Functional Estrogen Receptors in the Mitochondria of Breast Cancer Cells

Ali Pedram^*, Mahnaz Razandi^*, Douglas C. Wallace, and Ellis R. Levin^*^||

^* Division of Endocrinology, Veterans Affairs Medical Center, Long Beach, Long Beach, CA 90822; Department of Medicine, University of California, Irvine, Irvine CA 92717; Department of Biochemistry, University of California, Irvine, Irvine CA 92717; ^|| Department of Pharmacology, University of California, Irvine, Irvine CA 92717; and Department of the Center for Molecular and Mitochondrial Medicine and Genetics, University of California, Irvine, Irvine CA 92717

Submitted November 4, 2005; Revised January 26, 2006; Accepted February 15, 2006
Monitoring Editor: M. Bishr Omary

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Steroid hormones have been reported to indirectly impact mitochondrialfunctions, attributed to nuclear receptor-induced productionof proteins that localize in this cytoplasmic organelle. Herewe show high-affinity estrogen receptors in the mitochondriaof MCF-7 breast cancer cells and endothelial cells, compatiblewith classical estrogen receptors ER ${alpha}$ and ER $beta$ . We report thatin MCF-7, estrogen inhibits UV radiation-induced cytochromeC release, the decrease of the mitochondrial membrane potential,and apoptotic cell death. UV stimulated the formation of mitochondrialreactive oxygen species (mROS), and mROS were essential to inducingmitochondrial events of cell death. mROS mediated the UV activationof c-jun N-terminal kinase (JNK), and protein kinase C (PKC) ${delta}$ , underlying the subsequent translocation of Bax to the mitochondriawhere oligomerization was promoted. E2 (estradiol) inhibitedall these events, directly acting in mitochondria to inhibitmROS by rapidly up-regulating manganese superoxide dismutaseactivity. We implicate novel functions of ER in the mitochondriaof breast cancer that lead to the survival of the tumor cells.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Estrogen promotes the development, proliferation, migration,and survival of target cells including breast cancer. The actionsof estradiol (E2) have traditionally been thought to occur throughbinding nuclear steroid receptors (Jensen and Jacobson, 1962).Nuclear estrogen receptors (ER) transcribe genes whose proteinproducts lead to the biological actions of the sex steroid.Most mitochondrial proteins are transcribed in the nucleus andE2 and nuclear ER regulate some relevant genes in this respect.However, recent work has supported the idea that a second poolof ER, localized to the plasma membrane, also importantly contributesto the actions of E2 (Levin, 2001).

Additionally, a large pool of ER have been described in thecytoplasm of various target cells, but the precise localizationand functions are unclear. Recent data support the idea thatsome ER localize to the mitochondria of MCF-7 cells (Chen etal., 2004). However, it is largely unknown whether these receptorsparticipate in any actions of the steroid that impact the functionof this organelle or the whole cell.

In breast cancer, abnormal proliferation and the increased survivalof transformed cells are essential to the pathogenesis of thedisease (Wang, 2001; Chen et al., 2004). Tumor therapies forthis malignancy are particularly effective when cell survivalmechanisms are disrupted, inducing apoptotic cell death (Yuet al., 1998; Wang, 2001). Regarding apoptosis, a lynchpin eventfor many stimuli to enact this form of cell death is the releaseof cytochrome C from mitochondria into the cytoplasm, afterthe development of the mitochondrial transition pore. CytochromeC in the cytoplasm complexes to and oligomerizes apoptosis activatingfactor-1 (Apaf-1), leading to the activation of caspase 9 andthe effector caspase cascade. Effector caspases (such as caspases3, 7, and 10) cleave and activate many substrates that committhe cell irrevocably to death (Wang, 2001). Translocation ofcytochrome C to cytoplasm often precedes the decrease of themitochondrial membrane potential (Danial and Korsmeyer, 2004),another marker of subsequent cell death. Modulation of theseevents determines cell fate but whether and how E2 regulatesthe intrinsic mitochondrial pathway of apoptosis in breast canceris unknown.

Relevant to these considerations, we identify high-affinitymitochondrial ER compatible with classical ER ${alpha}$ and ER $beta$ in severalcell types. In breast cancer, E2/ER promotes the proliferationand survival of these malignant cells. We speculated that becausemitochondria are an essential part of both the extrinsic andintrinsic pathways of programmed cell death (Wang, 2001), themitochondrial ER pool might contribute through several mechanismsto cell survival. We therefore determined how radiation inducesthe key mitochondrial events of apoptosis and the role of mitochondrialER to prevent many of these steps.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Cell Culture and Plasmid Preparation
MCF-7 and bovine aortic or mouse brain capillary EC were isolatedand cultured as previously described (Razandi et al., 2000,2004a). The targeting of the E domain of ER ${alpha}$ to the mitochondriawas accomplished as follows. The mouse ER ${alpha}$ -E domain was subclonedby RT-PCR using the primers 5'-TTGGATCCGAACAGCCTGGCCTTGTC-3'and 5'-AAACCGGTGTGGGCGCATGTAGGC-3'. The PCR product was clonedusing the TOPO TA 2.1 cloning kit (Invitrogen, Carlsbad, CA),into BamHI and AgeI restriction sites on the pECFP-Mito vector(Clontech, Palo Alto, CA). The vector was confirmed by sequencing.Nuclear and membrane-targeted E domain construction and validationwas previously described (Razandi et al., 2003, 2004b).

Mitochondrial Isolation
Mitochondria were isolated by the method adapted from Trounceet al. (1996). Subconfluent MCF7 cells or BAEC cells were collectedby gentle scraping and centrifuged at 1000 rpm for 5 min topellet the cells. Cell pellets were washed once with phosphate-bufferedsaline (PBS) and twice with buffer A (0.25 M sucrose, 210 mMD-mannitol, pH 7.8). Final cell pellets were resuspended inbuffer A containing 1 mM EDTA and DNase (prevent aggregationby released DNA) and protease inhibitor cocktail (Sigma, St.Louis, MO). Cells were homogenized using 15–20 strokesof the pestle of a tight-fitting Dounce homogenizer until $~$ 90%of the cells were broken. Homogenates were centrifuged at 1000x g for 10 min to pellet the nuclear fraction. The supernatantswere layered onto a discontinues sucrose gradient (1.0–2.5M) made up in buffer containing 10 mM Tris, pH 7.6, 2 mM EDTA,2 mM DTT, protease inhibitor cocktail, and 1 mM phenylmethylsulfonylfluoride. The mixtures were centrifuged at 2000 rpm for 30 minat 4°C producing a top layer (cytosol) and a mitochondriallayer at the 1.0–1.5 M sucrose gradient interface. Themitochondrial fractions were removed from the centrifuge tubewith a 22-gauge needle and 1-ml syringe, washed in four volumesof mannitol/sucrose buffer, and centrifuged at 1000 rpm for15 min at 4°C. The pellets containing mitochondria weresuspended in PBS, pH 7.4, sampled for protein concentration(BCA method), and stored at –80°C until further analysis.Mitochondrial protein was determined by the method of Lowry.

