Differential Effect of Ethanol on PC12 Cell Death

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	Articles by Rabin, R. A.

Vol. 287, Issue 1, 359-365, October 1998

Differential Effect of Ethanol on PC12 Cell Death¹

Jan Oberdoerster, Angela R. Kamer and Richard A. Rabin

Department of Pharmacology and Toxicology, School of Medicine and Biomedical Sciences (J.O., R.A.R.) and Department of Oral Biology, Department of Oral and Maxillofacial Surgery, School of Dental Medicine (A.R.K.), State University of New York at Buffalo, Buffalo, New York

	Abstract

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Our goal was to examine the effects of ethanol on cell death using rat pheochromocytoma (PC12) cells as a neuronal model.Withdrawal of serum for 24 hr increased the number of PC12 cellslabeled with ethidium homodimer indicating an increase in celldeath. Inclusion of 50 mM ethanol during the serum deprivationfurther increased the amount of ethidium fluorescence by 39%.Although reducing the serum concentration from the usual 15 to4% did not alter cellular viability, a significant increase inthe amount of ethidium fluorescence was observed in PC12 cellsincubated for 24 hr in the presence of 4% serum and 150 mM ethanol.No change in viability was observed in cells exposed to either150 mM ethanol in the presence of 15% serum or 50 mM ethanol inthe presence of 4% serum. Inclusion of ethanol during serum deprivationincreased the amount of soluble DNA found in the 15,000 × g supernatant.Similarly, using the terminal deoxynucleotidyl transferase dUTPnick-end labeling method to visualize DNA fragmentation in situ,ethanol caused a 213% increase in the number of PC12 cells labeledduring serum withdrawal. Agarose gel electrophoresis of the DNAisolated from cells maintained in the absence of serum yieldedthe classical DNA laddering pattern of 180 to 200 bp fragmentssuggestive of apoptosis. Ethanol caused a concentration-dependentincrease in the amount of DNA laddering in cells deprived of serum.Furthermore, ethanol significantly potentiated the DNA ladderingof cells maintained in 4% serum. In contrast to the ethanol-inducedincrease in cell death when serum factors were reduced or withdrawn,150 mM ethanol lowered by 34% the number of ethidium-labeled PC12cells observed after a 30-min exposure to 2 mM H₂O₂. Similarly,agarose gel electrophoresis of the DNA from H₂O₂-treated cellsdid not display DNA laddering. This study demonstrates that: 1)ethanol antagonizes the trophic action of serum factors; 2) pharmacologicallyrelevant ethanol concentrations significantly potentiate apoptosisafter serum withdrawal and 3) this enhancement appears specificfor apoptosis.

	Introduction

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FAS is a series of malformations and abnormalities occurring in children exposed to ethanol in utero and is the leading nongeneticcause of mental retardation in the world (West et al., 1994).The primary features of children with FAS are growth deficiencies,including microencephaly, craniofacial dysmorphology and centralnervous system dysfunction such as deficits in memory, attentionand IQ. In rodents, ethanol exposure during development significantlyreduces the size of the brain as well as brain/body weight ratios(Grant and Samson, 1982; Pierce and West, 1986). Similarly, magneticresonance imaging of individuals exposed prenatally to alcoholshow a reduction in the size of several brain areas includingthe diencephalon, basal ganglia and anterior vermis of the cerebellum(Mattson et al., 1992; Sowell et al., 1996). The ethanol-inducedmicroencephaly appears to be due to a decrease in cell numberas exposure of rats to ethanol in utero or during early postnataldevelopment reduces the number of neurons in the inferior olive(Napper and West, 1995), and principal sensory nucleus (Miller,1995), as well as decreasing the number of cerebellar Purkinjeand granule cells (Bonthius and West, 1990; West et al., 1990).Similarly, the addition of in vitro ethanol to primary culturesof cerebellar granule cells (Pantazis et al., 1993), neural crestcells (Chen and Sulik, 1996) and various transformed cell lines(Pantazis et al., 1992; Klein et al., 1996) results in a reductionin cell number.

