Palmitate-induced apoptosis in neonatal cardiomyocytes is not dependent on the generation of ROS

doi:10.1152/ajpheart.00726.2001

Palmitate-induced apoptosis in neonatal cardiomyocytes is not dependent on the generation of ROS

Diane L. M. Hickson-Bick, Genevieve C. Sparagna, L. Maximilian Buja, and Jeanie B. McMillin

Department of Pathology and Laboratory Medicine, University of Texas Medical School, Houston, Texas 77030

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

The saturated fatty acid palmitate induces apoptosis in neonatal rat cardiomyocytes. This apoptosis is associated with earlymitochondrial release of cytochrome c and a subsequent loss ofmitochondrial membrane potential. Recent reports implicate a rolefor reactive oxygen species (ROS) in palmitate-induced apoptosis.We studied the role of ROS in palmitate-induced apoptosis in theneonatal rat cardiomyocyte and report no evidence of ROS involvement.ROS production, nitric oxide production, and nuclear factor- $kappa$ Bactivation were not increased above those observed using the nonapoptoticfatty acid oleate. Indeed, the production of ROS was significantlyhigher in cells treated with oleate. Furthermore, the presenceof antioxidants and ROS scavengers did not attenuate the inductionof apoptosis by palmitate. Variations in the fatty acid-to-albuminratio from 2:1 to 7:1 had no effect on the absence of ROS productionor on the extent of apoptosis. No evidence was found for an increasein oxidative protein modification in palmitate-treated cells.Our results lead us to conclude that oxidative stress does notplay a role in palmitate-inducedapoptosis.

antioxidants; nitric oxide; mitochondria; nuclear factor- $kappa$ B

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

RECENT STUDIES HAVE SHOWN that the saturated long- chain fatty acid (LCFA) palmitate induces apoptosis in many cell typesincluding cardiomyocytes (4), hematopoetic cells (19), pancreatic $beta$ -cells (23), and astrocytes (2). The intracellular accumulationof LCFAs in nonadipose tissues is cytotoxic and associated withcellular dysfunction and cell death. In the Zucker diabetic fattyrat, accumulation of LCFA in the pancreatic $beta$ -cell leads to apoptotic $beta$ -cell death (23) and diabetes, whereas in the heart, cardiomyocytelipid accumulation is associated with cardiomyopathy and increasedcardiomyocyte apoptosis (32). In humans, diabetic cardiomyopathyis associated with increased myocardial lipid deposition, whichmay contribute to the clinical manifestations of this disease(21). Chronic intracellular accumulation of LCFA is thereforeassociated with many pathophysiological states. The mechanismsby which excess LCFA accumulations induce cell damage and celldeath are not completelydelineated.

Cardiomyocyte apoptosis has been implicated in myocardial ischemia and reperfusion injury, pathological conditions also associatedwith elevations in myocardial LCFA. Several studies have implicatedthe production of reactive oxygen species (ROS) in ischemia-reperfusioninjury (for a review, see Ref. 13). It remains to be determinedwhether the local increase in fatty acids contributes to the apoptoticcell death observed in this acutesituation.

Mitochondrial $beta$ -oxidation of fatty acids is the major source of energy for the heart. Mitochondria are also central to stress-inducedprogrammed cell death. In addition, in nonphagocytic cells, theseorganelles are the principal site of ROS production, via the electrontransport chain. Increased ROS production has been associatedwith the induction of apoptotic cell death in several cell types(for a review, see Ref. 10). Furthermore, exposure of neonatalcardiomyocytes to hydrogen peroxide or superoxide anion (O)induces apoptosis (30). Whether apoptosis induced by LCFAs isassociated with an increased production of ROS has clinical andpharmacological implications both in the acute treatment of ischemia-reperfusioninjury or in chronic situations associated with long-term exposureto high circulating fatty acidlevels.

