Equol increases cancer potential via c-Myc upregulation

نویسندگان

  • Columba de la Parra
  • Luis D. Borrero-Garcia
  • Ailed Cruz-Collazo
  • Robert J. Schneider
  • Suranganie Dharmawardhane
چکیده

Epidemiological studies implicate dietary soy isoflavones as breast cancer preventives, especially due to their anti-estrogenic properties. However, soy isoflavones may also have a role in promoting breast cancer, which has yet to be clarified. We previously reported that equol, a metabolite of the soy isoflavone daidzein, may advance breast cancer potential via upregulation of the eukaryotic initiation factor 4GI (eIF4GI). In estrogen receptor negative (ER-) metastatic breast cancer cells, equol induced elevated levels of eIF4G which were associated with increased cell viability and the selective translation of mRNAs that use non-canonical means of initiation, including internal ribosome entry site (IRES), ribosome shunting, and eIF4G enhancers. These mRNAs typically code for oncogenic, survival, and cell stress molecules. Among those mRNA’s translationally increased by equol was the oncogene and eIF4G enhancer, c-Myc. Here we report that siRNA-mediated knockdown of cMyc abrogates the increase in cancer cell viability and mammosphere formation by equol, and results in a significant downregulation of eIF4GI (the major eIF4G isoform), as well as reduces levels of some, but not all, proteins encoded by mRNAs that are translationally stimulated by equol treatment. Knockdown of eIF4GI also markedly reduces an equol-mediated increase in IRES-dependent mRNA translation and the expression of specific oncogenic proteins. However, eIF4GI knockdown did not reciprocally affect c-Myc levels or cell viability. This study therefore implicates c-Myc as a potential regulator of the cancer promoting effects of equol via upregulation of eIF4GI and selective initiation of translation on mRNAs that utilize noncanonical initiation, including certain oncogenes. http://www.jbc.org/cgi/doi/10.1074/jbc.M114.617415 The latest version is at JBC Papers in Press. Published on January 15, 2015 as Manuscript M114.617415 Copyright 2015 by The American Society for Biochemistry and Molecular Biology, Inc. by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 2 INTRODUCTION Isoflavones are found in nutritionally relevant amounts in soybeans comprising ~3.5 mg/gm soy protein in traditional soy foods. Studies have reported a range of 1-25 μM soy isoflavones in the human circulation following consumption of soy products, which is sufficient for physiological activity (1-4). Due to the structural similarity to 17β estradiol, these phytoestrogens have been extensively studied for their potential estrogenic or antiestrogenic effects in breast cancer (5;6). Moreover, soy isoflavones may have additional estrogen-independent effects in aggressive ERbreast cancers (5;7). Daidzein is the second most prominent isoflavone in soy and approximately 70% of daidzein can be metabolized by the intestinal microflora to the metabolite equol (8). Only ~3050% of humans have the gut microflora necessary to convert daidzein to equol (8;9); therefore, not all humans are affected by equol. Equol is also chemically similar to estrogen and has 80 times more ERβ affinity than daidzein (10-12). The effects of equol, specifically in ERbreast cancers, or established aggressive breast cancers, remains unclear and requires additional study (7;8;13;14). At high concentrations (50-350 μM), equol has been implicated in inhibition of cancer cell growth, invasion, tumor progression, and cancer risk (15-19), while low physiological concentrations of equol reportedly increases cancer cell proliferation (14;20). In ER+ human breast cancer cells, equol increases estrogenic activity and cell proliferation, but does not affect tumor growth in mice (20-23). Dietary daidzein also failed to reduce mammary tumor growth in rats when metabolized to ~1μM equol in serum (24), although others have shown inhibitory effects of daidzein and equol on ER+ breast cancer cells and tumors (25;26). Thus, whether daidzein and equol prevents or promotes breast cancer in experimental models is not established, and may be concentration and ER status dependent. Accordingly, the molecular mechanisms by which equol acts on breast cancer cells need to be better understood, enabling recommendations for soy consumption in breast cancer patients. To this end, we previously tested the effect of individual and combined soy isoflavones on immune impaired (nude) mice with mammary tumors, established from ERcancer cells. We reported that dietary daidzein increases mammary tumor growth and metastasis (27). These findings support our recent in vitro studies which demonstrated that equol is the active metabolite of daidzein and increases breast cancer cell malignancy, primarily via upregulation of the eukaryotic initiation factor eIF4GI and its translation of mRNA encoding oncogenic proteins (28). Translational control has received increased attention in recent years due to its emerging significance in cancer development and progression (29). Translation initiation is typically the rate-limiting step and therefore, a primary site for regulation. Accordingly, the levels of two eukaryotic initiation factors that are members of the cap-initiation eIF4F complex, consisting of eIF4E (Cap binding protein) and eIF4G (initiation complex molecular scaffold), are frequently elevated