Extracellular Signal-Regulated Kinases Are Involved in the Antiapoptotic Effect of Endothelin-1

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Vol. 293, Issue 2, 514-521, May 2000

Extracellular Signal-Regulated Kinases Are Involved in the Antiapoptotic Effect of Endothelin-1

Jinshyun R. Wu-Wong, William J. Chiou and Jiahong Wang

Pharmaceutical Products Division, Abbott Laboratories, Abbott Park, Illinois

	Abstract

Top Abstract Introduction Experimental Procedures Results Discussion References

An imbalance between proliferation and apoptosis is an important causal factor for disorders involving abnormal cell accumulation.The role and mechanism of how G protein-coupled receptors arelinked to apoptosis are poorly understood. Endothelin-1 (ET-1),a 21-amino acid peptide that binds to G protein-coupled receptorswith mitogenic and vasoconstricting activities, suppressed apoptosisof human prostatic smooth muscle cells induced by paclitaxel treatmentor serum withdrawal. Serum withdrawal or paclitaxel (1-10 µM)treatment for 48 h resulted in DNA fragmentation, a characteristicof apoptosis. The addition of ET-1 attenuated DNA fragmentation.The attenuating effect of ET-1 on DNA fragmentation was not affectedby wortmannin, bisindolylmaleimide I, tyrphostin AG490, or AG1478.However, PD98059, an inhibitor for the extracellular signal-regulatedkinase (ERK) kinase, induced apoptosis, potentiated the effectof serum withdrawal on inducing apoptosis, and blocked the antiapoptoticeffect of ET-1. The ERK1/2 activity in these cells decreased rapidlyafter paclitaxel treatment or serum withdrawal, but was maintainedat a 2-fold higher level in the presence of ET-1 for at least4 h. These results suggest that the ERK1/2 pathway is activatedby ET-1, and blocking this pathway abolishes the antiapoptoticeffect of ET-1.

	Introduction

Top Abstract Introduction Experimental Procedures Results Discussion References

Apoptosis, or programmed cell death, has been shown to be involved in many critical biologic events including embryonic developmentand maintenance of normal tissue functions. In addition, apoptosisis involved in various pathologic situations. Disorders involvingaberrant cell accumulation such as tumor, restenosis, and benignprostatic hyperplasia are usually the result of an imbalance betweenproliferation and apoptosis. Apoptosis is characterized by changesin the cell membrane structure, internucleosomal fragmentationof genomic DNA, chromatin condensation, and nuclear disintegration.Mitogens and survival factors have been shown to play importantroles in regulating cell proliferation and apoptosis. These factors,by first binding to membrane receptors, trigger phosphorylationof various molecular targets, which then activate the downstreamsignaling cascades, leading to changes in cell death-regulatingproteins, and resulting in the life or the death of a cell. Thesignaling pathways involved in the apoptosis-preventive effectsof growth factor receptors with intrinsic tyrosine kinase activitiesare gradually becoming known, such as activation of phosphatidylinositol3-kinase and extracellular signal-regulated kinases 1/2 (ERK1/2)by insulin-like growth factor-1 in PC12 cells (Párrizas et al.,1997), and stimulation of nuclear factor $kappa$ B by insulin in Chinesehamster ovary cells overexpressing insulin receptors (Bertrandet al., 1998). As a comparison, the roles and the underlying mechanismsof G protein-coupled receptors (GPCRs) in apoptosis remain muchlessunderstood.

Endothelin (ET) is a peptide with 21-amino acid residues (Yanagisawa et al., 1988). Three distinct members of the ET family,ET-1, ET-2, and ET-3, have been identified in humans through cloning(Inoue et al., 1989). The effects of ETs on mammalian organs andcells are initiated by their binding to GPCRs found in varioustissues and cells (Sokolovsky, 1992). Two types of mammalian ETreceptors, ET_A and ET_B, have been characterized and purified (Wadaet al., 1990; Kozuka et al., 1991), and their cDNA have been cloned(Arai et al., 1990; Sakurai et al., 1990). ET_A receptors are selectivefor ET-1 and ET-2, whereas ET_B receptors bind ET-1, ET-2, andET-3 with equal affinity. ET-1 is known to activate protein kinaseC (PKC), epidermal growth factor (EGF) receptor kinase, and theERK pathway (Douglas and Ohlstein, 1997), and is a mitogen forvarious cells, including smooth muscle cells (Wu-Wong et al.,1994; Yoshizumi et al., 1998) and cancer cells (Bagnato et al.,1995; Pagotto et al., 1995; Nelson et al., 1997). ET-1 is thoughtto play important roles in various pathophysiologic conditionsincluding cell growthdisorders.