We have previously shown that palmitate causes apoptosis in rat neonatal cardiac myocytes manifested by cytochrome c release,mitochondrial membrane potential loss, mitochondrial swelling,inhibition of carnitine palmitoyltransferase I- $beta$ , inhibition ofcomplex III, caspase-3-like activation, poly(ADP-ribose) polymerase(PARP) cleavage, and DNA laddering (8, 26). In this study,we examined the role of ROS in palmitate-induced apoptosis byemploying several techniques including ROS-sensitive fluorescentdyes, antioxidants, nitric oxide (NO) measurement, nuclear factor(NF)- $kappa$ B translocation, and protein carbonylation to detect evidenceof oxidative stress during palmitate-inducedapoptosis.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Primary cell culture. Neonatal rat cardiac myocytes were prepared according to McMillin et al. (16) using 1- to 2-day-old Sprague-Dawley rat pups.Myocytes were plated at 2 × 10⁶ cells/60-mm dish or on glass coverslips for microscope studiesand maintained for 60 h in DMEM containing 0.3 g/l glutamine,4.5 g/l glucose, and 10% calf serum. The medium was replaced with0.5 mM fatty acid (palmitic or oleic acid) bound to BSA in DMEMin the absence of serum. Fatty acid bound to BSA in the molarratio of 2:1 or 7:1 was prepared using the method of Goldsteinet al. (6), dialyzed against DMEM, and filter sterilized. Thefinal concentration of fatty acid in the stock solutions was measuredusing a semimicro analysis kit (Wako Chemicals; Richmond, VA).Neonatal rat fibroblasts were isolated by removing the fibroblastlayer from the Percoll gradient. All experiments with fibroblastswere done with cells passaged two to threetimes.

Determination of free fatty acid concentrations. Unbound fatty acids were measured using the acrylodated intestinal fatty acid-binding (ADIFAB) protein (Molecular Probes;Eugene, OR) method developed by Richieri (20). The concentrationof unbound fatty acids was calculated using the ratio of fluorescenceintensities of bound to unbound ADIFAB indicator at 505 and 432nm, respectively, using calculations and constants outlined onthe product datasheet.

Caspase-3-like activity. Caspase-3-like activity was measured by following the cleavage of the fluorescent substrate, Ac-Asp-Glu-Val-Asp-7-amido-4-methylcoumarin (Ac-DEVD-AMC; Calbiochem; San Diego, CA), as describedpreviously (8).

Microscopy for ROS generation. Oxidant generation studies were carried out on glass coverslips. The cells were incubated for 3 or 19 h in fatty acid-containingmedium; 5 µM (final concentration) of either the peroxide-sensitivefluorescent dye 2',7'-dichlorodihydrofluorescein diacetate (DCFH-DA),or the superoxide-sensitive dye dihydroethidium (DHE) (both fromMolecular Probes) was then added in DMSO. The medium was removedafter 1 h at 37°C, and the cells were washed and placed in HEPES-DMEMwithout serum. Intracellular fluorescence was monitored usinga temperature-regulated (37°C) Wallach/Olympus America Concordereal-time fluorescence imaging spectrophotometer and an OlympusIX70 inverted fluorescence microscope with a ×40 objective. Imageacquisition was with a fast-scan 12-bit charge-coupled devicecamera. Signal-based averaging was used to quantitate the fluorescencesignal from five to six fields of cells. Control cells were treatedwith 6 mM hydrogen peroxide for 1 h before the addition of thefluorescentdye.

Protein oxidation. The changes in oxidatively modified protein were measured using the Oxyblot protein oxidation detection kit (Intergen) andSDS-PAGE. The hydrogen peroxide control was obtained by incubationof cells with 6 mM H₂O₂ for 1h.

NO measurement. Total nitrate plus nitrite was measured using a colorimetric assay kit (Cayman; Ann Arbor, MI) based on the Griess reaction.Where noted, 0.5 mM N^G-monomethyl-L-arginine (L-NMMA) was added along with the fattyacid to inhibit NOformation.