Saturation Binding Studies
Saturation and competitive binding of ³H-estradiol were carriedout on whole cells as described (Razandi et al., 2003), andthe cells then were fractionated into plasma membrane, nuclear(Razandi et al., 2004b), and mitochondrial isolates by sucrosegradient centrifugation. Unlabeled E2 from 0.01 to 1000 nM wasused for competition, and the studies were carried out at 60min at 37°C. Free [³H[17- $beta$ -E2 was separated by resin adsorptionof the ligand–receptor complex using the hydroxylapatite(HAP) technique (Wecksler and Norman, 1999). Binding was analyzedby Scatchard analysis, using the LIGAND binding computer program.Purity of the subcellular isolates was established by Westernblot of fractional proteins after SDS-PAGE separation and transferto nitrocellulose. Antibodies used were from Santa Cruz Biotechnology(Santa Cruz, CA) and detection was accomplished using the ECLkit (Amersham, Indianapolis, IN).

ER Detection in Mitochondria
MCF-7 cells were cultured on coverslips overnight and then incubatedfor 20 min with Mitotracker dye (red; Molecular Probes, Eugene,OR) that localizes to the mitochondria. After washing with PBS,the cells were fixed with paraformaldehyde and permeabilizedwith 0.2% Triton-X and then incubated with antibody to eitherthe C-terminus of ER ${alpha}$ (Santa Cruz Biotechnology) or the N-terminusof ER $beta$ (Zymed, South San Francisco, CA; Razandi et al., 2004a).This was followed by second antibody conjugated to FITC (greencolor). ER antibodies preabsorbed with purified ER ${alpha}$ or ER $beta$ protein,or nonspecific IgG were used as additional negative controls.Western blot of specific proteins in isolated mitochondria,plasma membrane, and nuclear cell fractions was also performed,and samples from each condition were normalized by measuringthe total protein (Bradford assay). Antibodies were from SantaCruz Biotechnology.

Manganese Superoxide Dismutase Assay
Superoxide dismutase (SOD) activities were determined from protein-normalizedaliquots from each condition, using a Superoxide Dismutase AssayKit (Cayman Chemical, Ann Arbor, MI). Tetrazolium salt was usedfor detection of superoxide radicals, and the radicals generatedby provided xanthine oxidase were quenched by known amountsof exogenous SOD. This generated a standard curve for comparisonto cell samples containing endogenous SOD activity. MCF-7 cellswere collected by scraping and centrifuged, and the pelletswere sonicated in cold buffer containing sucrose. In some experiments,a mitochondrial extract was prepared. The cell or mitochondrialextract supernatant was centrifuged at 1500 x g for 5 min at4°C and then centrifuged at 10,000 x g for 15 min at 4°C.The resulting supernatant contained cytosolic SOD (CuZnSOD),and the pellet contained mitochondrial SOD (MnSOD). Also, inwhole cell preparations, we used 2 mM potassium cyanide to inhibitboth Cu/Zn-SOD and extracellular SOD, resulting in the detectionof only MnSOD activity. The samples were analyzed using a platereader with a 450-nm filter. Each data point was performed intriplicate, and the results from multiple experiments were combinedand reported as mean absorption ± SE.

Mitochondrial Functions in Apoptosis
MCF-7 cells were exposed to 50 Joules of UV irradiation in 1s to induce apoptosis (Razandi et al., 2000, 2004a). The cellswere processed for Western blotting of cytochrome C, both releasedinto cytosol and remaining in mitochondria over a 4-h period.Some cells were exposed to 10 nM E2 just before irradiationand for the duration of the experiment. In additional experiments,HCC-1569 were transiently transfected to express the E domainof ER ${alpha}$ , incorporated into plasmids that included cell membrane,mitochondrial, or nuclear targeting sequences (Clontech), thecells were recovered overnight, and similar studies were carriedout.

Decreases in the mitochondrial membrane potential were evaluatedusing the Apo Alert Mitochondrial Membrane Sensor Kit (ClontechLaboratories). MCF-7 cells cultured on coverslip were exposedto UV ± 10 nM E2 with or without ICI182780 and then leftfor 4 h. Cells were also exposed to ICI alone or E2 alone ascontrols. When using HCC-1569 cells, the cells were grown oncoated glass bottom culture dishes (MatTek, Ashland, MA). Aftertransient transfection with the E domain of ER ${alpha}$ targeted to differentcompartments, cells were synchronized and treated as described.At the end of the treatment, all cells were washed in PBS andincubated with Mitosensor dye (5 µg/ml) for 20 min at37°C. The cells were examined at 20x by fluorescent confocalmicroscopy using a band-pass filter. The Mitosensor dye aggregatesin the mitochondria of healthy cells and shows red fluorescence.In apoptotic cells, the mitochondrial membrane potential isaltered; Mitosensor cannot accumulate in the mitochondria andremains as a green fluorescent monomer in the cytoplasm.

ROS Formation
Cultured cells were loaded with 10 µM 2'7'-dichlorodihydrofluorescindiacetate (CM-H2DCFDA, Molecular Probes) for 1 h before theapoptotic stress. In cells, esterases cleave the acetate estersto release free CM-H2DCF, which is nonfluorescent. After oxidationby ROS, CM-H2DCF is converted to green-fluorescing dichlorofluorescein(DCF; Curtin et al., 2002). After brief UV exposure, the cellswere left for 4 h, then washed, fixed, and permeabilized withPBS containing 20% ethanol and 0.1% Tween 20. In some experiments,10 nM E2 was added for 4 h. Cell extracts were centrifuged,and supernatants collected. DCF fluorescence was quantifiedwith a fluorescence plate reader using 450-nm excitation and530-nm emission filters. Confocal microscopy provided a qualitativeassessment. The study was carried out three times, and the meanand SD were analyzed by ANOVA plus Schefe's test at a p <0.05 level of significance.