We and others have shown previously that ET-1 protects smooth muscle cells and endothelial cells from serum withdrawal- orpaclitaxel-induced apoptosis (Shichiri et al., 1997, 1998; Wu-Wonget al., 1997). However, the signaling pathways leading to theantiapoptotic effect of ET-1 are still generally unknown. Thegoal of this study is to investigate the possible mechanism involvedin the antiapoptotic effects of ET-1 in primary culture humanprostatic smooth muscle cells (HPrSMC). Our results show thatthe ERK1/2 pathway is activated by ET-1, and that blocking thispathway abolishes the antiapoptotic effect of ET-1. The resultssuggest that ERK1/2 may play a role as the downstream mediatorfor the antiapoptotic effect of ET-1.

	Experimental Procedures

Top Abstract Introduction Experimental Procedures Results Discussion References

Materials. ET-1 was obtained from American Peptide Company (Sunnyvale, CA). Other reagents were of analyticalgrade.

Cell Culture. Human prostatic smooth muscle cells were obtained from Clonetics (San Diego, CA) and grown in SmGM medium containing 5% fetalbovine serum (FBS). Only cells with a passage number <9 are usedin this study. Cell viability was examined using the trypan blueexclusionmethod.

Apoptosis Detection by Enzyme-Linked Immunosorbent Assay (ELISA). Cells in 96-well plates were treated with test agents in the presence of paclitaxel or in serum-free medium (SFM) for 48 h(or as indicated) at 37°C. At the end of the incubation, cellswere lysed in 200 µl of lysis buffer (catalog no. 1544675; RocheMolecular Biochemicals, Indianapolis, IN). The cell lysates werecollected and centrifuged at 200g for 10 min. The samples wereassayed for apoptosis using an ELISA kit according to the manufacturer'sinstruction (catalog no. 1544675; Roche Molecular Biochemicals).The ELISA uses monoclonal antibodies directed against DNA andhistones in a quantitative sandwich enzyme-based format. The amountof histone-associated DNA fragments (mono- and oligonucleosomes)in the cell lysates was determined at A₄₀₅ in aspectrophotometer.

DNA Synthesis. Cells in 96-well plates were cultured in growth medium until at ~70% confluency. Cells then were cultured in 0.2 ml/well SFMfor 48 h and treated with FBS or ET-1 in the presence of 0.5 µCi/well[³H]thymidine for another 48 h. After the incubation, each wellwas washed with 0.2 ml of PBS, and then incubated with 0.2 mlof ice-cold 10% trichloroacetic acid for 30 min at 4°C. Each wellwas then washed again with 0.2 ml of 10% trichloroacetic acid.Materials not soluble in trichloroacetic acid were dissolved in0.1 N NaOH for scintillationcounting.

Immunocytostaining and Confocal Microscopy. Cells were grown in two-chamber slides in SmGM medium containing 5% FBS. Cells were then put into SFM for 48 h and then stimulatedwith or without ET-1 or 5% FBS for different periods of time.Afterward, cells were washed with PBS for 30 s, fixed with a fixingsolution (0.1% glutaldehyde, 2% formalin, 80 mM PIPES, 5 mM EGTA,1 mM MgCl₂, 0.5% Triton X-100) for 7 min, washed again with PBSfor 5 min, and placed in methanol at $-$ 20°C. The slides were transferredinto ice-cold acetone at $-$ 20°C for 7 min, rinsed with PBS forthree times, and incubated with PBS plus 10% donkey serum for30 min at room temperature. The slides were then incubated withan anti-phosphorylated ERK1/2 monoclonal antibody derived frommice (1000-fold dilution; New England Biolabs, Beverly, MA) inPBS with 2% donkey serum for 24 h at 4°C. After the incubation,slides were rinsed with PBS for three times and then incubatedwith Cy3-conjugated donkey anti-mouse IgG (100-fold dilution;Jackson ImmunoResearch Lab, West Grove, PA) for 30 min at 37°Cin a humidified chamber, followed by another three rinsing withPBS. The slides were mounted, and pictures were taken using aBio-Rad (Richmond, CA) MRC1000 confocal microscope linked to animageanalyzer.