Electrophoretic mobility shift assays. Nuclear extracts from primary rat neonatal cardiac myocytes were prepared as previously described (17). Double-strandedDNA probes containing the sequences for the NF- $kappa$ B-binding region(CTAGCAGTTGAGGGGACTTTCCCAGGCG) or sequence-specific mutated strands(CTAGCAGTTGAGGGttCTgTtCCAGGCG) were synthesized by Operon Technologies(Alameda, CA). Electrophoretic mobility shift assay reaction mixturesincluded 6 µg nuclear extract, 25 mM HEPES, 100 mM KCl, 0.1% NonidetP-40 (vol/vol), 1 mM dithiothreitol, 5% glycerol, and 50 ng PolydIdCas a nonspecific competitor in a 20-µl reaction volume. Afterincubation for 10 min at room temperature, 0.3 ng of radiolabeledprobe was added, and the reaction was incubated for 20 min. Whenincluded, an antibody against the p65 subunit of NF- $kappa$ B (SantaCruz Biotechnology; Santa Cruz, CA) or 100-fold molar excess ofcold probe was added during the first incubation. Protein-DNAcomplexes were separated on a 4% nondenaturing polyacrylamidegel at 25°C.

Statistics. The significance of the changes reported was determined using Student's t-test for nonpaired variates measured against thecontrol experiments using oleate. Data are presented as means±SE.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

ROS production by myocytes. The membrane-permeable dye DCFH-DA enters cardiomyocytes and produces a fluorescent signal after intracellular oxidation byROS such as hydrogen peroxide and the hydroxyl radical (29).Neonatal cardiomyocytes were incubated in palmitate or the controlfatty acid oleate for 4 or 20 h. We have previously shown thatexposure of these cells to palmitate for 4 h is sufficient toinduce mitochondrial cytochrome c release, whereas after 20 h,palmitate causes caspase-3-like activation, increased ceramideproduction, and DNA laddering (8, 26). With the use of videomicroscopy of live cells and examination of multiple fields ofcells, we were unable to detect any increase in fluorescence inpalmitate-treated cells over control oleate-treated cells at eithertime. Addition of hydrogen peroxide to these cells elicited anintense signal (Fig. 1).

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Fig. 1. Hydrogen peroxide and hydroxyl radical production by neonatal cardiomyocytes. Neonatal cardiomyocytes were incubated with dichlorodihydrofluorescein-diacetate (DCFH-DA) and treated with no fatty acid (FA; A), no FA plus 6 mM H₂O₂ for 1 h (B), oleate for 4 h (C) or palmitate for 4 h (D), or oleate for 20 h (E) or palmitate for 20 h (F). Images were acquired as described in METHODS. Magnification is ×400.

DHE also freely enters myocytes and is oxidized by ROS, particularly superoxide, to yield fluorescent ethidium (1, 29).Ethidium can pass into the nucleus, and subsequent binding ofethidium to DNA results in an amplified fluorescent signal. Incubationof cardiomyocytes with palmitate did not lead to an increasedoxidation of DHE. After both 4 and 20 h in the nonapoptotic fattyacid oleate, the DHE fluorescence was significantly higher thanin the palmitate-treated cells (Fig. 2). Because under physiologicalconditions an estimated 2-5% of O₂ utilized by mitochondria isreduced by single electron transfer by electrons that escape fromthe electron transport chain (27, 28), this increased productionof ROS by oleate-treated cells may be attributed to the increasedlevel of substrate $beta$ -oxidation over palmitate-treated cells (8).Inhibition of mitochondrial electron transport at complex I withrotenone or complex III with antimycin A resulted in increasedsuperoxide formation (Fig. 2). The fluorescent signals for cellstreated with antimycin A and rotenone were essentially saturatedunder the conditions employed, preventing a quantitative comparisonbetween these cells and the cells incubated in fatty acids.

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Fig. 2. Superoxide production in cardiomyocytes. Neonatal cardiomyocytes were treated with BSA (no FA), oleate, or palmitate for 4 h (solid bars) or 20 h (open bars). Dihydroethidium (DHE) was added for the last hour of incubation (see METHODS). The average nuclear fluorescence intensity was measured by signal averaging of the nuclear region. Control cells were maintained in serum-containing media and then treated for 1 h with antimycin A (anti A) or rotenone. Error bars represent means ± SE; n = 15-20. **Significantly different from oleate (4 h), P < 0.001; *significantly different from oleate (20 h), P < 0.001.