Bax Dimerization and Translocation
MCF7 cells at near confluency were synchronized and then subjectedto UV irradiation ± E2 for 6 h except control cultures(sham irradiated). Isolated mitochondria were washed, and thecross-linker, dithiobis (DSP; Pierce, Rockford, IL), was addedin dimethyl sulfoxide. Cross-linking for 30 min at room temperaturepreceded centrifugation at 10,000 x g for 15 min, and the mitochondriapellet was suspended in lysis buffer. Anti-Bax monoclonal antibody(6A7, Sigma) was preincubated with protein A Sepharose. Thecell lysates were normalized for protein content, and 500 µgof total protein in Chaps-containing lysis buffer was addedto the tube containing Bax antibody-loaded beads and incubatedat 4°C overnight. After rinsing, beads were collected andBax protein was eluted with sample buffer for Western blotting.The separated proteins were transferred to nitrocellulose followedby blocking with 5% (wt/vol) nonfat milk powder in buffer. Membraneswere probed with primary antibody followed by peroxidase-conjugatedsecondary antibody, visualized using an ECL detection kit.

Interfering RNA to PKC and MnSOD Studies
Double-stranded RNA for PKC ${delta}$ , PKC ${epsilon}$ , PKC $beta$ (control), or MnSOD orGFP (control) was obtained from Santa Cruz Biotechnology (SC-36521,36252,29450)or Dharmacon (Boulder, CO; M-009784). We transfected 2.5 µgeach of the siRNAs in MCF-7 using OLIGOfectamine as described(Razandi et al., 2004b), recovered and synchronized the cellsover 48 h, and then carried out the various experiments. Immunoblotsfor the proteins were carried out 48 h after transfection tovalidate the protein knockdown and specificity of the constructs.

PKC and JNK Activity
PKC ${delta}$ and PKC ${epsilon}$ activities were determined as phosphorylation ofthe protein isoform at the active site. Cells were exposed tovarious conditions and the cells were lysed, then separatedby SDS-PAGE, transferred to nitrocellulose, and immunoblottedwith antibodies to tyrosine 311 (PKC ${delta}$ ) or serine 729 (PKC ${epsilon}$ ; SantaCruz) or with antibodies to determine total PKC protein. JNKactivity was determined as previously described (Razandi etal., 2000). SP600125 (JNK1 inhibitor) and Rottlerin (PKC ${delta}$ inhibitor)were from Calbiochem (San Diego, CA). PKC isoform activity againstpeptide substrate was also determined. Cells were incubatedwith 10 nM E2 in the presence of absence of UV exposure for4 h. PKC ${delta}$ or PKC ${epsilon}$ was immunoprecipitated from MCF-7 cells lysateusing specific antibodies (Santa Cruz), and the proteins werenormalized for an in vitro activity assay. The tube activityassay included ³²P-ATP, substrate peptide (glycogen synthasekinase; Calbiochem), and normalized PKC isoform protein fromeach experimental condition. PKC activity was determined aftera 30-min incubation at 30°C, and the phosphorylated substratewas identified after SDS-PAGE. Total PKC protein was determinedby Western blot for sample normalization.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Identification of Mitochondrial ER
We first established high-affinity, saturable ER in plasma membrane,nucleus, and mitochondrial cell fractions of MCF-7 cells (K_d= 0.2–0.3 nM; Figure 1A, left). Approximately 85% of receptorswere present in the nucleus, 5% in the plasma membrane, and10% in the mitochondria. The lack of contamination of cell fractionswas demonstrated by Western blot for integral membrane (5'nucleotidase[NT]), nuclear (transportin and NTF2), and mitochondrial proteins(cytochrome C; Figure 1A, right). High-affinity mitochondrialER were also found in endothelial cells (EC; unpublished data).

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Figure 1. High-affinity ER in mitochondria (A). Left, competition binding of [³H]17 $beta$ -E2 to nuclear, mitochondrial, and cell membrane fractions of MCF-7 cells. K_ds for nuclear, mitochondrial, and cell membrane receptors were 0.283, 0.290, and 0.287 nM, respectively, calculated by Scatchard analysis using the LIGAND computer program. The studies were repeated twice. Right, purity of cell fractions. Immunoblots of membrane protein (5'NT), nuclear proteins (transportin and NTF), Golgi protein ( $beta$ -COP) and mitochondrial protein (cytochrome C) were carried out in the MCF-7 cell fractions. (B) Western blot of MCF-7 (left) or bovine aortic EC (right) cell fractions. Cell lysate was immunoprecipitated with specific antibodies to the ER ${alpha}$ and ER $beta$ isoforms, normalized for protein, and proteins were separated by gel electrophoresis, transferred, and then immunoblotted. Molecular weight markers are shown. (C) Immunofluorescence confocal microscopy of ER ${alpha}$ (left) and ER $beta$ (right) in MCF-7. The cells were cultured on coverslips and then incubated for 20 min with Mitotracker dye (red; Molecular Probes). After washing, the cells were fixed and permeabilized and then incubated with antibody to either ER isoform, followed by second antibody conjugated to FITC (green color). Overlap is seen in yellow. (D) Lack of mitochondrial ER in ER ${alpha}$ /ER $beta$ deleted cells. EC were isolated from the capillaries of mice bred for combined ER ${alpha}$ and ER $beta$ deletion (DERKO). Confocal microscopy fails to show any ER in any cell compartment in EC from DERKO mice, whereas EC from wild-type mice show receptors for each ER isoform in various cell locations.

Using antibodies to traditional ER isoforms, we determined inMCF-7 cells that endogenous ER ${alpha}$ and ER $beta$ are present in plasmamembrane, nucleus, and mitochondrial cell fractions. The overallcellular ER $beta$ protein is considerably less abundant than ER ${alpha}$ (Figure 1B,left), consistent in that ER $beta$ is produced in low abundance inbreast cancer (Fuqua and Cui, 2004

). Interestingly, the smallamount of ER $beta$ is concentrated in mitochondria. This is differentfrom EC, where ER $beta$ (and ER ${alpha}$ ) are predominantly expressed in thenucleus, and the relative amount of ER ${alpha}$ exceeds ER $beta$ in mitochondria(Figure 1B, right). Confocal microscopy confirmed ER ${alpha}$ in membrane,nuclear, and mitochondrial cell compartments of the MCF-7 cell(Figure 1C, left). ER $beta$ was also detected (Figure 1C, right),and both ER isoforms colocalized with the mitochondria specificdye, Mitotracker. Again, ER $beta$ was predominantly found in the mitochondriaof MCF-7 (Figure 1C, right). Antibodies preabsorbed with purifiedER ${alpha}$ or ER $beta$ protein or nonspecific IgG showed no staining of proteinsin the cells (unpublished data).