Mitogen-Activated Protein Kinase (MAPK) Activity Assay. Cells were plated at a density of 5 × 10⁴ cells/ml in 6-cm dishes. After different treatments, cells were washed with PBS twiceand lysed in 0.3 ml of buffer A (10 mM Tris, pH 7.4, 150 mM NaCl,2 mM EGTA, 2 mM DTT, 1 mM sodium orthovanadate, 1 mM phenylmethylsulfonylfluoride, 10 µg/ml leupeptin, 10 µg/ml aprotinin, 2 µg/ml pepstatinA). Cells were homogenized using a microultrasonic cell disrupter(Kontes, Vineland, NJ) and then centrifuged at 42,000g for 20min. The supernatant was collected. Protein content was determinedby the Bio-Rad dye-binding protein assay. The MAPK activity wasdetermined using an assay kit (catalog no. RPNS84; Amersham PharmaciaBiotech, Piscataway, NJ) according to the manufacturer's instructions.Briefly, 15 µl of the cell lysate was mixed with 15 µl of a reactionmixture containing [ $gamma$ -³³P]ATP (1 µCi/reaction) and a synthetic peptide (NH₂-KRELVEPLTPAGEAPNQALLR-COOH)as the substrate for ERK1/2. The mixture was incubated at 30°Cfor 30 min. The reaction was terminated by adding 10 µl of a stopsolution. The sample (30 µl) was applied to a phosphocellulosemembrane. The membrane was washed extensively in 75 mM phosphoricacid and then in water. The radioactivity on the membrane wasdetermined by a liquid scintillationcounter.

To validate the specificity of the MAPK assay, two control experiments were conducted in which cellular extracts were preparedfrom cells that were serum-starved for 48 h, followed by treatmentwith or without ET-1 for 5 min. First, the cellular extract wasincubated with the peptide substrate in the assay mixture as describedabove and then analyzed by SDS/polyacrylamide gel electrophoresis(PAGE). The gel was sliced into 2-mm pieces for radioactivitydetermination. The radioactivity was detected only in slices correspondingto the position of the peptide at ~2500 kDa in samples treatedwith 10 nM ET-1 (data not shown). These results show that onlythe peptide substrate was specifically phosphorylated by ERK1/2in the MAPK assay. In the second experiment, the extract was fractionatedby an anion exchanger Mono-Q column. Fractions were assayed forthe MAPK activity and also analyzed in Western blot using antibodiesspecific for ERK1 and ERK2. For a detailed description of themethods on anion exchange chromatography, see our previous report(Wu-Wong and Opgenorth, 1998

). The results (data not shown) indicatethat in samples from cells treated with ET-1, the kinase activitycolocalized with the ERK1/2 proteins detected by Western blot.No activity was detected in fractions that did not stain positivefor ERK1/2. When the samples from cells without ET-1 treatmentwas fractionated, no activity was detected in anyfraction.

The specificity of this assay for ERK1/2 was confirmed further by the immunoprecipitation study describedbelow.

Immunoprecipitation. A mixture of 0.5 ml of lysis buffer (50 mM Tris-HCl, pH 7.5, 150 mM NaCl, 1% Nonidet P40, 0.5% sodium deoxycholate) with 100µl of a protein G-agarose bead slurry (~50%) and anti-ERK1/2 antibodies(5 µg/each) derived from rabbits (Santa Cruz Biotechnology, SantaCruz, CA) was incubated for 24 h at 4°C to form agarose-boundimmune complexes. Cells in 10-cm dishes were lysed with 1 ml oflysis buffer and then centrifuged at 25,000g for 20 min at 4°C.The supernatant (0.5 ml) was incubated with agarose beads containingthe preformed anti-ERK1/2 antibody-protein G complexes for 2 hat 4°C. The agarose beads were collected by centrifugation at12,000g for 20 s and washed twice with wash buffer (50 mM Tris-HCl,pH 7.5, 0.1% Nonidet P40, 0.05% sodium deoxycholate, 1 ml/sample/wash).To determine ERK1/2 activities, beads were resuspended in 60 µlof buffer A and assayed as describedabove.

