ ₁ and $gamma$ ₂ subunits. The antagonism by GHB seems not to be mediated bya direct action at GABA_AR because GHB failed to potentiate theeffects of GABA or diazepam on Cl currents mediated by GABA type Areceptor.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

Ethanol elicits its central effects through modulation of neurotransmission mediated by various receptors, especially thatmediated by GABA type A receptors (GABA_AR) (Crews et al., 1996;Mehta and Ticku, 1999a). GABA_AR are heterogeneous in that theycomprise various combinations of subunits (Barnard et al., 1998).The absence or presence of particular $alpha$ subunit isoforms in thesereceptors confers selectivity for certain drugs (Barnard et al.,1998). Different $alpha$ subunits also mediate distinct pharmacologicalactions of benzodiazepines, including sedative-hypnotic (Rudolphet al., 1999), anxiolytic, and myorelaxant (Low et al., 2000)effects. Long-term treatment either of rats or of cultured neuronswith drugs that modulate GABAergic function, such as benzodiazepines(Holt et al., 1996; Follesa et al., 2001), barbiturates (Tyndaleet al., 1997), and steroids (Yu et al., 1996; Concas et al., 1998;Follesa et al., 1998; Smith et al., 1998a,b; Follesa et al., 2000)affects the expression of the genes for various GABA_AR subunits.Long-term ethanol administration also affects the subunit compositionand, consequently the functional properties, of native GABA_AR(Morrow et al., 1990; Mhatre et al., 1993; Devaud et al., 1997).The pharmacological profile of ethanol is highly similar to thatof benzodiazepines. Long-term exposure to ethanol, like that tobenzodiazepines, also results in the development of toleranceand dependence. The precise molecular mechanism by which prolongedethanol consumption modifies GABA_AR function, however, has remainedunknown.

Benzodiazepines are among the safest and most effective drugs used in the treatment of alcohol withdrawal syndrome. $gamma$ -Hydroxybutyricacid (GHB), a GABA metabolite naturally present in the brain thatin pharmacological doses modulates a variety of neurotransmissionsystems (Gessa et al., 1968; Bernasconi et al., 1999), has alsobeen proposed for use in the treatment of persons with this condition(Gallimberti et al., 1992; Addolorato et al., 1998). Althoughspecific recognition sites for GHB have been identified in thebrain (Benavides et al., 1982), it remains unclear whether allthe effects of this compound are mediated by these sites. GHBreduces the self-administration of alcohol and suppresses alcoholwithdrawal signs in alcohol-preferring rats (Fadda et al., 1989).In humans, a single dose of GHB has been shown to suppress alcoholwithdrawal symptoms for several hours, and repeated administrationincreases the number of days of abstinence from alcohol and reducesthe number of drinks per day (Gallimberti et al., 1992). However,the molecular mechanism responsible for these effects is notknown.

We have recently shown that long-term exposure to and subsequent withdrawal of benzodiazepines, zaleplon, zolpidem, or neurosteroidsresult in selective changes in the expression of specific GABA_ARmRNA and polypeptide subunits and in GABA_AR function in culturedcerebellar granule cells (Follesa et al., 2000, 2001, 2002). Inparticular, discontinuation of long-term treatment of the culturedneurons with diazepam both resulted in a selective increase inthe abundance of the $alpha$ ₄ subunit mRNA and polypeptide and prolongeda decrease in the amounts of the $alpha$ ₁ and $gamma$ ₂ subunit mRNA and correspondingprotein that was already apparent during long-term drug exposure(Follesa et al., 2001). These changes in mRNA and correspondingprotein produced changes in receptor function (Follesa et al.,2001). Long-term diazepam administration produced a reductionin the efficacy of this drug in potentiating the GABA-evoked Cl currents (Follesa et al., 2000, 2001). In the same article, wedemonstrated that withdrawal from diazepam or imidazenil was associatedwith both a reduced ability of diazepam to potentiate GABA actionand the ability of flumazenil to potentiate GABA action. Thiseffect of flumazenil in withdrawal cells resulted from the increaseof the $alpha$ ₄ subunit mRNA and corresponding protein (Follesa et al.,2000, 2001).

Given that long-term ethanol administration and withdrawal elicit neurochemical and molecular effects similar to those inducedby drugs able to activate GABA_AR (Morrow et al., 1990; Mhatreet al., 1993; Devaud et al., 1997), we have now studied primarycerebellar granule cell cultures subjected to abrupt discontinuationof ethanol treatment and evaluated the effects of diazepam andGHB during ethanol withdrawal on the gene expression and functionof the GABA_AR. The use of this exemplified model system will providenew insights that might help to understand, the role played bysingle subunits of the GABA_AR duringwithdrawal.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

Cell Culture. Primary cultures of cerebellar neurons enriched in granule cells were prepared from cerebella of 8-day-old rats. After culturefor 8 days, these cells contain the mRNAs for all 14 subunitsof the GABA_AR with an expression pattern similar to that apparentin the postnatal developing cerebellum but different from thatobserved in the adult rat cerebellum. Cells were plated (12.5× 10⁶ cells in 10 ml per dish) in 100-mm dishes that had been coatedwith poly(L-lysine) (10 µg/ml; Sigma, St. Louis, MO). For theelectrophysiological recording, cells were plated (3 × 10⁵ cells in 1 ml) in multiwell plates containing, in each well,12-mm round coverslips coated with poly(L-lysine). Cells fromeither type of plating were cultured in basal Eagle's medium (Invitrogen,Carlsbad, CA) supplemented with 10% heat-inactivated fetal bovineserum (Invitrogen), 2 mM glutamine, gentamicin (100 µg/ml; Sigma),and 25 mM KCl. Such a high concentration of potassium was necessaryto induce a persistent depolarization, which promotes the survivalof granule cells. Cytosine arabinofuranoside (final concentration,10 µM; Sigma) was added to the cultures 18 to 24 h after platingto inhibit the proliferation of non-neuronalcells.