To further support the idea that mitochondrial ER ${alpha}$ and ER $beta$ derivefrom the same genes coding for classical nuclear ER isoforms,we examined EC from combined ER ${alpha}$ /ER $beta$ knockout mice (DERKO) (11).Wild-type EC demonstrated endogenous ER ${alpha}$ in several cell locations,most prominently in the nucleus, and ER $beta$ was found substantiallyin mitochondria. In contrast, DERKO EC produced no detectableER in any region of the cells (Figure 1D). Thus, in EC, mitochondrialER derive from the same genes (ER ${alpha}$ or ER $beta$ ) that also produce nuclearand membrane ER (Razandi et al., 2004b).

ER Functions in the Cell Survival of Breast Cancer
Breast cancer cells respond to irradiation by undergoing apoptoticcell death (Xia and Powell, 2002). We previously reported thatE2 inhibits radiation-induced cell death in MCF-7 cells (Razandiet al., 2000, 2004a). In part, this resulted from membrane-initiatedsteroid signaling to activation of ERK and PI3 kinases, perhapsimpacting the mitochondria. E2/ER inhibition of JNK activitythrough undetermined ER pools or mechanisms also contributed(Razandi et al., 2000, 2004a). Nuclear and membrane ER alsosignal to the up-regulation of genes such as Bcl2 (Dong et al.,1999), the protein products of which promote long-term cellsurvival. Whether E2 acts directly at mitochondrial ER to impactcell fate is unknown.

To understand whether E2 influences apoptotic events in themitochondria, we determined the release of cytochrome C fromthis organelle in UV-irradiated MCF-7 cells. UV induced themaximal translocation of cytochrome C from mitochondria intothe cytoplasm at 60 min, significantly prevented by E2 (Figures 2A,left and right). Cytochrome C redistribution was also visualizedin the intact cell, and ICI182780, an estrogen receptor antagonist,substantially although incompletely blocked the action of E2(Figure 2B). Irradiation of MCF-7 cells also decreased the mitochondrialmembrane potential, reflecting the commitment to apoptosis (Figure 2C).The shift from mainly red to green color occurred as the dyefailed to be taken up in the mitochondria of dying cells. E2significantly decreased the numbers of cells showing loss ofmembrane potential by $~$ 60%, substantially prevented by ICI182780.

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Figure 2. Mitochondrial effects of E2. (A) Left, cells were treated with brief UV exposure (50 J/s) and abundance of cytochrome C was determined in MCF-7 cell fractions by Western blot for up to 240 min. The study was repeated. Right, E2 prevents UV-induced cytochrome C release into the cytosol at 60 min. MCF-7 were briefly exposed to UV in the presence or absence of E2, and steroid was continued for 60 min. (B) A predominantly mitochondrial distribution of cytochrome c (control) changed to a largely diffuse cytosolic pattern in response to UV, prevented by E2. MCF-7 were briefly exposed to UV, with or without 10 nM E2, or E2+ICI182780 (1 µM; ER antagonist) for 60 min. After fixing and permeabilizing the cells, incubation with the first antibody to cytochrome C was followed by second antibody conjugated to FITC. The study was repeated. (C) MCF-7 were briefly exposed to UV, the cells incubated with or without E2 or ICI182780 for 4 h, and then loss of membrane potential was determined using the Apo-Alert kit (Clontech) as described in Materials and Methods. Decreased mitochondrial membrane potential was seen as a color change from predominantly red to green. As controls, cells were also exposed to ICI or E2 alone without significant effect (unpublished data).

Role of Mitochondrial ER
To determine whether E2 acted at mitochondrial ER, we targetedthe ligand-binding domain (E domain) of ER ${alpha}$ to the plasma membraneor nucleus (exclusive targeting to these pools shown in Razandiet al. 2004b

), or to the mitochondria of ER negative, HCC-1569breast cancer or CHO cells. Expression of the E domain in mitochondriawas demonstrated by substantial overlap with Mitotracker dyeand by Western blot of cell fractions (Figure 3A). We then examinedcytochrome C translocation.

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Figure 3. E domain of ER ${alpha}$ mediates E2 effects at the mitochondria. (A) Left, expression of the mitochondrial-targeted E domain of ER ${alpha}$ . CHO cells were transfected to express the E domain of ER ${alpha}$ (green) targeted to the mitochondria, using a targeting vector containing a mitochondrial localization sequence (Clontech). Mitotracker dye indicates the mitochondria (red). The merged panel shows virtually complete colocalization of ER with Mitotracker dye (orange-yellow). Right, Western blot of ER ${alpha}$ E domain targeted to the mitochondria and expressed in HCC-1569 cells. Western blot of cell fractions was accomplished with an antibody to the ER ${alpha}$ ligand-binding domain (H222). (B) The E domain of ER ${alpha}$ was targeted to the plasma membrane, mitochondria, or nucleus in HCC-1569 cells. Western blot of cytochrome C in cytoplasm at 60 min post-UV in the presence or absence of 10 nM E2 treatment is shown. The study is representative of two experiments. (C) Mitochondrial membrane potential and apoptosis in E domain-targeted HCC-1569 cells. Cells were briefly exposed to UV, then ±E2, or E2 alone, and membrane potential/apoptosis was determined at 4 h. Control cells were transfected but sham exposed to UV. The bar graph represents the mean plus SEM from three combined studies, 200 cells counted per condition in each. *p < 0.05 for control or E2 alone versus UV, ⁺p < 0.05 for UV+E2 versus UV by ANOVA plus Schefe's test. (D) ER ${alpha}$ and ER $beta$ mediate E2 action at the mitochondria. Isolated mitochondria from MCF-7 cells were exposed to UV ± 10 nM of E2, PPT, or DPN, and cytochrome C release into the incubation medium or in the mitochondrial pellet was determined by Western blot at 60 min. The representative study was repeated twice additionally.