SDS/PAGE and Western Blot Analysis. Samples (20 µl/sample) were resolved by SDS/PAGE using a 12% gel (Novex, San Diego, CA), and proteins were transferred electrophoreticallyto a polyvinylidene difluoride membrane (Immobilon-P, 0.45-µmpore size; Millipore, Burlington, MA) for Western blotting. Themembrane was blotted for 1 h at 25°C with nonfat dry milk (5%)in Tris-buffered saline/Tween 20 (TBST; 10 mM Tris, pH 8.0, 0.15M NaCl, 0.1% Tween 20), and then incubated with antiphosphorylatedERK1/2 antibodies derived from rabbit (Santa Cruz Biotechnology)in TBST for 1 h at 25°C. The membrane was washed with TBST andincubated with a horseradish peroxidase-labeled anti-rabbit antibodyfor 1 h at 25°C. The paper was then incubated with detection reagentcontaining luminol in an alkaline buffer. The specific bands werevisualized by exposing the paper to blue light-sensitive autoradiographyfilms.

	Results

Top Abstract Introduction Experimental Procedures Results Discussion References

Suppression of Apoptosis in HPrSMC by ET-1. Consistent with our previous findings (Wu-Wong et al., 1997), Fig. 1A shows that paclitaxel (1 µM), a tubulin-binding agent,induced apoptosis in HPrSMC, which was partially blocked by 10nM ET-1 (a 47% decrease). The incidence of apoptosis was assayedby an ELISA that measures mono- and oligonucleosomes in cell lysates.The presence of mono- and oligonucleosomes, an indication forDNA fragmentation, is one of the characteristics of cells undergoingapoptosis (Bonfoco et al., 1995).

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Fig. 1. Effect of ET-1 on apoptosis and proliferation. A, paclitaxel-induced apoptosis; cells in 96-well plates were fed with SmGM medium containing 5% FBS 24 h before the experiments. Cells were then treated with 1 µM paclitaxel in the presence or absence of 10 nM ET-1 for 48 h at 37°C. Apoptosis was measured by an ELISA that detects histone-associated DNA fragments. Each value represents mean ± S.D. of three determinations. B, serum withdrawal-induced apoptosis; cells cultured in 96-well plates were serum-starved in the presence or absence of ET-1 (concentrations as indicated) for 48 h at 37°C. Apoptosis was measured as in A. Each value represents mean ± S.D. of three determinations. C, DNA synthesis; cells in 96-well plates were incubated in SFM for 48 h and then treated with or without ET-1 or FBS (concentrations as indicated) for another 48 h in the presence of [³H]thymidine (0.5 µCi/well). Each value represents the mean ± S.D. of four determinations. The statistical significance was determined by the paired Student's t test.

Apoptosis also could be induced by depriving cells of serum. Figure 1B shows that the A₄₀₅ value for cells cultured in 5%FBS was 0.037 ± 0.006. On serum withdrawal for 48 h, the valuewas increased to 0.287 ± 0.023, suggesting that serum withdrawalinduced apoptosis in these cells. Figure 1B shows that ET-1 partiallyblocked apoptosis induced by serum deprivation. Although the blockadewas not 100%, ET-1 was very potent in suppressing apoptosis withan approximate EC₅₀ value of 0.1 nM. This effect is consistentwith the EC₅₀ values observed in other ET-1-mediated biologicresponses (Wu-Wong et al., 1996

, 1999

As noted previously (Wu-Wong et al., 1997

), the A₄₀₅ values from experiment to experiment did vary, possibly because differentbatches of cells and different assay kits were used for differentexperiments.

Interestingly, although ET-1 protected these cells from apoptosis, ET-1 did not have a significant effect on stimulating DNAsynthesis, whereas 10% FBS stimulated DNA synthesis by >10-foldduring a 48-h incubation period (Fig. 1C).

These results suggest that ET-1 exhibits protective effects against apoptosis induced by either paclitaxel treatment or serumstarvation.

Effects of Kinase Inhibitors on Apoptosis. To investigate whether a protein kinase is involved in the antiapoptotic effect of ET-1, we took advantage of the availabilityof pharmacologic tools for kinases that were shown previouslyto be activated by ET-1.

Figure 2A shows that for cells cultured in growth medium continuously, bisindolylmaleimide (bisindo; an inhibitor for PKC)did not have a significant effect on inducing apoptosis. Also,bisindo did not potentiate or reduce the effect of serum withdrawalon inducing apoptosis. Figure 2C shows that when ET-1 (100 nM)was added in the absence of serum, the A₄₀₅ value decreased to30% of control, a 70% reduction in DNA fragmentation. In the presenceof 1 and 5 µM bisindo, the antiapoptotic effect of ET-1 was stillobserved, although slightly reduced. Similar results were obtainedfor tyrphostin AG1478, an inhibitor for the EGF receptor kinase,wortmannin, an inhibitor of PI3K, and AG490, a JAK-2 inhibitor.The results suggest that EGF receptor kinase, PKC, PI3K, and JAKmay not play an important role in the protective effect of ET-1against apoptosis induced by serum withdrawal.