After 3 days in culture, the cells were exposed for 5 days to ethanol at the indicated concentrations. In some ethanol-withdrawalexperiments, the medium containing ethanol was then replaced withethanol-free medium containing GHB (at the indicated concentrations)or diazepam (10 µM). Ethanol was diluted in medium, GHB was dissolvedin medium, and diazepam was dissolved in dimethyl sulfoxide andsubsequently diluted in medium. Control cells were treated withthe corresponding vehicle. The culture medium was replaced everyday with fresh medium containing the indicateddrug.

Probe Preparation. The cDNA for each subunit of the GABA_AR studied was prepared as described previously (Follesa et al., 1998) by reverse transcriptionand polymerase chain reaction (PCR). In brief, cDNA prepared fromrat brain (1-10 ng) was amplified by PCR with TaqDNA polymerase(2.5 U; PerkinElmer, Boston, MA) in 100 µl of standard buffer(100 mM Tris-HCl, pH 8.3, 500 mM KCl, 15 mM MgCl₂, and 0.01% gelatin)containing 1 µM each of specific sense and antisense primers and200 µM of each deoxynucleoside triphosphate. The primer pairsfor the various subunits of the GABA_AR were designed to includecDNA sequences with the lowest degree of intersubunit homology(Follesa et al., 1998). The primers used to amplify the $alpha$ ₆ subunitcDNA were 5'-GGGAAAAAGTCAATTGCTCAC-3' and 5'-CTCCTTATTAATCC-3'(upstream and downstream, respectively). The reaction was performedin a thermal cycler (Eppendorf) for 30 cycles of 94°C for 45 s,60°C for 1 min, and 72°C for 1 min, with a final extension at72°C for 15 min. The PCR products were separated by electrophoresis,visualized by staining with ethidium bromide, excised from thegel, purified, and cloned into the pAMP 1 cloning vector (Invitrogen).Escherichia coli DH5 $alpha$ was transformed with the resulting plasmids,which were subsequently purified from the bacteria and the cDNAinserts were sequenced with a Sequenase DNA sequencing kit (USB,Cleveland, OH). The determined nucleotide sequences were 100%identical to the respective previously published sequences. Plasmidscontaining the cDNA fragments corresponding to the various GABA_ARsubunits were linearized with restriction enzymes (Follesa etal., 1998) and then used as templates, together with the appropriateRNA polymerase (SP6 or T7) to generate [ $alpha$ -³²P]UTP-labeled cRNA probes for RNase protectionassays.

RNA Extraction and Measurement of GABA_AR Subunit mRNAs. Total RNA was isolated from cultured cerebellar granule cells by the guanidine isothiocyanate method as described previously(Follesa et al., 1998) and quantified by measurement of absorbanceat 260 nm. An RNase protection assay for the semiquantitativedetection of the GABA_AR $alpha$ ₁, $alpha$ ₄, $alpha$ ₆, $gamma$ ₂L, and $gamma$ ₂S subunit mRNAswas performed as described previously (Follesa et al., 1998).In brief, 25 µg of total RNA was dissolved in 20 µl of hybridizationsolution containing 150,000 cpm of ³²P-labeled cRNA probe for a specific GABA_AR subunit mRNA (specificactivity, 6 × 10⁷ to 7 × 10⁷ cpm/µg) and 15,000 cpm of ³²P-labeled cyclophilin cRNA (1 × 10⁶ cpm/µg). Given that cyclophilin is expressed widely among tissues,including the brain, and that its gene is most likely regulatedin an "on or off" manner, we used cyclophilin mRNA as an internalstandard for our measurements (Follesa et al., 1998). The hybridizationreaction mixture was incubated overnight at 50°C and then subjectedto digestion with RNase, after which RNA-RNA hybrids were detectedby electrophoresis (on a sequencing gel containing 5% polyacrylamideand urea) and autoradiography. The amounts of GABA_AR subunit mRNAand cyclophilin mRNA were determined by measuring the opticaldensity of the corresponding bands on the autoradiogram with adensitometer (GS-700; Bio-Rad, Hercules, CA); this instrumentis calibrated to detect saturated values, so that all our measurementswere in the linear range. The data were normalized by dividingthe optical density of the protected fragment for each receptorsubunit mRNA by that of the respective protected fragment forcyclophilin mRNA. The amount of each receptor subunit mRNA wastherefore expressed in arbitraryunits.