Because we were unable to detect any increase in ROS production associated with palmitate-induced apoptosis in neonatal myocytesby fluorescent video microscopy, we studied the effect of variousantioxidants and ROS scavengers on palmitate-induced apoptosis,as assessed by the activation of caspase-3-like proteins (Table1). Incubation of cells in the presence of palmitate and 4,5-dihydroxy-1,3-benzenedisulphonic acid (DBDA, Tiron), a cell-permeable nonenzymaticsuperoxide scavenger, or 5-aminosalicylic acid (5-ASA), a powerfulscavenger of hydroxyl radicals, did not prevent activation ofcaspase-3-like proteins. Pyrrolidine dithiocarbamate (PDTC), afree radical scavenger and metal chelator, also did not reducecaspase-3-like activation. Trolox (water-soluble vitamin E), ascavenger of lipid peroxyl radicals, was not effective in reducingcaspase-3-like activation by palmitate. Glutathione plays a centralrole in cellular antioxidant defense, and its loss may rendercells more prone to oxidative stress. Cardiomyocytes were thereforetreated with N-acetyl cysteine (NAC), a precursor compound forglutathione formation and previously shown to increase the glutathionecontent of cardiomyocytes (9). NAC was also unable to attenuatepalmitate-induced apoptosis in these cells (Table 1).

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Table 1. Caspase-3-like DEVDase activities with FA plus various antioxidants

Effect of levels of unbound fatty acids and cell type on ROS production. Other investigators have reported that in Chinese hamster ovary (CHO) cells, palmitate induces the formation of ROS (14).Because these results do not agree with our observations in cardiomyocytes,we hypothesized that these differences were a result of differentfatty acid-to-BSA ratios employed or, alternatively, cell type-specificdifferences. These authors used a fatty acid-to-BSA ratio of 8:1,as opposed to the physiological ratio of 2:1 that we employed.We predicted that their preparations would contain a higher concentrationof unbound fatty acid, which could be deleterious to the cell.We measured spectrofluorimetrically, using the ADIFAB protein,the unbound fatty acid in fatty acid bound to BSA at a ratio of7:1 and 2:1 (Fig. 3). Increasing the fatty acid-to-BSA ratio from2:1 to 7:1 resulted in a nearly sixfold increase in unbound fattyacid (66.7 ± 26.4 vs. 381.0 ± 63.6 nM). However, varying the fattyacid-to-BSA ratio did not increase the DCFH-DA fluorescence incardiomyocytes (Fig. 4), indicating that an increased level ofmedia free fatty acids does not lead to increased ROS production.Similarly, we were unable to observe any increases in fluorescencein rat fibroblasts (Fig. 4) or CHO cells (data not shown) afterincubation with either 2:1 or 7:1 palmitate-to-BSA ratios. Thissuggests that the lack of a ROS response is not cell type specificor restricted to cells with an increased dependency of fatty acidmetabolism over glucose metabolism. It has been documented thatfibroblasts are subject to apoptosis induction during serum deprivation(12). An increased level of ROS production in fibroblasts maintainedin serum-free media without fatty acid supplementation (Fig. 4B)indicates that apoptosis induced by serum deprivation may involveROS synthesis.

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Fig. 3. A: representative fluorescence spectra of FA-BSA mixtures at different ratios of FA to BSA using the acrylodated intestinal fatty acid-binding (ADIFAB) protein technique. B: calculated levels of unbound FA ([FFA]) in FA-BSA mixtures of different molar ratios. See METHODS for details. Error bars represent means ± SE; n = 4.

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Fig. 4. Hydrogen peroxide and hydroxyl radical production by fibroblasts. Fibroblasts were incubated with DCFH-DA for 1 h after treatment with 6 mM H₂O₂ for 1 h (A), serum-free medium for 20 h (B), oleate for 4 h (C), palmitate for 4 h (D), oleate for 20 h (E), or palmitate for 20 h (F). Magnification is ×400. Images were collected as described in METHODS. A signal-averaged quantification of the dichlorofluorescein fluorescence intensities for cardiomyocytes and fibroblasts is given for comparison.