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Fig. 2. Effect of kinase inhibitors on apoptosis. A and B, cells in 96-well plates were treated with various kinase inhibitors for 48 h in the presence or absence of 5% FBS. Wortmannin (Wort), 1 µM; bisindolylmaleimide (Bisindo), 5 µM; tyrphostin AG490, 5 µM; AG1478, 1 µM; genistein, 10 µg/ml; PD98059 (PD), 80 µM. C and D, cells in 96-well plates were cultured in SFM for 48 h in the presence or absence of various kinase inhibitors with or without 100 nM ET-1. Concentrations for inhibitors: as indicated or PD98059, 80 µM. Apoptosis was measured by an ELISA that detects histone-associated DNA fragments. Each value represents mean ± S.D. of four determinations. In all experiments, cells were fed with SmGM medium containing 5% FBS 24 h before the treatments. In C, each inhibitor was tested in an independent experiment. Data were first converted to percentage of control (no ET-1) and then compiled into C.

Figure 2, A and B, show that genistein, a general kinase inhibitor, and PD98059, an inhibitor for ERK kinase (MEK-1), exhibitedsignificant effects on apoptosis signaling. Both genistein andPD98059 induced apoptosis in these cells cultured in growth medium.In addition, both agents potentiated the effect of serum withdrawalon inducing apoptosis. Figure 2D shows that although ET-1 protectedcells from apoptosis induced by serum withdrawal, the antiapoptoticeffect of ET-1 was no longer observed in the presence of PD98059.These results show that PD98059 induces apoptosis and blocks theantiapoptotic effect of ET-1, suggesting that the ERK1/2 pathwaymay play an important role in the protective effect of ET-1 againstapoptosis induced by serumwithdrawal.

Activation of ERK1/2 by ET-1. We then examined the effect of ET-1 on ERK1/2 by various approaches. Figure 3A shows that both ET-1 (10 nM) and bFGF (10 ng/ml)induced the phosphorylation of ERK1/2. Very little phosphorylationof ERK1/2 was observed in control cells that were serum-starvedfor 48 h. In Fig. 3B, the ERK1/2 activity was determined usinga synthetic peptide (see Experimental Procedures) as the substrateafter ERK1/2 was immunoprecipitated by anti-ERK1/2 antibodies.The result shows that ET-1 at 10 nM stimulated the activity ofERK1/2 by 20-fold. As a comparison, bFGF at 10 ng/ml stimulatedthe activity of ERK1/2 by 13-fold. In Fig. 3C, the ERK1/2 activitywas determined in cellular extracts directly (without immunoprecipitationby anti-ERK1/2 antibodies) using the same assay. Similar to thatshown in Fig. 3B, ET-1 exhibited a profound effect on stimulatingthe activity of ERK1/2. As expected, PD98059 inhibited the effectof ET-1 by >75%. Figure 3D shows the translocation of ERK1/2 fromcytoplasm to nucleus on ET-1 stimulation. Cells after serum withdrawal(top) showed very faint staining with the anti-phosphorylatedERK1/2 antibody, suggesting that the MAPK activity was low. WhenET-1 was added to cells, positive staining in the nucleus increasedgreatly at 5 and 15 min (middle and bottom). At 30 min, the nuclearstaining was less than that at 5 and 15 min, but still more intensethan that at time 0 (data not shown). Similar results were obtainedwhen FBS (5%) was added to cells after serum withdrawal (datanot shown). These results obtained from different approaches indicatethat ET-1 exhibits a profound effect on activating ERK1/2 in thesecells. Furthermore, in combination with the control studies describedin Experimental Procedures, the MAPK assay using the syntheticpeptide as the substrate proves to be an accurate and useful methodfor determining the ERK1/2 activity quantitatively.