Metabolic Activity of Cerebellar Granule Cells. The metabolic activity of live cerebellar granule cells was measured with the resazurin (TOX-8) system (Magnani and Bettini,2000). Resazurin (Sigma) is a dye that is blue in its oxidizedform and red in its reduced form. Bioreduction of the dye by viablecells can thus be monitored spectrophotometrically and providesan indicator of cellular energy status. Cerebellar granule cells(7 × 10⁵) were cultured in 24-well plates coated with poly(L-lysine) andcontaining 1 ml of minimum essential medium devoid of phenol red(Invitrogen) per well. They were treated for 5 days with ethanol(100 mM) and then subjected to ethanol withdrawal in the absenceor presence of GHB or diazepam as described above. Four replicawells were used for each treatment. After ethanol withdrawal for3 or 6 h, 100 µl of TOX-8 stock solution was added to each well,and the plate was incubated for 2 h in the dark under standardconditions (37°C, humidified atmosphere containing 5% CO₂). Theabsorbance of the dye was then measured at wavelengths of 600and 690 nm. The absorbance of blank wells containing culture mediumand the appropriate drug but lacking cells was also determined.The mean value of blank wells was subtracted from that of theexperimental wells to yield net absorbance values. Metabolic activitywas determined as the change in absorbance caused by resazurinreduction, and data are expressed as percentage change in metabolicactivity relative to that of control cells (not treated with ethanol).To verify that changes in metabolic activity were not caused bycell death, we also counted with a hemocytometer the number ofviable cells in each well after their removal with trypsin andstaining with trypanblue.

Whole-Cell Patch-Clamp Electrophysiological Recording. Immediately before recording, coverslips were transferred to a perfusion chamber (Warner Instruments, Hampden, CT), and cerebellargranule cells were visualized under a Nikon upright microscopeequipped with Nomarski optics. Membrane potentials were clampedat $-$ 60 mV with a Axopatch 200-B amplifier (Axon Instruments, UnionCity, CA). The resting membrane potential for the recorded neuronswas approximately $-$ 60 mV. Recording pipettes (borosilicate capillarieswith filament, outer diameter 1.5 mm; Sutter Instruments, Novato,CA) were prepared with a two-step vertical puller (Sutter Instruments)and had resistances between 4 and 6 M $Omega$ . Pipette capacitance andseries resistances were compensated, the latter at 60%. Currentsthrough the patch-clamp amplifier were filtered (eight-pole bessel,2 kHz) and digitized at 5.5 kHz using commercial software (pClamp8.1; AxonInstruments).

The external solution contained 130 mM NaCl, 5 mM KCl, 2 mM CaCl₂, 1 mM MgCl₂, 10 mM HEPES, pH 7.3, and 11 mM glucose (allchemicals from Sigma). The internal solution contained 140 mMCsCl, 2 mM MgCl₂, 1 mM CaCl₂, 10 mM EGTA, 10 mM HEPES, pH 7.3,and 2 mM 5'-ATP-Na₂ (all chemicals from Fluka, Buchs, Switzerland).Drugs were applied with a fast-exchange flow-tube perfusion systemdriven by motor (Warner Instruments Co.). GABA was applied ata concentration of 1 to 3 µM, which induced a current with anamplitude of 5 to 10% of the maximal response (EC₅₁₀).Flumazenil (3 µM) was applied at 30-s intervals. All experimentswere performed at room temperature (23-25°C). Data were analyzedby pClampFit 8.01 (Axon Instruments, Union City, CA). Modulationof GABA-evoked Cl currents by flumazenil is presented as percentage change, [(I'/I) $-$ 1] × 100%, where I is the average of control responses obtainedbefore application and after washout of drugs, and I' is the averageof agonist-induced response obtained from the same cell in thepresence ofdrugs.

Electrophysiological Recording Cloned GABA_AR. The human $alpha$ ₁, $beta$ ₂, and $gamma$ ₂L subunit cDNAs were subcloned into the pCDM8 vector (Invitrogen) for nuclear injection. Oocytes wereisolated from Xenopus laevis as described. A mixture of the threesubunit cDNAs (0.5 ng each in a total volume of 30 nl) was injectedinto the animal pole of each oocyte (Colman, 1984). One to 4 daysafter injection, oocytes expressing recombinant $alpha$ ₁₂₂Lreceptors were placed in a chamber (volume, ~100 µl) and perifused(2 ml/min) with modified Barth's solution (MBS) comprising 88mM NaCl, 1 mM KCl, 2.4 mM NaHCO₃, 10 mM HEPES-NaOH, pH 7.5, 0.82mM MgSO₄, 0.33 mM Ca(NO₃)₂, and 0.91 mM CaCl₂. GABA was dissolvedin MBS and applied for 30 s. Diazepam was dissolved in dimethylsulfoxide and then diluted in MBS; the final concentration ofsolvent in MBS was 1% and did not affect GABA responses. GHB wasdissolved in H₂O and then diluted in MBS. Diazepam and GHB wereeach applied for 60 s before their coapplication for 30 s witha concentration of GABA that induced a current with an amplitudeof 5 to 10% of the maximal response (EC₅₁₀).