The above reductions in cell number could be due to decreased proliferation, altered migration or increased cell death. Ethanoltreatment has been shown to cause a concentration-dependent decreasein proliferation of the neuron-like PC12 cells (Pantazis et al.,1992) as well as human astroglia in culture (Kane et al., 1996).Although neuronal proliferation in vivo also appears to be alteredby prenatal exposure to ethanol (Miller, 1986, 1988), at leastcerebellar Purkinje cells are more vulnerable to ethanol duringdifferentiation rather than during neurogenesis (Marcussen etal., 1994). In addition to alterations in cell proliferation,in utero ethanol exposure of rats has been reported to delay neuronalmigration and cause neuronal movement to ectopic locations (Miller,1993).

The ethanol-mediated reductions in neuronal number could be due to increased cell death; however, there is a paucity of dataon this subject. During normal development as many as 50% of theneurons in some regions of the central nervous system are lostvia a form of cell death referred to as apoptosis (Oppenheim,1991; Raff et al., 1993). This apoptotic death appears to be primarilycontrolled by a limiting supply of target-derived growth factorsand thus allows a matching of neuronal populations to target size.In addition to this developmental programmed cell death, apoptoticdeath also is observed in response to insults such as ethanol.An increase in the number of apoptotic cells in the livers ofmicropigs and rats was reported after chronic administration ofethanol (Yacoub et al., 1995; Halsted et al., 1996). Similarly,acute treatment of hepatocytes, lymphocytes and thymocytes withethanol increased the number of apoptotic cells (Slukvin and Jerrells,1995; Kurose et al., 1997). In a preliminary report, Hamby-Masonet al. (1996) noted an increase in the number of apoptotic cellsin various brain areas after postnatal exposure of rats to ethanol.

Our investigation was undertaken to determine the effects of ethanol on neuronal cell death using rat PC12 pheochromocytomaas a model system. These studies demonstrate that ethanol caninduce apoptosis in neuronal cells. In addition, pharmacologicallyrelevant concentrations of ethanol potentiate the apoptosis inducedby removal of serum factors. This is in contrast to the ethanol-inducedreduction in cell death caused by H₂O₂.

	Materials and Methods

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Materials. Cell culture media and agarose was purchased from Gibco BRL (Grand Island, NY). Fetal calf serum was purchased from HyCloneLaboratories (Logan, UT) and horse serum from JRH Biosciences(Lenexa, KS). The ethidium homodimer was purchased from MolecularProbes (Eugene, OR). For TUNEL assays, the biotin-16-dUTP waspurchased from Boehringer Mannheim (Indianapolis, IN), TdT andTdT buffer from USB (Cleveland, OH) and strepavidin-peroxidaseand hematoxylin from Zymed Laboratories (San Francisco, CA). ProteinaseK was purchased from Fisher Biotech (Fair Lawn, NJ) and RNaseA from Boehringer Mannheim. All other chemicals were purchasedfrom common commercial suppliers.

Tissue culture. PC12 cells were maintained at 37°C in DMEM containing 25 mM glucose, 4 mM glutamine and supplemented with 15% serum (i.e.,5% heat-inactivated horse serum, 10% fetal calf serum), 100 U/mlpenicillin and 100 µg/ml streptomycin. For experiments, PC12 cellswere removed from the culture plates by trituration in DMEM andcentrifuged at 800 × g for 3 min. The cell pellet was resuspendedin DMEM and the cells again centrifuged at 800 × g for 3 min.This procedure was repeated and the washed cells were plated ontocollagen-coated tissue culture plates in either serum-free orserum-containing medium. Ethanol exposure was carried out by includingethanol in the media and incubating the plates at 37°C in plasticdesiccators containing an atmosphere of 95% air, 5% CO₂ that wassaturated with the appropriate concentration of ethanol. Thissystem has been shown to result in an approximate 20% loss ofethanol from the medium after 2 days (Rabin, 1988).