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Fig. 3. Effects of ET-1 on ERK1/2. A, phosphorylation of ERK1/2. Cells were serum-starved for 48 h at 37°C and then treated with or without ET-1 (10 nM) or bFGF (10 ng/ml) for 5 min. Cellular extracts were prepared and analyzed by SDS/PAGE and Western blotting using an anti-phosphorylated ERK1/2 antibody as described in Experimental Procedures. B, determination of ERK1/2 activity after immunoprecipitation. Cells were treated as in A. ERK1/2 were immunoprecipitated and then assayed for the kinase activity as described in Experimental Procedures. Radioactivity, but not nanomoles per milligram per minute, was reported for the ERK activity because the protein content of ERK1/2 could not be determined accurately in the immunoprecipitates. C, determination of ERK1/2 activity in cellular extracts. Cells were serum-starved as in A. Cells were then treated with 80 µM PD98059 for 1 h before stimulated with 10 nM ET-1 for 5 min. Cellular extracts were prepared and assayed for the ERK1/2 activity directly without immunoprecipitation. D, ERK1/2 translocation. Cells in chamber slides were serum-starved for 48 h at 37°C and then treated with ET-1 (10 nM) for different time periods. Cells were then fixed and immunostained as described in Experimental Procedures.

Activity of ERK1/2 after Paclitaxel Treatment and Serum Withdrawal. To investigate the effect of ET-1 and paclitaxel treatment on the ERK1/2 pathway, the activity of ERK1/2 after paclitaxeltreatment in the presence or absence of ET-1 was examined by usingthe quantitative MAPK assay with the synthetic peptide as thesubstrate. It is important to note that to keep the experimentalconditions similar to the apoptosis studies noted previously,cells were fed with SmGM containing 5% FBS 24 h before the treatment.Figure 4A shows that when cells were treated with paclitaxel,the ERK1/2 activity decreased to 30% of control (the activityat time 0) at 1 h and stayed at that level for $>=$ 8 h. When ET-1was added together with paclitaxel, the ERK1/2 activity was maintainedat a level similar to that at time 0 for up to 4 h. Even at 8h, the ERK1/2 activity in the presence of ET-1 was 51% higherthan that in the absence of ET-1. Figure 4B shows the resultsfrom a more detailed examination of the ERK1/2 activity in thefirst hour of treatment with paclitaxel and ET-1. The ERK1/2 activityat time 0 was 0.57 ± 0.01 nmol/mg/min. On treatment with paclitaxel,the ERK1/2 activity was slightly increased by 39% at 5 min andthen decreased to 45% of control at 20 min, a 55% decrease inthe activity compared with that at time 0. The addition of ET-1(10 nM) in the presence or absence of paclitaxel stimulated theactivity of ERK1/2 in a transient manner, reaching a peak at 2.47± 0.05 nmol/mg/min after 5 min of incubation at 37°C and decliningto nearly the level at time 0 within 20 min. When ET-1 was addedwith paclitaxel, the ERK1/2 activity was maintained at ~2-foldof that in the presence of paclitaxel without ET-1 at 1 h afterthe treatment.

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Fig. 4. Determination of the ERK1/2 activity after paclitaxel treatment. Cells were fed with SmGM medium containing 5% FBS 24 h before the experiments. Cells were then treated with paclitaxel (1 µM) for different time periods in the presence or absence of 10 nM ET-1 without a medium change. Cellular extracts were prepared, and the ERK1/2 activity was determined as described in Experimental Procedures. Each value represents mean ± S.D. of three determinations.

It may be worth noting that there is variation from experiment to experiment regarding when the ERK1/2 activity starts todecrease after paclitaxel treatment, possibly because differentbatches of cells behave differently. However, a clear differencebetween paclitaxel alone and paclitaxel plus ET-1 was always observedat 60 min andbeyond.

Similar studies were performed to investigate the effect of serum withdrawal in the presence or absence of ET-1 on the ERK1/2activity. Figure 5A shows that the ERK1/2 activity in cells fed24 h before with SmGM containing 5% FBS was 0.36 ± 0.01 nmol/mg/min.On serum withdrawal, the ERK1/2 activity decreased rapidly to64% of control (the activity at time 0) in the first 10 min andthen decreased to 16% of control at 20 min, reaching a low constantlevel at 0.084 ± 0.012 nmol/mg/min, which was maintained duringthe 48-h study period. From 10 separate experiments, the MAPKactivity at 48 h after serum withdrawal was 0.060 ± 0.029 nmolP_i/mg/min. When ET-1 was added to cells after serum withdrawal,a transient spike in the ERK1/2 activity was observed (Fig. 5A).The ERK1/2 activity increased to 0.97 ± 0.05 nmol/mg/min at 5min (a 2.7-fold increase in comparison to time 0) and then decreasedto 0.24 ± 0.04 nmol/mg/min at 20 min, which was >3-fold of theactivity without ET-1 at the corresponding time. Even at 4 h afterserum withdrawal, the ERK1/2 activity in the presence of ET-1was still maintained at that level, 2.9-fold higher than thatin the absence of ET-1. As a comparison, Fig. 5B shows that whenFBS (5%) was added to cells after serum withdrawal, the ERK1/2activity at 5 min was increased to 3.5-fold of control (time 0).The MAPK activity then gradually decreased. After 4 h, the MAPKactivity was at a similar level to that at time 0.