Statistical Analysis. Data are presented as means ± S.E.M. and were subjected to analysis of variance (ANOVA) followed by Scheffé's F test. A pvalue of <0.05 was considered statisticallysignificant.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

Effects of Long-Term Ethanol Treatment on GABA_AR Subunit mRNA Abundance. Cerebellar granule cells were incubated for 5 days in the absence or presence of 10, 50, or 100 mM ethanol, after which theabundance of GABA_AR $alpha$ ₁, $alpha$ ₄, $alpha$ ₆, $gamma$ ₂L, and $gamma$ ₂S subunit mRNAs wasdetermined. Ethanol had no significant effect on the amounts ofthe $alpha$ ₁ (Fig. 1A), $alpha$ ₄ (Figs. 1B and 3), and $alpha$ ₆ (see below) subunitmRNAs. In contrast, ethanol induced a dose-dependent decreasein the abundance of the $gamma$ ₂L and $gamma$ ₂S splice variant mRNAs, withthe amounts of these transcripts being reduced by 32 and 23%,respectively, after incubation of cells with 100 mM ethanol (Fig.1, C and D).

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Fig. 1. Effects of long-term exposure to various ethanol concentrations on the abundance of GABA_AR $alpha$ and $gamma$ subunit mRNAs in cultured cerebellar granule cells. Cells were incubated for 5 days in the absence (control) or presence of 10, 50, or 100 mM ethanol, after which the amounts of GABA_AR $alpha$ ₁ (A), $alpha$ ₄ (B), $gamma$ ₂L (C), and $gamma$ ₂S (D) subunit mRNAs were measured by RNase protection assay. Data are means ± S.E.M. of values from three independent experiments and are expressed as a percentage relative to control values. *, p < 0.05; **, p < 0.01 versus control (ANOVA and Scheffé's F test).

Effects of Ethanol Withdrawal on GABA_AR Subunit mRNA Abundance. We next investigated the effects of ethanol withdrawal on the abundance of GABA_AR subunit mRNAs by incubating cerebellar granulecells first with 100 mM ethanol for 5 days and then in the absenceof ethanol for 3, 6, 12, or 24 h. Ethanol withdrawal induced adecrease in the abundance of the $alpha$ ₁ subunit mRNA that was alreadysignificant after 3 h, maximal after 6 h ( $-$ 29%), and no longerapparent at 24 h (Fig. 2A). Six hours after ethanol withdrawal,the abundance of the $alpha$ ₆ subunit mRNA was also significantly reduced[control cells, 100.0 ± 8.1%; cells treated with 100 mM ethanolfor 5 days, 105.6 ± 2.6%; cells subjected to ethanol withdrawalfor 6 h, 72.8 ± 2.6% (p < 0.05 versus control); data are means± S.E.M. of values from three independent experiments]. Threehours after ethanol withdrawal, the abundance of the $gamma$ ₂L and $gamma$ ₂Ssubunit mRNAs remained decreased by extents similar to those apparentduring long-term treatment. The amounts of these mRNAs declinedfurther with time, achieving minimal values (36 and 24%, respectively)12 h after ethanol withdrawal, before returning to control valuesat 24 h (Fig. 2, C and D). In contrast to the effects of ethanolwithdrawal on the abundance of the $alpha$ ₁, $alpha$ ₆, and $gamma$ ₂ subunit mRNAs,discontinuation of ethanol treatment induced a marked increasein the amount of the $alpha$ ₄ subunit mRNA (Figs. 2B and 3). This increasewas maximal (+46%) 3 h after ethanol withdrawal, remained significantat 6 h, and was no longer apparent at 12 h.

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Fig. 2. Time course of the effects of ethanol withdrawal on the abundance of GABA_AR subunit mRNAs in cerebellar granule cells. Cells were incubated first for 5 days with 100 mM ethanol and then for the indicated times in the absence of this agent. The amounts of GABA_AR $alpha$ ₁ (A), $alpha$ ₄ (B), $gamma$ ₂L (C), and $gamma$ ₂S (D) subunit mRNAs were determined by RNase protection assay. Data are means ± S.E.M. of values from three independent experiments and are expressed as a percentage relative to the corresponding value for control cultures incubated in the absence of ethanol. *, p < 0.05; **, p < 0.01 versus control (ANOVA and Scheffé's F test).

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Fig. 3. GABA_A receptor $alpha$ ₄ subunit mRNA detection by RNase protection assay, representative experiment. Autoradiograph showing positions of the GABA_A receptor $alpha$ ₄ subunit and cyclophilin (internal standard) mRNAs on a urea/polyacrylamide electrophoresis gel. Cells were treated with ethanol (100 mM; 5 days) (chronic ethanol) or subject to 3h withdrawal (ethanol withdrawal). Control cells were treated with solvent. The total RNA was extracted (as described under Materials and Methods) from cerebellar granule cells 8 days in culture. On each lane, 25 µg of total RNA from individual plates were loaded. Ethanol withdrawal produced up-regulation of the $alpha$ ₄ subunit mRNA (+53 as calculated by densitometry in this autoradiogram), whereas chronic ethanol did not significantly modify the levels of the $alpha$ ₄ subunit mRNA (+7% as calculated by densitometry in this autoradiogram). The mean values of several experiments are shown in Fig. 2B.

Effect of Ethanol on Neuronal Metabolism. Neither treatment with 100 mM ethanol for 5 days nor subsequent ethanol withdrawal for 6 h seemed to affect the morphologyof cerebellar granule cells (Fig. 4). In contrast, spectrophotometricmeasurement of resazurin reduction revealed that, whereas long-termethanol treatment did not effect the metabolic activity of thecultured cells, ethanol withdrawal induced a time-dependent decreasein metabolic activity (Fig. 5A). This impairment in cellular metabolismwas not attributable to cell death, given that the percentageof viable cells was not affected by either long-term ethanol treatmentor ethanol withdrawal (Fig. 5B).