NO production and palmitate-induced apoptosis. NO production by inducible NO synthase (iNOS) has been implicated in ischemia-reperfusion injury and apoptosis of cardiomyocytes(31). Superoxide generated by mitochondria can interact withNO to form peroxynitrite (ONOO), which can induce mitochondrial dysfunction and apoptosis andexacerbate the apoptotic effect of superoxide alone. We examinedthe role of NO production in palmitate-induced apoptosis of neonatalcardiomyocytes by measuring the total production of nitrite plusnitrate over the course of a 20-h incubation in fatty acid-BSA(2:1) or serum-free medium alone (Fig. 5). NO production by palmitate-treatedcells was significantly lower than that of oleate-treated cellsfor periods up to 12 h, at which time no difference was seen.Addition of the cell-permeable iNOS inhibitor L-NMMA reduced theproduction of nitrate plus nitrite in both oleate- and palmitate-treatedcells during a 16-h incubation (Fig. 6A) but failed to reducethe induction of caspase-3-like activity at this time (Fig. 6B).

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Fig. 5. Nitric oxide (NO) production. Neonatal cardiomyoctes were treated with oleate (open squares), palmitate (solid circles), or serum-free medium (shaded triangles) for 0-20 h, and total nitrate plus nitrite levels were quantified. Error bars represent means ± SE; n = 3-6.

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Fig. 6. NO inhibition does not affect caspase-3-like activity. Cardiomyoctes were treated with either BSA (no FA), oleate, or palmitate (Palm) for 16 h in the presence (open bars) or absence (solid bars) of N-monomethyl-L-arginine (L-NMMA). Total nitrate plus nitrite (A) and caspase-3-like activity (B) were quantified from the same samples. Error bars represent means ± SE; n = 3.

NF- $kappa$ B binding activity and effect of superoxide dismutase inhibition on palmitate-induced apoptosis. Binding activity of NF- $kappa$ B, a redox-regulated transcription factor, was found to be very low in the nucleus of cardiomyocytesmaintained in serum alone. Addition of 0.5 mM fatty acid-1.6%BSA increased the translocation of NF- $kappa$ B from the cytosol to thenucleus (Fig. 7A). No significant difference was observed betweenNF- $kappa$ B translocation in oleate- or palmitate-incubated cells. Toconfirm the specificity of the NF- $kappa$ B binding activity, we performedsupershift assays with a polyclonal antibody to the NF- $kappa$ B p65subunit (Fig. 7B). The binding of NF- $kappa$ B was also competed with100-fold excess of unlabeled probe but not with mutant probe (Fig.7B). Quantification and averaging of the palmitate-to-oleate signalratio for several gels confirmed that there was no significanttime-dependent difference in NF- $kappa$ B binding between cells maintainedin these two fatty acids (Fig. 7C). Thus while incubation of cardiomyocyteswith fatty acids increases NF- $kappa$ B binding, this signaling mechanismis not involved in palmitate induction of apoptosis.

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Fig. 7. Nuclear binding activity of nuclear factor (NF)- $kappa$ B. A: cardiomyocytes were treated for up to 20 h with oleate or palmitate, and electophoretic mobility shift assays (EMSAs) were run to quantify NF- $kappa$ B binding. A band indicating nonspecific (NS) binding is included for gel loading comparisons. B: nuclear extract from a representative 12-h palmitate-treated sample was run with a 100-fold excess of unlabeled wild-type NF- $kappa$ B oligomers (100× Wt), 100-fold excess of unlabeled mutant oligomers (100× Mt), or an antibody to the p65 subunit of NF- $kappa$ B (Ab ss) to produce a supershift shown by the arrow (SS). C: numerical comparison of the palmitate-to-oleate signal ratio for NF- $kappa$ B binding. The NF- $kappa$ B signal ratio for palmitate to oleate at each time was calculated from the means ± SE for several gels (n = 3).

Inhibition of superoxide dismutase. Our data demonstrate that cardiomyocytes do not increase production of ROS when incubated with palmitate. We examined whetherincreasing the level of ROS production in these cells increasedthe apoptotic response of these cells as assessed by the activationof caspase-3-like activity. Addition of diethyldithiocarbamicacid (DDC), an inhibitor of cytosolic (Cu, Zn) superoxide dismutase,to cells incubated in palmitate for 16 h causes an increase inthe nuclear translocation of NF- $kappa$ B (Fig. 8). DDC inhibition ofsuperoxide dismutase has been shown to increase superoxide generationin neonatal rat cardiac myocytes (24), and we demonstrated thatthe caspase-3-like activity of both oleate- and palmitate-incubatedcells increased in the presence of increasing concentrations ofDDC (Table 2). However, the caspase-3-like activity of oleate-treatedcells in the presence of DDC, even at a concentration (100 µM)previously shown to induce apoptosis (24), never attained thelevels achieved by palmitate incubation alone (without DDC).