Evaluation of cell death. PC12 cells, which were plated onto collagen-coated 24-well plates (0.8-1 × 10⁶ cells/well), were incubated for 1 hr in PBS containing 3 µg/mlof the DNA-binding fluorophore ethidium homodimer. Ethidium fluorescencewas measured using a fluorescent plate reader (535 nm excitation,645 nm emission). Preliminary studies had established that a 1-hrloading time resulted in maximum ethidium-DNA fluorescence.

Evaluation of DNA fragmentation. Cells were incubated in lysis buffer (5 mM Tris, 20 mM EDTA, 0.025% Triton X-100, pH 7.4) for 30 min on ice and then centrifugedat 15,000 × g for 15 min. The resulting pellet was resuspendedin 2 ml lysis buffer and briefly sonicated. The DNA contents ofthe 15,000 × g supernatant (fragmented DNA) and pellet were measuredusing the DNA-binding fluorophore Hoechst-33342 (2 µg/ml) as previouslydescribed (Labarca and Paigen, 1980). Salmon sperm DNA was usedas a standard, and DNA fragmentation was expressed as percenttotal DNA [i.e., DNA_sup/(DNA_sup + DNA_pellet)].

In situ detection of DNA fragmentation by TUNEL. PC12 cells, which were plated onto collagen-coated glass coverslips (8 × 10⁴ cells/cm²), were fixed in 4% formaldehyde for 15 min and then incubatedwith 100% ethanol for 5 min. The TUNEL reaction was performedby incubating the coverslips at 37°C in a final volume of 50 µlTdT reaction buffer (100 mM Na cacodylate, 0.2 mM 2-mercaptoethanol,2 mM CoCl₂ · 6 H₂O, 16 units TdT, 1.25 nM biotin-16-dUTP, pH 7.2).After 60 min, cells were incubated for 15 min with 30 mM Na citratecontaining 300 mM NaCl. The cells were then rinsed in distilledH₂O and covered with a 2% bovine serum albumin blocking solutionfor 10 min. The biotinylated 3'-OH DNA ends were visualized byreaction with strepavidin-peroxidase, and cells were counter-stainedwith hematoxylin following manufacturer directions (Zymed Laboratories).The extent of apoptosis was quantified by counting the numberof apoptotic events in a minimum of 20 randomly chosen fieldson each coverslip using 400× magnification. Nonspecific biotinylationwas evaluated by incubating sister coverslips in the above assaybuffer but in the absence of TdT. Additional sister coverslipsalso were used for a determination of both protein and DNA content.

Evaluation of DNA laddering. Cells were incubated on ice in lysis buffer (20 mM Tris, 5 mM EDTA, 0.025% Triton X-100, pH 7.5) for 30 min, and an aliquotof the cell lysate removed for determination of protein and DNAcontent. The lysate was centrifuged at 15,000 × g for 20 min,and the resulting supernatant incubated with RNase A (250 µg/ml)and Proteinase K (100 µg/ml) for 2 hr at 37°C. The samples wereextracted twice with phenol/chloroform (1:1) and once with chloroform.DNA was precipitated by incubating the sample for 30 min at $-$ 20°Cin 2 volumes 95% ethanol containing 0.3 M Na acetate. The samplewas then centrifuged at 20,000 × g for 15 min at 4°C, and theresulting pellet was either air dried or dried under vacuum ina Savant SpeedVac. The DNA pellet was resuspended in loading buffer(10 mM Tris, 1 mM EDTA, 5% glycerol, 0.25% bromphenyl blue, pH7.5), and the entire sample was then subjected to electrophoresison a 2% agarose gel using a TBE running buffer (89 mM Tris, 89mM boric acid, 2 mM EDTA, pH 8.3) containing 0.5 µg/ml ethidiumbromide. The cumulative fluorescence intensity of each of thelower bands (i.e., intensity of the DNA ladder) was measured usinga Bio-Rad Molecular Imaging system (Bio-Rad Lab., Hercules, CA).