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Fig. 4. Light micrographs of live rat cerebellar granule cells in culture. Top, control cells; middle, cells treated with 100 mM ethanol for 5 days; bottom, cells subjected to ethanol withdrawal for 6 h. Magnification, 50×.

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Fig. 5. Effects of chronic treatment with and withdrawal of ethanol on the metabolic activity (A) and viability (B) of cerebellar granule cells. A, cells were treated with 100 mM ethanol for 5 days (chronic EtOH) and then subjected to ethanol withdrawal for 3 or 6 h. Cellular metabolic activity was assessed by the spectrophotometric determination of resazurin reduction. Data are expressed as percentage change in metabolic activity relative to the metabolic activity of control cells not exposed to ethanol and are means ± S.E.M. of values from three independent experiments. *, p < 0.05 versus control (ANOVA and Scheffe's test). B, after measurement of metabolic activity, the cells were harvested by exposure to trypsin, and the number of viable cells was counted with a hemocytometer after staining with trypan blue. Data are means ± S.E.M. of three independent experiments.

Effects of Diazepam and GHB on Ethanol Withdrawal. Exposure of cerebellar granule cells to diazepam (10 µM) at the time of ethanol withdrawal completely antagonized the withdrawal-inducedincrease in the abundance of the $alpha$ ₄ subunit mRNA (Fig. 6A). Thereplacement of ethanol with diazepam also blocked the ethanolwithdrawal-induced impairment in cellular metabolism (Fig. 6B).

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Fig. 6. Antagonism by diazepam both of the increase in the abundance of the GABA_AR $alpha$ ₄ subunit mRNA (A) and of the impairment in cellular metabolism (B) induced by ethanol withdrawal in cerebellar granule cells. Cells were incubated first for 5 days with 100 mM ethanol and then for 3 h (A) or 6 h (B) after ethanol withdrawal in the absence or presence of 10 µM diazepam. The abundance of the $alpha$ ₄ subunit mRNA was measured by RNase protection assay (A) and cellular metabolic activity was measured with resazurin (B). Data are means ± S.E.M. of values from three independent experiments and are expressed as percentage change relative to the values for control cultures not exposed to ethanol. *, p < 0.01 versus ethanol withdrawal without diazepam (ANOVA and Scheffé's F test).

We also examined the effects of exposing cells to various concentrations (10 µM to 100 mM) of GHB at the time of ethanol withdrawal.GHB inhibited in a dose-dependent manner the increase in the abundanceof the $alpha$ ₄ subunit mRNA induced by discontinuation of ethanol treatment.Only the highest concentration tested (100 mM) resulted in completelyeffective inhibition (Fig. 7A), whereas the concentration of 50mM inhibited only partially but not significantly with a P valueof 0.094234. At a concentration of 100 mM, GHB also completelyprevented the ethanol withdrawal-induced impairment in cellularmetabolism, whereas at a concentration of 50 mM, the inhibitionwas only partial but significant (Fig. 7B). In contrast, neitherdiazepam nor GHB, at concentrations that blocked the ethanol withdrawal-inducedincrease in the abundance of the $alpha$ ₄ subunit mRNA, had a significanteffect on the decrease in the abundance of the $alpha$ ₁ or $gamma$ ₂ subunitmRNAs induced by ethanol withdrawal (Fig. 8).

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Fig. 7. Dose-dependent antagonism by GHB both of the increase in the abundance of the GABA_AR $alpha$ ₄ subunit mRNA (A) and of the impairment in cellular metabolism (B) induced by ethanol withdrawal in cerebellar granule cells. Cells were incubated first for 5 days with 100 mM ethanol and then for 3 h (A) or 6 h (B) after ethanol withdrawal in the absence or presence of the indicated concentrations of GHB. The abundance of the $alpha$ ₄ subunit mRNA was measured by RNase protection assay (A) and cellular metabolic activity was measured with resazurin (B). Data are means ± S.E.M. of values from seven (A) or three (B) independent experiments and are expressed as percentage change relative to the values for control cultures not exposed to ethanol. *, p < 0.05; **, p < 0.01 versus ethanol withdrawal without GHB (ANOVA and Scheffé's F test).

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Fig. 8. Lack of effect of GHB or diazepam on the decrease in the abundance of GABA_AR $alpha$ ₁ (A), $gamma$ ₂L (B), and $gamma$ ₂S (C) subunit mRNAs associated with ethanol withdrawal in cerebellar granule cells. Cells were incubated first for 5 days with 100 mM ethanol and then for 3 h after ethanol withdrawal in the absence or presence of 100 mM GHB or 10 µM diazepam. The amounts of GABA_AR mRNAs were determined by RNase protection assay. Data are means ± S.E.M. of values from three independent experiments and are expressed as percentage change relative to the values for control cultures not exposed to ethanol. *, p < 0.01 versus control (ANOVA and Scheffé's F test).