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Fig. 5. Determination of the ERK1/2 activity after serum withdrawal. Cells were fed with SmGM medium containing 5% FBS 24 h before being serum-starved for different time periods in the presence or absence of 10 nM ET-1 (A) or 5% FBS (B) with or without 80 µM PD98059 (PD). Cellular extracts were prepared, and the ERK1/2 activity was determined as described in Experimental Procedures. Each value represents mean ± S.D. of three determinations.

The effect of PD98059 was also examined. Figure 5, A and B, show that pretreatment of cells with PD98059 for 30 min completelyabolished the effects of both ET-1 and FBS on stimulating andmaintaining the MAPK activity (Fig. 5, A andB).

These results show that paclitaxel treatment and serum withdrawal down-regulated the ERK1/2 activity and that ET-1 was ableto activate and maintain the ERK1/2 activity in the presence ofpaclitaxel or under serum-withdrawalcondition.

	Discussion

Top Abstract Introduction Experimental Procedures Results Discussion References

The role that GPCRs play in apoptosis is controversial. Ligands for GPCRs have been shown to be both antiapoptotic and proapoptotic.For example, sphingosine-1-phosphate, a bioactive lipid that bindsto the GPCR Edg-1, is shown to suppress apoptosis in HL-60 andPC12 cells (Van Brocklyn et al., 1998). On the other hand, activationof angiotension II type 2 receptor promotes apoptosis in a ratpheochromocytoma cell line and a mouse fibroblast cell line involvingthe dephosphorylation of MAPKs (Yamada et al., 1996). RegardingET, we and others (Shichiri et al. 1997, 1998) have shown thatET is antiapoptotic in smooth muscle cells, fibroblasts, and endothelialcells, whereas Okazawa et al. (1998) reports that ET induces apoptosisin A375 human melanoma cells. It is possible that different GPCRsin different cells and tissues play opposite roles in promotingor inhibiting the survival of cells. Studies on the involvementof ET-1 in regulating apoptosis pathways are still in the earlyphase. Very little is known about how ETs modulate apoptosis andwhether the anti- versus proapoptosis effects of ETs in differentcells are mediated by the same or different pathways. The roleof the ET system in regulating apoptosis remains an interestingand potentially important area for futureresearch.

ET-1 activates various kinases, including PKC, EGF receptor kinase, and MAPK. These kinases all have been shown to be involvedin apoptosis signaling. For example, that PKC plays a role inapoptosis has been shown in HL-60 cells. Treating HL-60 cellswith 12-O-tetradecanoylphorbol-13-acetate, a PKC activator, resultsin the inhibition of apoptosis (Stadheim and Kucera, 1998). Inhibitionof EGF receptor kinase leads to the induction of apoptosis inhuman carcinoma cell line HN5 (Modjtahedi et al., 1998). Furthermore,activation of ERK1/2 is shown to be antiapoptotic (Párrizas etal., 1997; Stadheim and Kucera, 1998; Yan and Green, 1998). Ourresults show that inhibitors of PKC and JAK do not significantlyaffect apoptosis induced by serum withdrawal in HPrSMC. As a comparison,PD98059, an inhibitor of MEK-1, induces apoptosis in cells culturedin medium containing 5% FBS, potentiates apoptosis induced byserum withdrawal, and completely abolishes the antiapoptotic effectof ET-1. Previously Shichiri et al. (1998) have shown that inTGR-1 fibroblasts, PD98059 itself does not induce apoptosis butis able to abolish the antiapoptotic effect of ET-1, suggestingthat ERK1/2 seems to mediate the antiapoptotic effect of ET-1in those cells, a finding that is consistent with our observation.Furthermore, we show that although the ERK1/2 activity decreasesrapidly after serum withdrawal or paclitaxel treatment in HPrSMC,the addition of ET-1 prevents the rapid fall in the ERK1/2 activityand sustains the ERK1/2 activity at a higher level for at least4 h after serum withdrawal or paclitaxel treatment. The effectof ET-1 on ERK1/2 is also substantially inhibited by PD98059.Taken together, these data show that ERK1/2 is important for thesurvival of HPrSMC and suggest a role of ERK1/2 in the antiapoptoticeffect of ET-1. Because cells used in this study are primary culturehuman cells with passage numbers <9, it is difficult to transfectthese cells with dominant-negative mutants of ERK1/2 to confirmthe observation made by using the kinase inhibitors. However,we feel that the observation is particularly important, becausethe cell system used in this study is of human origin and is inthe natural state without artificialmanipulation.