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Fig. 8. NF- $kappa$ B with various diethyldithiocarbamic acid (DDC) concentrations. Cardiomyocytes were treated with palmitate for 16 h in the presence of various concentrations of DDC, and the resulting nuclear extracts were used for EMSA (inset). Intensities of the NF-kB bands were quantified by signal averaging.

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Table 2. Caspase-3-like activity of cardiomyocytes incubated for 20 h in the presence of FA and varying concentrations of DDC

Protein oxidation and palmitate-induced apoptosis. Oxidative stress-induced injury can involve the selective modification of intracellular proteins. We measured the levels ofoxidatively modified proteins using Oxyblot analysis, which detectsprotein carbonyl formation. We were unable to detect changes inprotein carbonylation in cardiomyocytes incubated with eitheroleate or palmitate for 4 or 20 h (Fig. 9) compared with cellsincubated in serum-free medium alone. A change in the proteincarbonylation pattern was observed when cells were incubated inhydrogen peroxide for 1 h.

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Fig. 9. Oxyblot to measure oxidatively modified proteins. Cardiomyocytes were treated for 4 or 20 h with serum-free medium (SF), oleate, or palmitate. As a control, they were also treated with 6 mM H₂O₂ for 1 h. Bands, oxidatively modified proteins; arrows, areas showing bands modified in H₂O₂-treated cells.

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Palmitate, but not oleate, induces apoptosis in neonatal cardiac myocytes. We have previously shown that this apoptosis ischaracterized by an early mitochondrial release of cytochromec and a loss of mitochondrial membrane potential (26). Laterevents include an increase in ceramide synthesis, inhibition ofmitochondrial electron transport complex III, activation of caspase-3-likeenzymes, and DNA laddering (8, 26). Increased productionof ROS have been implicated in stress induction of apoptosis incardiac myocytes and reported to be involved in palmitate-inducedapoptosis of CHO cells (14).

Mitochondrial oxidative phosphorylation represents a process by which the oxidation and reduction of a multicomponent complex,the electron transport chain, reduces O₂ to H₂O and the changein free energy is conserved by the phosphorylation of ADP to ATP.The terminal step is the transfer of four electrons to O₂ by cytochromec oxidase to form H₂O. However, partially reduced forms of O₂may be formed during this process, forming superoxide and hydrogenperoxide by one and two electron transfers, respectively. Superoxidedismutase efficiently and rapidly dismutes superoxide to the lessreactive H₂O_2. In the presence of transition metals, H₂O₂ cangive rise to the more reactive hydroxyl radical (OH·) by Fentonchemistry. Superoxide may also be converted to the very reactiveperoxynitrite in the presence ofNO.

We employed a variety of techniques to measure the production of ROS species. We could not detect an increased productionof ROS by cells incubated in palmitate at 4 h, a time when mitochondrialcytochrome c release can be measured, or 20 h, when caspase-3-likeactivity and ceramide accumulation is maximal. Similarly, thepresence of ROS scavengers (DBDA, 5-ASA, and PDTC) during palmitateincubation was unable to prevent apoptosis as measured by caspase-3-likeactivity. No increase in NO synthesis in palmitate- over oleate-incubatedmyocytes was observed. Increasing myocyte ROS by the inhibitionof superoxide dismutase with DCC increases the level of caspase-3-likeactivation and apoptosis, indicating that ROS can induce apoptosisin these cells but that this is distinct from, and additive to,the effect ofpalmitate.

Putative downstream targets of ROS signaling are alterations in the intracellular redox state and the oxidative modificationof proteins. The intracellular redox state is controlled primarilyby the buffering capacity of the intracellular thiols glutathioneand thioredoxin. These thiols reduce oxidative stress by reducingH₂O₂ levels. Increasing the thiol buffering capacity of myocyteswith the glutathione precursor NAC (9) did not prevent palmitate-inducedapoptosis. We were also unable to detect any oxidative modificationofproteins.