Functional Characterization of GABA_AR after Long-Term Ethanol Treatment and Withdrawal. To evaluate the functional consequences of the increase in $alpha$ ₄ subunit mRNA induced by ethanol withdrawal, we examined theability of flumazenil in modulating the GABA_AR function by patch-clampelectrophysiological recording of single cerebellar granule cellsin culture. The modulatory action of flumazenil in granule cellsthat underwent extended treatment with ethanol was similar tothat measured in control granule cells (Fig. 9). In contrast,in ethanol-withdrawn granule cells, 3 µM flumazenil potentiates(+53 ± 5%) the GABA-evoked Cl current [Fig. 9a result consistent with the ethanol withdrawal-inducedup-regulation of the $alpha$ ₄ subunit in these cells (see Fig. 2 and3)]. Finally, the substitution of 10 µM diazepam or 100 mM GHBfor ethanol abolished the positive modulation of 3 µM flumazenilinduced by ethanol withdrawal (Fig. 9). This finding is in agreementwith the capability of these drugs to abolish the ethanol withdrawal-inducedup-regulation of the $alpha$ ₄ subunit (see Figs. 6A and 7A).

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Fig. 9. Potentiation of GABA_AR function by flumazenil in ethanol withdrawn cerebellar granule cells: reversal by diazepam and GHB. Cells were treated with 100 mM ethanol for 5 days (chronic) or subjected to ethanol withdrawal for 6 h (withdrawal). In other two groups of cells, 10 µM diazepam (withdrawal+diazepam) or 100 mM GHB (withdrawal+GHB) were substituted for ethanol for 6h. Whole-cell patch-clamp electrophysiological recording was performed by applying GABA at a concentration of 1 to 3 µM, which induced a current with an amplitude of 5 to 10% of the maximal response (EC₅₁₀). GABA was then coapplied with flumazenil 3 µM. A, representative electrophysiological recording traces of the indicated experimental groups. B, means ± S.E.M. values of 6 (control and chronic) to 7 (withdrawal, withdrawal+diazepam, withdrawal+GHB) recordings from individual neurons expressed as percentage of flumazenil potentiation of the response to GABA. *, P < 0.01 versus control; #, P < 0.01 versus withdrawal.

Lack of Effect of GHB on GABA_AR Function. Finally, we examined whether GHB affects the function of recombinant $alpha$ ₁ $beta$ ₂ $gamma$ ₂L GABA_AR expressed in X. laevis oocytes. GHB (10µM to 100 mM) had no effect on Cl currents induced by GABA at an EC_{5 to 10} (6 to 10 µM) (Fig. 10A).In the absence of GABA, GHB was also unable to activate directlythe GABA_AR complex at concentrations up to 100 mM (data not shown).Moreover, GHB (1 to 50 mM) failed to affect the enhancement ofGABA-evoked Cl currents induced by 1 µM diazepam (Fig. 10B). These results weresupported by our recent observation that GHB also fails to modulatethe GABA-evoked Cl currents in cerebellar granule cells and hippocampal pyramidalneurons in culture (E. Sanna, unpublished observations).

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Fig. 10. Lack of effect of GHB on the function of recombinant GABA_AR ( $alpha$ ₁₂₂L) expressed in X. laevis oocytes. A, oocytes were exposed to the indicated concentrations of GHB for 1 min before coapplication with GABA at an EC_{5 to 10} (6 to 10 µM) for 30 s. B, oocytes were exposed to GHB alone at the indicated concentrations (open bars), to GHB plus 1 µM diazepam (striped bars), or to 1 µM diazepam alone (solid bars) for 1 min before respective coapplication with GABA at an EC_{5 to 10} for 30 s. Data in A and B are expressed as percentage change of the GABA-induced Cl current and are means ± S.E.M. of values from four oocytes.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

We have shown that long-term exposure of primary rat cerebellar granule cells to a high concentration (100 mM) of ethanolresults in a decrease in the abundance of GABA_AR $gamma$ ₂ subunit mRNAs,consistent with the previous observation that prolonged alcoholadministration induces a reduction in GABAergic transmission inrat brain (Sanna et al., 1993). This effect of long-term ethanoltreatment in cultured cerebellar granule cells is similar to thatof long-term treatment with benzodiazepines or neurosteroids inthe same culture system (Follesa et al., 2000, 2001). Long-termethanol treatment did not affect the abundance of $alpha$ ₁, $alpha$ ₄, or $alpha$ ₆subunit mRNAs in the culturedneurons.

In an attempt to characterize the mechanism responsible for the development of ethanol dependence, several laboratories havepreviously examined the effects of ethanol on the abundance ofGABA_AR subunit mRNAs and peptides in the brain, obtaining differentresults that seem to depend on the method and time of intoxicationused or the brain region examined (for review, see Grobin et al.,1998). Ethanol administration for 12 weeks has thus previouslybeen shown to induce a decrease in the abundance of the $alpha$ ₁ subunitmRNA and peptide in the rat hippocampus (Charlton et al., 1997);such treatment for shorter time (2 weeks), however, had no effectin hippocampus, cerebellum, and frontal cortex (Charlton et al.,1997). Other studies, on the contrary, show that the amount ofthe $alpha$ ₁ subunit itself was reduced in the cerebral cortex and cerebellumby long-term treatment of rats with ethanol, whereas in the cerebellum,the $alpha$ ₆ subunit was increased (for review, see Grobin et al., 1998).These last observations were not fully supported by binding studies;in fact, an increase or no change in [³H]zolpidem binding was observed in the same brain areas (for review,see Grobin et al., 1998). With such a decrease in the expressionof the $alpha$ ₁ mRNA subunit and peptide, however, one should expecta decrease in [³H]zolpidem binding. A more recent study (Mehta and Ticku, 1999b),in agreement with our present data, demonstrated that long-termethanol administration did not result in down-regulation of GABA_ARassemblies containing the $alpha$ ₁ subunit in the rat cerebral cortexor cerebellum, as determined by labeling of the receptors with[³H]muscimol, [³H]flunitrazepam, [³H]Ro 15-4513, or [³H]zolpidem and immunoprecipitation with antibodies specific forthe $alpha$ ₁ subunit. This last observation, although consistent withour data, is in disagreement with a previous study from the samegroup, in which long-term ethanol treatment increased the [³H]Ro 15-4513 binding (Mhatre et al., 1988).