In HCC-1569 cells containing the mitochondrial-targeted E domain,E2 prevented the cytochrome C effects of UV (Figure 3B). UValso reduced the mitochondrial membrane potential in all cells,but this was significantly reversed by sex steroid in mitochondrialER-targeted cells (Figure 3C). In ER null breast cancer cellsexpressing the pcDNA3 plasmid (strict control), there were noE2 effects (unpublished data), supporting the need for ER tomediate E2 actions. Interestingly, plasma membrane targetingof the ER ${alpha}$ E domain also supported E2 reversal of both UV effects(Figure 3, B and C). Perhaps this resulted from ERK or PI3 kinasesignaling from the membrane to cell survival (Razandi et al.,2000

, 2004a

By contrast, targeted expression of the E domain in the nucleusdid not significantly impact cytochrome C translocation or mitochondrialmembrane potential, determined 1 and 4 h, respectively, afterUV exposure. This nuclear only model fully supports E2-inducedproliferation of breast cancer cells (Razandi et al., 2004b),and a comparably truncated ER ${alpha}$ supports nuclear transcription(Lopez et al., 1999). We also targeted a full-length ER ${alpha}$ to thenucleus and found a similar failure of E2 to reverse these eventsof apoptosis (unpublished data).

As a second model, we isolated mitochondria from MCF-7 cells,the purity established as in Figure 1A. UV stress induced therelease of cytochrome C from mitochondria into the incubationmedium (Figure 3D). E2 prevented this (lane3), indicating directaction at this cytoplasmic organelle. To determine which ERisoform mediates this action, mitochondria were exposed to UVin the presence of 10 nM E2, PPT (an ER ${alpha}$ agonist), or DPN (anER $beta$ agonist; Harrington et al., 2003). Each inhibited cytochromeC release, but the ER $beta$ agonist was more potent than the ER ${alpha}$ agonist.Taken together, the combined effects of ER ${alpha}$ and ER $beta$ agonists wereroughly equivalent to the inhibition by E2, likely reflectingcontributions from each mitochondrial ER isoform to steroidaction.

Mechanisms of ER Action in Mitochondria
How does mitochondrial ER protect the viability of irradiatedcells? In cancer, reactive oxygen species (ROS) are importantto apoptosis induced by radiation, chemotherapeutic agents,and many cell stressors (Benhar et al., 2002). In most stresscircumstances, mitochondria generate the great majority of ROS(Finkel and Holbrook, 2000). ROS generation here is normallya result of oxidative phosphorylation, and several of the respiratorycomplexes produce ROS as a result of electron transport betweencomplexes (Curtin et al., 2002). Complexes I and III (especiallythe latter) have been particularly implicated during stress-relatedROS formation.

We first determined that UV induced a strong generation of ROS,substantially reversed by N-acetlycystine (NAC), a nonspecificinhibitor of ROS generated at multiple sites in the cell. Inhibitionof ROS generation also occurred in the presence of Rotenone,a specific inhibitor of the mitochondrial complex I, and potentlyby Mito-Q (Figure 4A). Rotenone either enhances (Ohnishi etal., 2005) or inhibits (Chapman et al., 2005; Sato et al., 2005)ROS formation, depending on the insult and coupled state ofmitochondria. Here, this compound inhibits ROS formation. TheMito-Q compound is a mitochondrial-targeted derivative of ubiquinone.By accepting electrons from complexes I and II, the reducedproduct, ubiquinol, strongly reduces ROS formation, influencingcomplex III function as well (Kelso et al., 2001; James et al.,2005). Mito-Q potently prevented ROS formation by UV, and E2substantially prevented UV-induced ROS in MCF-7 cells, reversedby the ER antagonist, ICI182780 (Figure 4B).

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Figure 4. Reactive oxygen species (ROS) underlies cell fate decisions. (A) MCF-7 cells were exposed to UV ± antioxidants NAC (N-acetylcystine) 5 mM, rotenone 2.5 µM, or Mito-Q 10 µM. ROS production was determined 4 h after UV exposure by confocal microscopy using the fluorescent indicator, CM-H2DCFDA, and quantified by spectroflourometry. The bar graph represents three studies combined. *p <0.05 for control versus UV, ⁺p < 0.05 for UV versus UV plus antioxidant. None of the antioxidant compounds had significant effects on ROS formation by themselves (unpublished data). (B) Estradiol/ER prevents UV-induced ROS formation. The cells were exposed to brief UV, with or without E2 or 1 µM ICI182780, and incubated for 4 h. The bar graph is data from three combined experiments. *p < 0.05 for control versus UV, ⁺p < 0.05 for UV versus UV+E2, ⁺⁺p < 0.05 for UV+E2 versus same plus ICI182780. (C) MCF-7 were exposed to UV ± 0.1–10 nM 17- $beta$ -E2, 10 nM 17- ${alpha}$ -E2, 10 nM progesterone (P) or testosterone (T), or 10 nM PPT or DPN. Steroid compounds were continued for the length of the experiment. Cell viability was determined by the MTT assay at 4 h. Decreased viability is shown by a loss of spectral absorbance to the dye. Data are from three experiments; *p < 0.05 for control versus UV, ⁺p < 0.05 for UV versus UV plus steroid. (D) MCF-7 were exposed to UV ± antioxidants and cell viability was determined by the MTT assay at 4 h. Data are from three experiments; *p < 0.05 for control versus UV, ⁺p < 0.05 for UV versus UV plus antioxidant. (E) Inhibitors of ROS generation reverse UV-induced cytochrome C release into the cytoplasm. A representative study shown here was repeated. Actin serves as loading control.

E2 dose-responsively acted as a survival factor for MCF-7 cells,with significant effects seen at 1 nM E2 (Figure 4C). In contrast,10 nM 17- ${alpha}$ -E2, progesterone, or testosterone did not block UV-inducedcell death, indicating steroid specificity. ER ${alpha}$ - and ER $beta$ -specificagonists each significantly prevented UV-induced cell viability,with the ER $beta$ agonist being slightly more potent (Figure 4C).We also determined that NAC, rotenone, and especially Mito-Qprevented UV-induced loss of cell viability (Figure 4D). Theseresults focus attention on mitochondrial ROS as regulated byUV and E2/ER to explain cell death and survival functions, respectively.

If mitochondrial ROS generation underlies the radiation-inducedmitochondrial death program, then preventing oxidant formationshould rescue these events. We found that UV-induced cytochromeC translocation was almost completely reversed by NAC, rotenone,and especially Mito-Q (Figure 4E). Additionally, Mito-Q preventedthe loss of membrane potential (unpublished data). Thus, localROS stimulation by UV and inhibition by E2 underlies mitochondrialcell fate events.