Alternatively, a more sensitive and rapid DNA extraction method was also used (Gong et al., 1994

). Briefly, cells were removedin one volume Hanks' buffered salt solution (HBSS) and storedat $-$ 20°C in five volumes 70% ethanol for 24 hr. To remove theethanol, cells were collected by centrifugation at 800 × g for5 min and washed three times with HBSS. The cell pellets (1-2× 10⁷ cells) were subsequently resuspended in 100 µl phosphate-citratebuffer (192 mM Na₂HPO₄, 4 mM citric acid, pH 7.8) and incubatedfor 40 min at room temperature. An aliquot was removed for proteindetermination, and the remaining sample was centrifuged at 1000× g for 5 min. The volume of the resulting supernatant was thenreduced in half in a Savant SpeedVac concentrator. Samples wereincubated for 30 min at 37°C with 0.03% Nonidet NP-40 and 0.4mg/ml RNase A, and then incubated an additional 30 min at 37°Cin the presence of 0.4 mg/ml Proteinase K. The entire sample wasthen electrophoresed on a 2% agarose gel as described above afteraddition of 10× loading buffer.

Total cell protein/DNA determinations. For the determination of total cellular protein, cells were incubated in 0.1 N NaOH and protein content measured using thecolorimetric Bio-Rad protein dye binding procedure with bovineserum albumin (fraction V) as a standard. For the determinationof total cell DNA, cells were incubated in 5 mM Tris, 20 mM EDTA,0.025% Triton X-100 (pH 7.4) and DNA content measured as describedabove using salmon sperm DNA as a standard.

Statistical analysis. The effect of ethanol on serum withdrawal-induced DNA laddering was evaluated using a paired t test. The effect of ethanolon cell death at the various serum concentrations was evaluatedusing two-way analysis of variance. The remaining data were analyzedusing analysis of variance and the post hoc Student-Newman-Keulspairwise comparison procedure.

	Results

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Because during development some 50% of the neurons normally undergo cell death due, at least in part, to a loss of neurotrophicfactors (Oppenheim, 1991; Raff et al., 1993), the effects of ethanolon death induced by serum withdrawal were studied. A 24-hr incubationin serum-free media significantly (P < .05) increased the numberof cells labeled with the cell impermeable DNA-binding fluorophoreethidium homodimer (fig. 1). Inclusion of 50 mM ethanol in theserum-free media caused a significant 39% potentiation in thenumber of ethidium-labeled cells (fig. 1). Similarly, treatmentwith 150 mM ethanol significantly potentiated the amount of celldeath after serum withdrawal by 125% (data not shown). Ethanol,however, does not appear to be accelerating cell death. Comparedto control cells, serum removal for 6 hr increased the amountof ethidium-labeled cells 190 ± 15.7 and 223 ± 20.3% in the absenceand presence of 150 mM ethanol, respectively (N = 8). Althougha 24-hr inclusion of 150 mM ethanol in the presence of 15% serumdid not alter cell viability, a 3-day exposure resulted in a statisticallysignificant 42 ± 9.6% increase in the amount of ethidium-labeledcells (P < .01; N = 7). The above increases in ethidium fluorescencewere not due to a direct effect of ethanol on membrane permeabilityas addition of 150 mM ethanol during the 1 hr loading with thedye did not alter ethidium labeling of cells (data not shown).

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Fig. 1. Ethanol potentiates cell death due to serum withdrawal. PC12 cells were treated for 24 hr with 50 mM ethanol in the presence or absence of 15% serum. Cell death was determined using the fluorescent DNA-binding probe ethidium homodimer. Data are expressed as arbitrary fluorescent units/mg protein and are plotted as mean ± S.E.M. (*P < .05, N = 10).