Given that the genes encoding for the $alpha$ ₁ and $alpha$ ₆ subunits are localized in the same cluster, the direction of change in theirgene expression should be the same, because these genes are coregulated(Holt et al., 1996). Our results in cerebellar granule cells inculture are consistent with the above hypothesis showing a similarpatterns of expression of the $alpha$ ₁ and $alpha$ ₆ genes in cells subjectedeither to long-term ethanol treatment (no change in abundance)or to ethanol withdrawal (a decrease in abundance). Thus, theapparent discrepancies in the effects of long-term ethanol exposureon the gene expression of these two subunits might be attributableto the difficulty in optimizing, in the studies "in vivo," thetiming between consecutive ethanol administrations so as to preventthe onset of withdrawal effects. On the contrary, in our modelsystem, it is very simple to perform ethanol withdrawal. Thus,the abrupt discontinuation of ethanol treatment resulted in adecrease in the abundance of the $alpha$ ₁ and $alpha$ ₆ subunit mRNAs, as wellas prolongation and enhancement of the decrease in the amountsof both $gamma$ ₂ subunit mRNAs. Ethanol withdrawal also induced a markedincrease in the abundance of the $alpha$ ₄ subunit mRNA. This lattereffect was rapid and therefore might be important in the onsetof withdrawal syndrome. These changes in GABA_AR gene expressionare identical to those induced by withdrawal of either benzodiazepines(Follesa et al., 2001), imidazopyridines and pyrazolopyrimidines(Follesa et al., 2002), or neurosteroids (Follesa et al., 2000).These molecular changes thus might reflect a common mechanismby which diazepam and ethanol trigger changes in receptor functionthat in vivo might account for the development of withdrawal symptoms.The presence of the $alpha$ ₄ subunit in recombinant GABA_AR is associatedwith a reduced sensitivity to classical benzodiazepine agonistsand to zolpidem as well as with a distinct pattern of regulation(positive rather than no allosteric modulation) by flumazenil.The patch-clamp studies demonstrated that in the ethanol-withdrawngranule cells, flumazenil positively modulates the GABA_AR function,in agreement with the observation that in these cells, ethanolwithdrawal produced up-regulation of the $alpha$ ₄ subunit mRNA. Thus,the increase in the abundance of the $alpha$ ₄ subunit mRNA induced bywithdrawal of ethanol, diazepam, or neuroactive steroids mightcontribute to changes in the sensitivity of GABA_AR to drugs andendogenousmodulators.

The effects of ethanol withdrawal on GABA_AR gene expression were accompanied by a decrease in cellular metabolic activity.This impairment in metabolism also might play a role in the developmentof dependence on ethanol or it might represent a homeostatic responseof the neurons to the sudden lack of ethanol in the culture medium.Long-term exposure to ethanol (100 mM) had no apparent effecton metabolic activity or on neuronal morphology and was not cytotoxic,given that the number of viable cells wasunchanged.

Benzodiazepines are one of the best treatments available for the life-threatening condition of alcohol withdrawal syndromein humans (Mayo-Smith, 1997). These drugs prevent the more severeclinical manifestations of the syndrome, such as seizures anddelirium. GHB has also more recently been proposed as an alternativetreatment to reduce alcohol consumption and craving in personswith alcoholism. In laboratory animals, GHB and alcohol exhibitcross-tolerance to their mutual side effects (Colombo et al.,1995). Moreover, GHB reduces self-administration of alcohol andsuppresses alcohol withdrawal signs in alcohol-preferring rats(Fadda et al., 1989). A comparison between benzodiazepines andGHB in the management of alcohol withdrawal syndrome in humansrevealed that GHB is as effective as diazepam and seems to reduceanxiety, agitation, and depression more rapidly (Addolorato etal., 1999).

The substitution of diazepam for ethanol after long-term ethanol treatment completely antagonized the marked increase in theabundance of the GABA_AR $alpha$ ₄ subunit mRNA, the decrease in cellularmetabolic activity induced by ethanol withdrawal, and the flumazenilpotentiation. The substitution of very high GHB concentrationsfor ethanol was as effective as diazepam in antagonizing the sameeffects. In contrast, neither diazepam nor GHB had any effecton the changes in the abundance of the $alpha$ ₁ and $gamma$ ₂ subunit mRNAsobserved during ethanol withdrawal. Given that the down-regulationof both $gamma$ ₂ subunits was trigged by long-term ethanol treatment,it is not surprising that diazepam did not antagonize this effect.On the other hand, it is more difficult to explain the lack ofeffect on the $alpha$ ₁ subunit. Nevertheless, we can hypothesize thathigher concentrations of diazepam might be necessary to overcomethe decrease of the $alpha$ ₁ subunit induced by ethanol withdrawal.Because the $alpha$ ₁ subunit has been demonstrated to mediate the sedative-hypnoticeffects of benzodiazepines (Rudolph et al., 1999), our speculationis supported by the clinical observation that to sedate patientsduring alcohol withdrawal massive doses and continuous infusionof benzodiazepines are necessary (Sellers et al., 1983).