How might E2 prevent ROS formation and does this stem from mitochondrialER? The dominant mitochondria-specific enzyme that reduces ROSformation in this organelle is MnSOD (Halliwell, 1999; Huanget al., 2000). MnSOD rapidly reduces superoxide, the main mitochondrialROS. We exposed whole cells or isolated mitochondria from MCF-7to UV ± E2 and assayed for MnSOD activity. E2 stronglyup-regulated MnSOD activity in MCF-7 cells, and UV partiallyprevented this action of the steroid (Figure 5A). Critically,isolated mitochondria responded to E2 with robust activationof MnSOD. We also determined the rapidity of E2 up-regulationof MnSOD activity; We found that E2 significantly stimulatedenzymatic activity in the cells between 10- and 20-min exposure(Figure 5B). The stimulation was ER mediated, because ICI182780prevented this action of E2 both at 20 min (Figure 5C, left)and at 4 h (right). We also found that mitochondrial MnSOD proteindid not significantly vary over this time under any condition(Figure 5C, right). The rapid up-regulation of MnSOD activitycoincides with the kinetics of kinase modulation by UV and E2.Interfering RNA that specifically knocked down MnSOD proteinsubstantially reversed the ability of E2 to prevent ROS generation(Figure 5D). Thus, E2 rapidly prevents ROS formation mainlythrough the exclusively mitochondrial SOD. However, cross-talkfrom other ER pools to the mitochondrial MnSOD enzyme mightcontribute to this effect in the intact cell.

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Figure 5. Estrogen upregulates MnSOD activity to inhibit ROS. (A) Isolated mitochondria or whole MCF-7 cells were exposed to UV ± E2, or E2 alone for 4 h, and MnSOD activity was determined using a kit (Cayman). Control is sham UV-irradiated cells. The data are from three combined experiments, *p < 0.05 for control versus E2, ⁺p < 0.05 for E2 versus E2 + UV. (B) Time course of MnSOD activity. MCF-7 cells were exposed to UV ± E2 and activity from discrete wells of cells was determined every 10 min for 1 h. Each data point is the mean of quintuplicate replicates, the study repeated a second time. (C) ER mediates E2 stimulation of MnSOD activity. MCF-7 cells or isolated mitochondria were exposed to brief UV and then incubated with 10 nM E2 in the presence or absence of 1 µM ICI182780, for 20 min (left) or 4 h (right). The bar graphs represent three experiments combined. *p < 0.05 for control versus E2, ⁺p < 0.05 for E2 versus same + either UV or ICI182780. Also shown is an immunoblot of MnSOD protein over 4 h in isolated mitochondria. (D) Left, validation of siRNA knockdown of MnSOD protein. Western blot for MnSOD or actin occurred 48 h after transfection of MCF-7 cells with either siRNA to MnSOD or GFP (control). Right, MCF-7 were transfected and recovered and then exposed to UV ± 10 nM E2. ROS were measured 4 h later and the data are from three combined experiments. *p < 0.05 for control versus UV, ⁺p < 0.05 for UV versus UV + E2, ⁺⁺p < 0.05 for UV + E2 versus same plus siRNA to MnSOD.

ROS Signals to JNK and PKC ${delta}$ Activation
E2 prevents UV radiation and taxol chemotherapy from inducingapoptotic breast cancer cell death in part by inhibiting JNKactivity through undetermined mechanisms (Razandi et al., 2000

).Here we found that UV-induced activation of JNK was substantiallyinhibited by all the antioxidants, especially Mito-Q (Figure 6A).The results implicate mitochondrial ROS as the critical regulatorof UV-induced JNK activation and suggest that E2 inhibitionof ROS shown here underlies the inhibition of kinase activity(Razandi et al., 2000

). We then asked whether JNK activationcontributes to mitochondrial apoptosis events. A specific inhibitorof JNK1 activity, SP 600125, partially prevented UV-inducedcytochrome C release into cytoplasm (Figure 6B) and also significantlyblocked UV-induced loss of mitochondrial membrane potential(unpublished data).

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Figure 6. Role of JNK in UV-induced cell death. (A) MCF-7 cells were exposed to UV in the presence of absence of Mito-Q, and JNK activity was determined sequentially over a 4-h period. The top panel shows the 30 min time point. A representative study is shown, repeated once. (B) Cells were briefly exposed to UV ± SP 600125, a JNK-1 inhibitor, the latter continued for 4 h. Cytochrome C in the cytoplasm was determined by Western blot, and the study was repeated.

Another important mediator of apoptosis in many cell insultmodels is the novel PKC isoform, PKC ${delta}$ (Steinberg, 2004). Thisisoform translocates to mitochondria in response to H₂O₂, whereit participates in the mitochondrial program of apoptosis (Majumderet al., 2001). By comparison, PKC ${epsilon}$ in some cell types contributesto cell survival (McJilton et al., 2003; Murriel and Mochly-Rosen,2003). We determined whether these PKC isoforms contributedto cell fate in MCF-7. After 30 min and persisting for 4 h,UV strongly activated PKC ${delta}$ , noted as tyrosine 311 phosphorylation(Figure 7A). E2 strongly inhibited this activation. Furthermore,UV-activated PKC ${delta}$ was significantly dependent on ROS (Figure 7B).We also determined PKC ${delta}$ activity, using a PKC substrate peptide(from glycogen synythase kinase; Figure 7C). We found that UVstimulated, whereas E2 prevented PKC ${delta}$ activation by UV. In contrast,PKC ${epsilon}$ phosphorylation and activity were stimulated at 4 h by E2but not by UV (Figure 7, A and C). Therefore, the two PKC isoformscould be differential mediators of cell fate in our system.

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Figure 7. PKC isoforms and cell fate. (A) Whole MCF-7 cells were exposed to brief UV ± E2, and then PKC ${delta}$ activity was determined with phospho-specific antibody to tyrosine 311 (activation site) at 30 min and 4 h, during the presence or absence of sex steroid. PKC ${epsilon}$ activity (serine 729 phosphorylation) was similarly determined. The study was repeated a second time, while specific PKC proteins were determined using separate antibodies to the PKC isoforms. (B) Cells were exposed to UV in the presence or absence of Mito Q and PKC ${delta}$ activity was determined. A representative experiment of three and total PKC ${delta}$ protein is shown is shown. (C) PKC isoform activity. MCF-7 were incubated with 10 nM E2 in the absence or presence of UV exposure, the cells were lysed, and PKC ${delta}$ or ${epsilon}$ protein was immunoprecipitated and then utilized for an in vitro activity assay using appropriate substrate. Data are from a single study, repeated once. Total PKC protein is shown as a loading control. (D) MCF-7 were transfected with 2.5 µg of siRNA to either PKC $beta$ , ${delta}$ , or ${epsilon}$ , and Western blotting for PKC ${delta}$ (left) and PKC ${epsilon}$ (right) occurred 48 h later. (E) Cells were transfected to express the various siRNAs, and experiments occurred 48 h later. Left, transfected and recovered cells were exposed to UV, and cytochrome C in cytoplasm was determined 4 h later. Right, cells were exposed to UV ± E2 in the presence/absence of siRNAs, and cytochrome C was determined. Actin protein is expressed both as a specificity control for the effects of PKC knockdown and as a protein loading control. The studies were repeated a second time.