The effect of ethanol on cells maintained in reduced serum also was evaluated using ethidium homodimer. Two-way analysis ofvariance of the cell death indicated both a significant effectof serum concentration (F_3,40 = 67.2, P < .0001), and a significantethanol treatment effect (F_1,40 = 67.2, P < .0001), as well asa significant ethanol/serum concentration interaction (F_3,40 =14.2, P < .0001). A posteriori statistical analysis indicatedthat lowering the serum concentration to 4 or 6% for 24 hr didnot alter cellular viability. Furthermore, a 3-day incubationin 4% serum did not lead to an increase in cell death; 4 ± 9.3%(N = 3) more cells were labeled with ethidium after 3 days in4% serum compared to sister plates maintained in the normal 15%serum for 3 days. The addition of 150 mM ethanol to cells maintainedin 4 or 6% serum, however, caused a significant induction of celldeath (fig. 2).

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Fig. 2. Ethanol exposure induces cell death at low serum concentrations. PC12 cells were treated with 150 mM ethanol in the presence of 15, 6, 4 or 1% serum (fetal calf serum and heat-inactivated horse serum at a ratio of 2:1) for 24 hr. Cell death was determined using the fluorescent DNA-binding probe ethidium homodimer. Data are expressed as arbitrary fluorescent units/mg protein and are plotted as mean ± S.E.M. (**P < .01, ***P < .001, N = 6). $bullet$ , 0 mM ethanol, $black-triangle$ , 150 mM ethanol.

To determine whether the increases in cell death by ethanol were specific to serum withdrawal, we investigated the effectof ethanol on free-radical induced cell death. PC12 cells exposedto 2 mM H₂O₂ in the presence of 15% serum displayed a significantincrease in cell death. However, contrary to cell death inducedby serum withdrawal, cotreatment with 150 mM ethanol significantlyreduced the amount of H₂O₂-mediated cell death by 34% (fig. 3).Cotreatment with a lower ethanol concentration (50 mM), however,did not significantly alter the free-radical induced cell death(data not shown).

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Fig. 3. Ethanol reduces cell death due to H₂O₂ exposure. PC12 cells were treated for 30 min with 150 mM ethanol in the presence or absence of 2 mM H₂O₂, and cell death was determined using the fluorescent DNA-binding probe ethidium homodimer. Data are expressed as arbitrary fluorescent units/mg protein and are plotted as mean ± S.E.M. (*P < .05, **P < .01, N = 8).

Ethanol has been reported to increase both apoptosis and necrosis (Koop et al., 1997; Zhong et al., 1993). Experiments weretherefore undertaken to determine which form of death was involvedin the above studies. Because cells undergoing apoptosis characteristicallycontain low molecular-weight DNA fragments due to internucleosomalcleavage of the chromatin into 180- to 200-bp fragments (Evansand Cidlowski, 1995), the effect of ethanol on DNA fragmentationwas evaluated. Serum withdrawal increased DNA fragmentation asindicated by a 149% increase in the relative amount of DNA inthe 15,000 × g supernatant of the cell lysate. This extent ofDNA fragmentation was further potentiated 74% by cotreatment with150 mM ethanol (fig. 4). Ethanol exposure in the presence of 15%serum did not alter DNA fragmentation.

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Fig. 4. Ethanol potentiates DNA fragmentation after serum withdrawal. Cells were treated for 24 hr with 150 mM ethanol in the presence or absence of 15% serum. DNA fragmentation was determined using the fluorescent DNA-binding probe Hoechst-33342. Data are expressed as percent total DNA [i.e., DNA_sup/(DNA_sup + DNA_pellet)] and are plotted as mean ± S.E.M. (**P < .01, N = 6).

The effects of ethanol on DNA fragmentation in situ were determined using the TUNEL technique which labels free 3'-OH endsof the DNA in the cells. Evaluation of the number of labeled cellsby phase-contrast microscopy demonstrated that serum withdrawalcaused a significant (P < .05) increase in the number of apoptoticevents (fig. 5). This increase was further potentiated 213% bythe addition of 150 mM ethanol. Ethanol treatment in the presenceof 15% serum did not alter the frequency of apoptotic events.This enhancement by ethanol of apoptosis induced by serum withdrawalwas observed whether the data were normalized to total cellularprotein (fig. 5) or total cellular DNA (data not shown).