The antagonism by diazepam and very high concentrations of GHB on the changes in $alpha$ ₄ subunit mRNA, consequent receptor function,and cellular metabolism induced by ethanol withdrawal supportthe possible crucial role of the $alpha$ ₄ subunit in the molecular mechanismsof withdrawal. Withdrawal from steroids has previously been shownto alter the kinetics of GABA_AR-mediated currents in the rat hippocampusas well as to increase both the abundance of the $alpha$ ₄ subunit andanxiety in pseudopregnant animals (Smith et al., 1998b). Furthermore,suppression of the increase in the abundance of the $alpha$ ₄ subunitprevents withdrawal signs associated with endogenous steroidsin a progesterone withdrawal paradigm (Smith et al., 1998a).

Whereas the antagonism by diazepam we observed is consistent with the specific action of this drug at the GABA_AR complex,the mechanism by which GHB induces this same effect is not clear.Consistent with previous data showing that GHB does not seem topossess affinity for [³H]muscimol, t-[³⁵S]butylbicyclophosphorothionate, or [³H]flunitrazepam binding sites (Serra et al., 1991; Bernasconiet al., 1992), our present results on the GABA_AR function indicatethat GHB does not directly affect the activity of the GABA_AR nordoes it affect the action of allosteric modulators such as benzodiazepines.The affinities of GHB for its own specific receptor and for theGABA_B receptor are in the nanomolar and micromolar ranges, respectively(Bernasconi et al., 1992). Thus, despite the similarities betweenthe pharmacological properties of GHB and those of sedative-hypnoticdrugs, the effects of GHB do not seem to be mediated by GABA_AR.Rather, most of the effects of GHB, especially those induced byhigh concentrations of this drug, seem to be mediated by GABA_Breceptors or to be nonspecific. Thus, both biochemical and behavioraleffects of high doses of GHB are reproduced or potentiated byGABA_B receptor agonists (Bernasconi et al., 1999). Moreover, likeGHB, the GABA_B receptor agonist baclofen also protects againstalcohol dependence (Bernasconi et al., 1999).

In our experimental paradigm, the antagonistic action elicited by GHB on the ethanol withdrawal-induced up-regulation of the $alpha$ ₄ subunit of the GABA_AR, receptor function, and cellular metabolismwere observed only at the concentration of 100 mM. This concentrationof GHB was very high compared with that hypothetically achievedin human studies (Addolorato et al., 1999). The physiologicalconcentration of GHB in the mammalian brain ranges from 2 to 5µM, but this amount could be increased by several orders of magnitudeafter exogenous administration of GHB (Gobaille et al., 1999).Thus, we can speculate that the antagonistic action of GHB invivo could be the result of a synergic interaction between theelevated concentration of GHB and other endogenous modulatorsof neurotransmission. Accordingly, both ethanol and GHB greatlyincrease the levels of GABA_AR active steroids in the rat brain(Morrow et al., 2001; Barbaccia et al., 2002). Thus, in vivo,a lower dose of GHB might be sufficient to antagonize the effectsof ethanol. The same might not hold be true in neurons in culture,where the concentrations of steroids (Follesa et al., 2000) areirrelevant.

In conclusion, our data demonstrate that the ethanol withdrawal-induced increase in the expression of the GABA_AR $alpha$ ₄ subunitgene in cultured rat cerebellar granule cells is prevented bydiazepam and very high concentrations (100 mM) of GHB, two ofthe most widely used drugs in the treatment of alcohol withdrawalsyndrome in humans. This action of GHB does not seem to be mediatedby specific activation of GABA_AR. A rapid and marked increasein the abundance of the $alpha$ ₄ subunit may thus contribute to thedevelopment of alcohol withdrawal symptoms that are amelioratedby both GHB anddiazepam.

	Footnotes

Received August 12, 2002; Accepted January 7, 2003

This study was supported by Ministero dell'Istruzione dell'Universita e della Ricerca grant2001055774.

Address correspondence to: Dr. Paolo Follesa, Department of Experimental Biology, University of Cagliari, Cagliari 09123, Italy. E-mail: follesa{at}unica.it

	Abbreviations

GABA_AR, GABA type A receptors; GHB, $gamma$ -hydroxybutyric acid; PCR, polymerase chain reaction; MBS, modified Barth's solution; ANOVA, analysis of variance.

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-Hydroxybutyric Acid and Diazepam Antagonize a Rapid Increase in GABAA Receptors 4 Subunit mRNA Abundance Induced by Ethanol Withdrawal in Cerebellar Granule Cells

$gamma$ -Hydroxybutyric Acid and Diazepam Antagonize a Rapid Increase in GABA_A Receptors $alpha$ ₄ Subunit mRNA Abundance Induced by Ethanol Withdrawal in Cerebellar Granule Cells