ROS have been implicated in signal transduction pathways leading to a modulation of the DNA-binding activities of the transcriptionfactor NF- $kappa$ B (15), implying a role for alterations in gene transcriptionas a response to oxidative stress. We report a significant increasein the DNA-binding activity of NF- $kappa$ B in cardiomyocytes incubatedin the presence of fatty acids. However, no significant differenceswere observed between the NF- $kappa$ B activities of cells incubatedin palmitate or oleate, implying no role for this signaling pathwayin palmitate-inducedapoptosis.

We observed that incubation of neonatal cardiac myocytes with fatty acids may lead to measurable ROS production. This ROSproduction is not, however, associated with palmitate-inducedapoptosis because higher levels of production are observed inoleate-incubated cells. Oleate-incubated cells have elevated ratesof $beta$ -oxidation compared with palmitate-incubated cells (8),providing increased electron movement through the electron transportchain and oxidative phosphorylation. Some small percentage ofelectrons escape from the electron transport chain, potentiallyat complex I and complex III. These electrons are capable of formingROS, explaining the higher measurable levels of ROS in oleate-incubatednonapoptoticcells.

Free fatty acids act as uncouplers of mitochondrial electron transport by means that are not fully defined but are probablyrelated to uncoupling proteins (UCPs) present within the cell(for a review, see Ref. 25). The heart has an abundant levelof these proteins, particularly UCP2 (5). It has been postulatedthat the mild uncoupling ability of fatty acids is sufficientto maintain the mitochondrial membrane potential below a thresholdlevel and prevent ROS formation by the respiratory chain (11).Differences in the uncoupling ability of oleate and palmitatehave also been reported in model mitochondrial vesicles (22).Uncoupling by fatty acids decreases production of ROS and oxidativestress. Generation of ROS from the electron transport chain requiresa high mitochondrial membrane potential (7). We previouslyreported that palmitate-induced apoptosis in the neonatal cardiomyocyteis associated with a decrease in the mitochondrial membrance potential,also decreasing the ability of the mitochondria to produceROS.

Our results are in direct opposition to those reported for palmitate-induced apoptosis in CHO cells measured using similarfluorescent dyes. These differences cannot be explained by thedifferent ratios of fatty acid to BSA employed. The pathologicallyhigh 8:1 fatty acid-to-BSA level employed by Listenberger et al.(14) is associated with an increased level of unbound fattyacids. However, even under similar conditions (7:1 fatty acid-to-BSAratio), neither oleate nor palmitate demonstrated augmentationof the ROS production observed using a 2:1 fatty acid-to-BSA ratio.Our measurements were made on beating myocytes using real-timevideo fluorescence microscopy. Because this requires visualizationof fluorescence, it could lead to an overestimation, rather thanan underestimation, of ROS production. We (26) previously reportedthat palmitate-induced apoptosis is associated with a mitochondrialloss of cytochrome c. Cytochrome c is a potent catalyst of dichlorofluoresceinoxidation, leading to an increase in DCFH-DA oxidation despitea lowered rate of ROS production (3). Nonetheless, no evidenceof DCFH-DA oxidation could beobserved.

In conclusion, and contrary to other reports, we are unable to find any evidence of ROS involvement in palmitate-induced apoptosis.In considering the bioenergetics of ROS production by mitochondriaand the known biophysical properties of fatty acids, this resultis not unexpected. Recent studies from our laboratory have shownthat the mitochondrial release of cytochrome c is directly relatedto a decrease in mitochondrial cardiolipin and associated alterationsin phospholipid metabolism (18). Although ROS production playsan important role in ischemia-reperfusion injury and apoptosisinduced by other means, palmitate-induced apoptosis involves otherpathways that lead to perturbations in cellularmetabolism.

	FOOTNOTES

Address for reprint requests and other correspondence: D. Hickson-Bick, Univ. of Texas Health Science Center, Dept. of Pathologyand Laboratory Medicine, 6431 Fannin, Houston, TX 77030 (E-mail:Diane.L.Bick{at}uth.tmc.edu).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

10.1152/ajpheart.00726.2001

Received 14 August 2001; accepted in final form 5 October 2001.

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