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Fig. 5. Ethanol increases in situ DNA fragmentation after serum withdrawal. After a 24-hr treatment with 150 mM ethanol in the presence or absence of 15% serum, in situ DNA fragmentation was determined by the TUNEL method. Data are expressed as number of apoptotic events/mg protein and are plotted as mean ± S.E.M. (*P < .05, N = 5).

Because necrosis also can cause DNA fragmentation and lead to TUNEL-stained cells (Yasuda et al., 1995; Grasl-Kraupp et al.,1995; Charriaut-Marlangue et al., 1995), the fragmented DNA fromthe 15,000 × g supernatant was electrophoresed on agarose gelsto determine whether the characteristic internucleosomal cleavageof the DNA into 180- to 200-bp fragments (i.e., DNA laddering)was present. Cells maintained in the absence of serum displayedthe ~200-bp DNA ladder (fig. 6a) which is suggestive of apoptosis(Evans and Cidlowski, 1995). Quantification of the DNA ladderingby summing the intensity of the DNA bands in each lane of thegel revealed that 150 mM ethanol significantly increased the ladderingpresent after serum withdrawal 142% (fig. 6b). This enhancementby ethanol of DNA laddering induced by serum withdrawal was seenwhether the data was normalized to total cellular protein (fig.6b) or total cellular DNA (data not shown). Also, DNA from cellstreated with 2 mM H₂O₂ did not exhibit any laddering (fig. 6a)indicating that this death was not apoptotic. Additional experimentswere carried out to confirm that DNA laddering also occurred with50 mM ethanol. For these studies, we used a phosphate-citrateDNA extraction method (Gong et al., 1994) which involves lesstissue handling than extraction with phenol/chloroform. Quantificationof the DNA laddering using this technique demonstrated that ethanolcaused a concentration-dependent potentiation of apoptosis. Alow ethanol concentration (50 mM) significantly potentiated DNAladdering 49% although a high ethanol concentration (150 mM) causeda 184% increase (fig. 7).

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Fig. 6. Ethanol treatment increases internucleosomal DNA cleavage after serum withdrawal. a, Cells were treated with 150 mM ethanol either for 24 hr in the presence or absence of 15% serum or for 30 min in the presence or absence of 2 mM H₂O₂. The DNA was then electrophoresed and visualized with ethidium bromide and UV trans-illumination. b, The extent of DNA laddering was determined by summing the intensity of the DNA bands in each lane of the gel. Data are expressed as arbitrary fluorescent units/mg protein and are plotted as mean ± S.E.M. (*P < .05, N = 6).

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Fig. 7. Ethanol potentiates apoptosis due to serum withdrawal. After a 24-hr treatment with 50 or 150 mM ethanol in the absence of serum, the extent of DNA laddering was determined by summing the intensity of the DNA bands in each lane of the gel. Data are expressed as arbitrary fluorescent units/mg protein and are plotted as mean ± S.E.M. (*P < .05, N = 6).

To determine whether the ethanol-mediated cell death at low serum concentrations was apoptotic, cells were treated with 150mM ethanol in the presence of 4% serum and the DNA in the 15,000× g supernatant subjected to agarose gel electrophoresis. A portionof the cells maintained in 4% serum were undergoing apoptosisas indicated by cleavage of DNA into ~200-bp fragments (fig. 8a).Quantification of the DNA laddering showed that ethanol significantlyincreased apoptosis 66% (fig. 8b). Bhave and Hoffman (1997) reportedthat ethanol increased apoptosis in cerebellar granule cells byinhibition of the trophic action of NMDA. Inclusion of 100 µMNMDA in the treatment conditions, however, did not alter PC12cell viability (data not shown).