To support this, we investigated PKC functions in the modulationof cytochrome C release. To do this, we first validated thatspecific siRNAs for PKC ${delta}$ and PKC ${epsilon}$ knock down the intended targetproteins (Figure 7D). Importantly, the PKC control siRNA toPKC $beta$ had no effects on either the ${delta}$ or ${epsilon}$ isoforms. Silencing PKC ${delta}$ substantially prevented UV-stimulated cytochrome C concentrationin cytosol, limited by our transfection efficiency ( $~$ 65%; Figure 7E,left). The siRNA for PKC $beta$ had no effect in this regard. In contrast,silencing PKC ${epsilon}$ partially reversed the inhibition of cytochromeC localization by E2 (Figure 7E, right). Again, the siRNA forPKC $beta$ had no effect, and PKC ${epsilon}$ knockdown showed no influence onUV-induced cytochrome C release (in the absence of E2). Collectively,PKC ${delta}$ contributes to UV-induced cell death via the mitochondria,whereas PKC ${epsilon}$ specifically enables a cell survival-related actionof the sex steroid.

Bax Translocation and Oligomerization at the Membrane
In response to many death stimuli, the proapoptotic proteinBax translocates to the mitochondria, where it undergoes oligomerization/activationand insertion into the outer mitochondrial membrane (Gross etal., 1998; Dejean et al., 2005). Active Bax then promotes therelease of cytochrome C from the mitochondria into the cytoplasm,stimulating the formation of the apoptosome (Jurgensmeier etal., 1998). We determined whether UV and E2 oppose each otherin these regards. Under control conditions, Bax exists as amonomer in the cytosol of the MCF-7 cells (Figure 8A, lanes1 and 5). UV caused both the dimerization and translocationof Bax to the mitochondrial fraction (lanes 2 and 6), significantlyprevented by E2. Antioxidants prevented UV-induced translocationof Bax to the mitochondria (Figure 8B) and the PKC ${delta}$ inhibitorrottlerin, substantially inhibited UV-induced Bax translocation(Figure 8C). JNK activation by UV also contributed, becausethe specific inhibitor of JNK1 activity, SP 600125, partiallyblocked Bax translocation to the mitochondria. Thus, the signalingthat results from mitochondrial ROS formation leads to Bax participationin mitochondrial apoptosis, the inhibition of which providesa mechanism for E2 survival effects (Figure 8D).

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Figure 8. Bax translocation to mitochondria (A) MCF-7 cells were exposed to UV ± E2. Bax localization and structure in cytosol and mitochondrial fractions were determined by Western blot using a specific antibody that detects BAX dimerization. The study was repeated two additional times. (B) MCF-7 cells were exposed to brief UV ± Mito-Q, NAC, or Rotenone for 4 h. Bax localization was then determined. The studies were repeated three times and the band intensity data were combined for the bar graph. *p < 0.05 for control versus UV, ⁺p < 0.05 for UV versus same + antioxidant. (C) MCF-7 were exposed to UV ± 10 µM SP 600125 (JNK 1 inhibitor), or 5 µM Rottlerin (PKC ${delta}$ inhibitor). The representative study was repeated. (D) Cartoon of estrogen action at mitochondria to prevent apoptosis.

DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

ER exist in the cytoplasm of many cells. However, it is unclearwhether cytoplasmic receptors simply serve as a reservoir, awaitingsignals for translocation to the nucleus or whether they functionas a distinct pool. Previous studies suggested that estrogenimpacts mitochondrial processes, perhaps underlying observeddifferences in the function of mitochondria from males and females(Borras et al., 2003). Estrogen effects in the cell, however,might result from nuclear (or plasma membrane) actions of E2/ERindirectly impacting mitochondrial function (Wang et al., 2003).Further, reports of mitochondrial actions of estrogen oftenutilized micromolar steroid concentrations, and so the physiologicalsignificance was unclear (Kipp and Ramirez, 2001; Morkunieneet al., 2002).

Here, we provide evidence that ER ${alpha}$ and ER $beta$ are present in themitochondria of two different target cells for E2 action. InEC, both ER ${alpha}$ and ER $beta$ exist predominantly in the nucleus, withsome enrichment of ER ${alpha}$ (compared with ER $beta$ ) in mitochondria. Incontrast, ER ${alpha}$ is localized mainly to the nucleus of MCF-7 cells,and ER $beta$ is highly enriched in the mitochondria. These studiesextend the findings of Chen et al. (2004), who reported thatboth ER isoforms are in the mitochondrial matrix of MCF-7, byimmunogold labeling and electron microscopy. Other reports suggestthat ER are present in the mitochondria of cardiomyocytes (Morkunieneet al., 2002; Yang et al., 2004), but this has been challengedin these cells (Forster et al., 2004). Recently, ER ${alpha}$ was identifiedin mitochondrial fractions from whole cerebral blood vessels(Stirone et al., 2005). Importantly, we find that mitochondrialER (and all cellular ER) are absent in EC isolated from combinedER ${alpha}$ /ER $beta$ knockout mice. This novel finding indicates that mitochondrialER are derived from the same genes that code for nuclear ER ${alpha}$ and ER $beta$ .