The antiapoptotic effect of ET-1 under serum withdrawal is extremely potent, with an approximate EC₅₀ value of 0.1 nM, whichis ~10-fold less than that in paclitaxel-induced apoptosis studieswith cells cultured in medium containing 5% FBS (Wu-Wong et al.,1997). However, it is important to note that the EC₅₀ value isconsistent with those observed in other ET-1-evoked biologic responses,especially under conditions with a low concentration of serumalbumin or other proteins. The primary reason for this differencein the EC₅₀ values in the presence or absence of serum albumincan be explained based on our previous finding that ET receptorligands, including ET-1, -3, and some receptor antagonists, exhibita high degree of binding to serum albumin and other human plasmaproteins (Wu-Wong et al., 1998). The addition of increasing dosesof plasma or serum albumin can incrementally decrease the potencyof ET-1 and vice versa. Therefore, it is expected that the EC₅₀in the absence of serum will be less than that in the presenceofserum.

During this study, we have never observed a complete inhibition of apoptosis by ET-1. As a comparison, addition of 5% FBScompletely blocked apoptosis. To test the possibility that degradationof ET-1 was responsible for the lack of complete inhibition, wehave conducted a series of experiments in which ET-1 was addedevery 4 h during the 48-h incubation period after serum withdrawal.A partial inhibition of apoptosis was still observed. It is possiblethat FBS, but not ET-1, is able to activate an ERK-independentpathway that is also involved in apoptosis signaling. Anotherpossibility may be linked to the fact that although ET-1 has aprofound effect on activating ERK1/2, the ERK1/2 activity in thepresence of ET-1 is maintained at a less active state than thatin the presence of FBS (Fig. 5). Also, it is interesting to notethat ET-1 does not stimulate cell growth in these cells (Fig.1C), although ET-1 is a mitogenic factor for human pericardialsmooth muscle cells (Wu-Wong et al., 1994). It appears that theeffect of ET-1 on activating ERK1/2 in the prostatic smooth musclecells is linked specifically to apoptosis, but not to cell proliferation.Previously, it has been shown that activation of ERK1/2 is required,but not sufficient, for cell growth in some cell types (Post etal., 1996; Hügl et al., 1998). Our observation in this studyis consistent with thatnotion.

In conclusion, our results strongly suggest that ERK1/2 is involved in ET-1 antiapoptotic signaling. However, we can- notrule out the possibility that other, yet-to-be-identified, pathwaysmay be involved. It will be necessary to examine proteins involvedin regulating apoptosis, such as bcl-2, bax, and bad, to developa better understanding of apoptosis signaling pathways involvingGPCRs.

	Acknowledgments

We thank Cathy Berg for excellent technical assistance in cell culture. We thank Dr. Terry J. Opgenorth for hiscomments.

	Footnotes

Accepted for publication January 20, 1000.

Received for publication July 6, 1999.

Send reprint requests to: Dr. Jinshyun R. Wu-Wong, T551, Abbott Laboratories, 5440 Patrick Henry Dr., Santa Clara, CA 95054. E-mail: ruth.r.wuwong{at}abbott.com

	Abbreviations

ERK, extracellular signal-regulatedkinase(s); GPCRs, G protein-coupled receptors; ET, endothelin; FBS, fetal bovine serum; PAGE, polyacrylamide gel electrophoresis; ELISA, enzyme-linked immunosorbent assay; HPrSMC, human prostatic smooth muscle cells; PI3K, phosphatidylinositol 3-kinase; PKC, protein kinase C; EGF, epidermal growth factor; SFM, serum-free medium; MAPK, mitogen-activated protein kinase; bisindo, bisindolylmaleimide.

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