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Fig. 8. Ethanol promotes apoptosis in cells maintained in the presence of 4% serum. a, After a 24-hr treatment with 150 mM ethanol in the presence of 4% serum, the DNA was electrophoresed and visualized with ethidium bromide and UV-transillumination. b, The extent of DNA laddering was determined by summing the intensity of the DNA bands in each lane of the gel. Data are expressed as arbitrary fluorescent units/mg protein and are plotted as mean ± S.E.M. (**P < .01, N = 6).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Neuronal survival requires the presence of neurotrophic factors. For example, during development a limiting supply of target-derivedneurotrophic factors appears to be responsible for the normalloss of many of the neurons (Oppenheim, 1991; Raff et al., 1993).Removal of neurotrophic factors by withdrawal of serum in vitrocauses cell death by apoptosis (see Deshmukh and Johnson, 1997).In our study the extent of PC 12 cell death induced by serum withdrawalwas increased by ethanol. The ethanol-induced potentiation ofcell death by serum deprivation does not appear to represent ageneralized response resulting from imposing multiple insultson the PC 12 cells. Rather, the effects of ethanol on cell viabilitydisplay specificity as inclusion of ethanol inhibited cell deathinduced by H₂O₂.

The enhancement of cell death by ethanol was concentration dependent and was observed with an ethanol concentration as lowas 50 mM. This ethanol concentration is comparable to or lessthan the blood alcohol level in neonatal rodents that inducesbehavioral deficits (Thomas et al., 1996), alters neurotransmitterlevels (Maier et al., 1996), retards brain growth (Maier et al.,1997) and causes loss of cerebellar Purkinje cells and granulecells (Napper and West, 1995; Goodlett et al., 1997). Human fetusesalso may be exposed to a comparable concentration of alcohol.In one study at a community hospital emergency room, women whoadmitted recent drinking had a mean blood alcohol level of 260± 13 mg/dl (i.e., $approx$ 56 mM), but showed little or no signs of intoxication(Urso et al., 1981). One mother whose child was diagnosed withthe FAS had a blood alcohol concentration of 345 mg/dl (i.e., $approx$ 81 mM) at the time of delivery (Church and Gerkin, 1988). Furthermore,much higher blood alcohol concentrations have been reported inwomen of child-bearing age (Hammond et al., 1973; Wells and Barnhill,1996) including one report of a 24-yr-old woman with a blood alcohollevel of 1510 mg/dl (i.e., $approx$ 328 mM) who was described as "... agitatedand slightly confused but alert, responsive to questioning, andoriented to person and place (though unclear as to time)" (Johnsonet al., 1982).

In addition to increasing the extent of cell death caused by serum withdrawal, ethanol also induced PC 12 cell death. Similarly,Chen and Sulik (1996) observed that a 48-hr exposure to ethanolresulted in a concentration-dependent decrease in the viabilityof mouse neural crest cells in culture. Conversely, Luo and Miller(1997) did not observe any affect of ethanol (400 mg/dl; $approx$ 87 mM)on cell death in three neuroblastoma cell lines. The effects ofethanol on cell viability, however, appear to involve a complexantagonistic interaction between the concentrations of ethanoland serum factors. Thus, no ethanol-induced death was observedin PC 12 cells with 150 mM ethanol in the presence of 15% serum,but when the serum levels were reduced to 4%, which maintainsthe cells without a loss of viability, 100 mM ethanol caused asignificant increase in cell death. Also as shown in figure 2,the amount of cell death induced by ethanol displayed a dramaticincrease as the serum levels were reduced to 1%. Others also havereported opposing actions of ethanol and trophic factors. Luoet al. (1997) reported that nerve growth factor and basic fibroblastgrowth factor, but not epidermal growth factor or insulin-likegrowth factor 1, diminished the ethanol-induced loss of 1-day-oldcerebellar granule cells in culture. Cui et al. (1997) found thatethanol blocked the protective effect of insulin-like growth factorI on the cytotoxic action of tumor necrosis factor in BALB/c3T3fibroblasts. Ethanol also blocked the proliferative effect ofvarious mitogenic growth factors on neuroblastoma cells (Luo andMiller, 1997).