Most importantly, we establish the first clear functions ofmitochondrial ER potentially impacting breast cancer cell survival.Breast cancer cells expressing the mitochondrial-targeted Edomain of ER ${alpha}$ largely do not undergo several components of mitochondrialcell death (Kroemer, 2003). Interestingly, cells expressingplasma membrane–targeted E domain also show these cellsurvival actions of E2. As a G-protein–coupled receptor(Levin, 2005), the membrane-localized pool of ER might signalto the mitochondria. In this regard, PI3K activation by membraneER contributes to breast cancer cell survival (Marquez and Pietras,2001; Fernando and Wimalasena, 2004; Razandi et al., 2004b),and PI3K and AKT suppress both Bax translocation to the mitochondria(Tsuruta et al., 2002) and subsequent release of cytochromeC (Jurgensmeier et al., 1998). We find that in cells expressingthe E domain of ER ${alpha}$ targeted to the cell membrane, wortmannin,a PI3 kinase inhibitor, partially reverses E2 prevention ofcytochrome C release (unpublished observations). This suggestsa cross-talk from membrane ER impacting mitochondria and cellviability.

In contrast, cells expressing a nuclear-targeted E domain ornuclear-targeted whole ER ${alpha}$ do not support these cell survivalactions. Nuclear ER importantly contribute to the long-termprotection against cell death by transcribing antiapoptoticgenes such as Bcl-2 (Dong et al., 1999). Shown here, the mitochondrialpool of ER blocked UV-induced cytochrome C release from mitochondriaat 30 min postradiation. Earlier mitochondrial events of apoptosiscan occur as rapidly as 10 min after insult, with cells dyinghours to days later (Green, 2005). Because the majority of ourcells undergo apoptosis by 4–6 h post-UV exposure, thetiming of our experiments is relevant.

We report that mitochondrial death/survival events in this settingare dependent on ROS formation. Specific compounds that preventROS formation from mitochondrial respiratory complexes (Kelsoet al., 2001; Sato et al., 2005) almost completely reverse UV-inducedapoptosis. E2 up-regulated the activity of MnSOD, the SOD thatonly exists in mitochondria, and silencing MnSOD reversed E2-inhibitionof ROS generation. Importantly, up-regulation of dismutase activityby E2 in isolated mitochondria and whole cells was comparableand rapid (10–20 min). This indicates that mediation ofMnSOD activity by E2 occurs mainly via mitochondrial ER. Preciselyhow this receptor pool signals to MnSOD activity requires furtherinvestigation of this novel finding. E2 also stimulates thetranscription of the MnSOD gene in other cell systems (Strehlowet al., 2003), prevented by ICI182780 and dependent on ERK MAPkinase (Borras et al., 2005). We did not see significant changesin MnSOD protein in the mitochondria during the more limited,4 h of E2 incubation with the cells.

What signals downstream of ROS mediate mitochondrial cell death?We found that ROS generated by UV induced PKC ${delta}$ and JNK activitiesand E2 prevented this. PKC ${delta}$ protein knockdown 1) partially preventedBax translocation and oligomerization at the mitochondria and2) prevented cytochrome C release and MCF-7 cell death. PKC ${delta}$ overexpression contributes to apoptosis through associationof the kinase with and modification of proapoptotic BCL-2 familymembers (Brodie and Blumberg, 2003; Murriel and Mochly-Rosen,2003). In contrast, PKC ${epsilon}$ has been implicated in the survivalof cardiomyocytes (Gray et al., 2004), prostate (McJilton etal., 2003), and lung cancer (Ding et al., 2002). Here we reportthe involvement of PKC ${epsilon}$ in breast cancer cell survival inducedby E2, limiting cytochrome C release. Further studies will beneeded to delineate the precise functions of this kinase.

We also found that UV-induced ROS lead to JNK activation, JNKpromoted Bax translocation and dimerization at the mitochondria,and E2 prevented each of these linked events. Radiation, chemotherapy,and tamoxifen activate JNK, contributing to breast cancer apoptosis(Mandlekar and Kong, 2001; Mingo-Sion et al., 2004). ROS up-regulatesJNK kinase activity by blocking JNK phosphatase function (Kamataet al., 2005). Others (Tsuruta et al., 2004) and we could notshow that Bax is directly phosphorylated by this mitogen-activatedprotein kinase. Tsuruta et al. (2004) recently determined thatJNK phosphorylates the 14-3-3 proteins that sequester BAX inthe cytoplasm, releasing Bax to translocate to the mitochondriawhere it undergoes oligomerization and inserts into the mitochondrialmembrane. This promotes pore formation and the release of cytochromeC into the cytoplasm (Jurgensmeier et al., 1998). Inhibitionof ROS-induced JNK provides a second mechanism by which E2 preventsBax involvement in mitochondrial death.

Which mitochondrial ER isoform mediates E2 effects? Specificagonists for either ER ${alpha}$ or ER $beta$ inhibited UV-induced cytochromeC release from isolated mitochondria; the ER $beta$ agonist was morepotent. In addition, targeting of the ER ${alpha}$ E domain only to themitochondria supported several cell survival functions of E2.Thus, both receptor isoforms appear to contribute to sex steroidaction in this organelle. Consistent with this, ER ${alpha}$ or ER $beta$ agonistsprevented UV-induced cell death, and steroid specificity wasshown in that neither progesterone nor testosterone affectedcell fate through mitochondria. Our results also suggest thatthe ligand binding/AF-2 region (E) is a functional domain forthis pool of ER ${alpha}$ .

Mitochondrial-generated ROS production may contribute to oncogenesisbecause cancer-causing mutations in mitochondrial DNA up-regulateROS formation (Petros et al., 2005). When produced in smallamounts, ROS can serve as a proliferation-related signalingmechanism (Preston et al., 2001). As recently reported, E2-inducedG1/S progression in breast cancer may in part be related tothis mechanism (Felty et al., 2005), a mechanism well describedfor signaling by many growth factor tyrosine kinase receptors(Aslan and Ozben, 2003). In contrast, adjuvant therapies forbreast cancer generate large amounts of ROS, essential to theinduction of cell death (Benhar and Levitzki, 2002). Directprevention by E2/ER of excessive mitochondrial ROS formationis a novel mechanism to prevent apoptotic cell death. Thus,it is the balance of ROS that mediates important aspects ofcarcinogenesis and provides a therapeutic target to alter tumorbiology.

ACKNOWLEDGMENTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

This work was supported by grants from the Research Serviceof the Department of Veteran's Affairs and the National Institutesof Health (CA-100366) to E.R.L.

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E05–11–1013)on February 22, 2006.

Abbreviations used: ER, estrogen receptor; ERK, extracellular-regulatedprotein kinase; JNK, c-Jun N-terminal kinase; MnSOD, manganesesuperoxide dismutase; PKC, protein kinase C; ROS, reactive oxygenspecies.

Address correspondence to: Ellis R. Levin (ellis.levin{at}med.va.gov).

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