The ethanol-induced enhancement of cell death by serum deprivation involves an increase in the extent of apoptosis. Inclusionof ethanol increased the amount of DNA fragmentation and the numberof TUNEL-stained cells after serum withdrawal. Furthermore, theextent of DNA laddering by serum deprivation was increased byethanol. Similarly, ethanol initiates cell death by inducing apoptosisas shown by the DNA laddering in cells exposed to ethanol in thepresence of 4% serum. An increase in DNA fragmentation and thenumber of TUNEL-stained cells was reported in hypothalamic cellcultures exposed to 200 mM ethanol (De et al., 1994). Additionof 100 mM ethanol also was reported to increase the amount ofTUNEL-stained cells in cultures of cerebellar granule cells exposedto a nondepolarizing concentration of KCl (Bhave and Hoffman,1997). This effect in the granule cells was secondary to an ethanol-inducedinhibition of the trophic action of NMDA (Bhave and Hoffman, 1997).A different mechanism, however, is responsible for the ethanol-inducedapoptotic death of the PC12 cells as inclusion of NMDA did notalter PC12 cell death. Ethanol also appears to induce apoptosisin vivo. Postnatal exposure of rats to ethanol was noted in apreliminary report to increase the number of TUNEL-stained cellsin various brain regions (Hamby-Mason et al., 1996). Similarly,Bannigan and Burke (1982) reported the appearance of pyknoticnuclei and other morphology evidence of apoptosis in the brainsof fetal mice that were exposed to ethanol.

The microencephaly observed in the FAS is due to a loss of neurons. Ethanol can reduce the number neurons by various mechanismsincluding an inhibition of proliferation (Miller, 1986, 1988;Pantazis et al., 1992; Kane et al., 1996) and an alteration inmigration (Miller, 1993). The above discussion indicates thatthe ethanol-induced neuronal loss in vivo also may involve anincrease in neuronal apoptosis. Compounding the ability of ethanolto elicit cell death by counteracting the effects of neurotrophicfactors are reports that ethanol reduces the levels of some neurotrophicfactors in vivo (Walker et al., 1992; Breese et al., 1993; MacLennanet al., 1995) although this has not been a consistent finding(Baek et al., 1994). Ethanol also has been reported to alter expressionof some neurotrophic factor receptors including decreasing theamount of the low affinity neurotrophin receptor, p75 (Luo etal., 1996; Luo and Miller, 1997; Dohrman et al., 1997). However,because p75 that is not bound by ligand induced cell death (Barrettand Georgiou, 1996), the ethanol-induced increase in apoptosisis not consistent with a reduction in p75 levels. The inductionof apoptosis by ethanol could involve the neurotrophin tyrosinekinase receptor, trkA, which promotes cell survival (Fagan etal., 1996), as this receptor was reported in some (Dohrman etal., 1997), but not all cases (Luo and Miller, 1997), to be decreasedby ethanol. Also, because ethanol inhibits tyrosine kinase activityof the insulin-like growth factor 1 receptor in C6 rat glioblastomacells and Balb/c 3T3 fibroblasts (Resnicoff et al., 1993, 1994),it is possible that a similar action on neurotrophin signalingcould be involved in the ethanol-induced increase in apoptosis.However, neither a reduction in trkA expression nor an inhibitionof receptor tyrosine kinase activity would appear to explain howethanol potentiates cell death caused by serum withdrawal.

	Acknowledgments

The technical assistance of Barbara Hughes is greatly appreciated.

	Footnotes

Accepted for publication May 12, 1998.

Received for publication December 26, 1997.

¹ This work was supported by United States Public Health Service Award AA 06207 and a Mark Diamond research Grant to J.O.

Send reprint requests to: Dr. Richard Rabin, Department of Pharmacology and Toxicology, 102 Farber Hall, School of Medicine and Biomedical Sciences, State University of New York at Buffalo, Buffalo, NY 14214-3000.

	Abbreviations

FAS, fetal alcohol syndrome; TdT, terminal deoxynucleotidyl transferase; TUNEL, terminal deoxynucleotidyl transferase dUTP nick-end labeling; HBSS, Hanks' balanced salt solution; DMEM, Dulbecco's minimal essential medium.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

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