in human cancers, and have been associated with poor prognosis and outcome (2931). Overexpression of eIF4GI is critical for the modes of translation initiation in eukaryotic cells that bypass or have a reduced requirement for eIF4E, including IRES-dependent mechanisms that allow the 40S ribosome to be directly recruited to the mRNA (32;33). It is thought that under the physiological stress conditions that exist in large tumors (i.e., growth arrest, amino acid starvation, hypoxia), cancer cells rely on noncanonical, eIF4E deficient, IRES-dependent translation of a subset of mRNAs encoding progrowth, pro-angiogenic and pro-survival proteins, such as, BCL2, Bcl -Xl, c-Myc, p120 catenin, and vascular endothelial growth factor A (VEGF) A, among others (29;34-36). In our recent study using MDA-MB 435 ERmetastatic breast cancer cells treated with equol, we showed that the transcription factor c-Myc was also elevated in addition to upregulated levels of eIF4GI and the increased translation of IREScontaining mRNAs that control cell survival and cell proliferation (28). This result is relevant because c-Myc is overexpressed in a variety of human cancers and plays an important role in multiple signaling pathways including cell growth, cell proliferation, metabolism, ribosome biogenesis, microRNA regulation, cell death, and cell survival (37-39). With the objective of determining whether the equol-mediated upregulation of eIF4G promotes by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 3 preferential synthesis of c-Myc, which has an IRES element (40), or whether c-Myc upregulation by equol leads to eIF4GI transcription, as shown in (41), we investigated the effects of silencing eIF4GI or c-Myc in equoltreated metastatic breast cancer cells. Here, we show that reducing eIF4GI levels results in a marked reduction in IRES dependent mRNA translation, decreased polysomal association of those mRNAs, and corresponding oncogenic protein levels of specific IRES-containing mRNAs. The increase in cell viability and mammosphere formation (an indicator of tumorigenic potential (42;43)) in response to equol was not affected until c-Myc was also targeted by siRNA, which in addition, significantly downregulated eIF4GI levels. Taken together, these data implicate c-Myc, and the consequent increase in eIF4GI followed by selective translation of oncogene mRNAs, in the pro-transforming effects of equol on breast cancer progression. EXPERIMENTAL PROCEDURES Cell culture – Metastatic variant of MDA-MB-435 (ER−) (gift of Dr. Danny Welch, The University of Kansas Cancer Center) and Hs578t (ER−) metastatic human breast cancer cells (American Type Culture Collection (ATCCC), Manassas, VA) were maintained in complete culture medium: Dulbecco’s Modified Eagle Medium (DMEM, Invitrogen, Houston, TX) supplemented with 10% fetal bovine serum (Invitrogen, Houston, TX) at 37°C in 5% CO2. The MCF-10A mammary epithelial cells (ATCCC) were maintained in DMEM supplemented with 10% horse serum, EGF, hydrocortisone, cholera toxin, and insulin, as described previously (44). Cell lines were authenticated and found to be mycoplasma free. Cell treatment – Quiescent mammary epithelial cells or metastatic cancer cells were treated with 0 (vehicle, 0.1% DMSO) or 25 μM of (R,S) Equol (LC Laboratories, Woburn, MA) in DMEM and 5% FBS media for 24 h. Western blotting – Cells were lysed and western blotted, as described in (27). Primary antibodies to eIF4E, eIF4GI, c-Myc, p120 catenin, Bcl-Xl, Cyclin-D1, GAPDH, JunB and β-actin proteins (Epitomics, Burlingame, CA, Cell Signaling, Danvers, MA, Sigma-Aldrich Comp., St Louis, MO) were used. The integrated density of positive bands was quantified using Image J software, as described in (27). Cell viability assay – Cell viability was determined by the CellTiter 96 Non-Radioactive Cell Proliferation kit according to manufacturer instructions (Promega, Madison, WI). Briefly, quiescent 1 x 10 MDA-MB-435 cells were added to each well of a 96-well plate and treated for 24 h with vehicle or 25 μM equol. Following equilibration, 15 μL/well of MTT (3-(4,5-dimethyl thiazol-2-yl)-2,5-diphenyl tetrazolium bromide) reagent was added and the plates incubated at 37°C for 4 h. Stop solution (100 μL) was added to each well, and the plates incubated to facilitate solubilization of newly formed formazan salts. The absorbance at 570 nm was measured using an ELISA plate reader. Real-Time reverse transcriptase polymerase reaction (RT-PCR) analysis – Real-time quantitative RT-PCR analysis was performed as described (28). Briefly, total RNA was extracted using the Qiagen RNeasy Kit (Qiagen, Valencia, CA). RNA concentration was detected using NanoDrop (NanoDrop Technologies,Wilmington, DE). RNA (0.5 μg) was used to synthesize cDNA using the iScript cDNA synthesis kit (Bio-Rad, Hercules, CA). RTPCR primers were as follows. MYC: forward, 5’TTCTCAGAGGCTTGGCGGGAAA-3’, reverse, 5’ TGCCTCTCGCTGGAATTACTACA-3’. B2microglobulin (B2M): forward, 5’GGCTATCCAGCGTACTCCAAA-3’, reverse, 5’CGGCAGGCATACTCATCTTTTT-3’. GAPDH: forward, 5’TTGCCATCAATGACCCCTTCA 3’, reverse, 5’CGCCCCACTTGATTTTGGA-3’. CCND1: forward, 5’TGGTGAACAAGCTCAAGTGGA3’. reverse, 5’ TGATCTGTTTGTTCTCCTCCGCCT-3’. eIF4GI: forward, 5’TTGTGGATGATGGTGGCT-3' reverse, 5’TTATCTGTGCTTTCTGTGGGT-3’. CTNND1: forward, 5’-TCCAGCAAACGATACAGTGG3’, reverse, 5’-GAACCACCTCTGGCTGAAAT-3’. Real-time reactions were performed using iQSYBR-Green PCR Master Mix (Bio-Rad, Hercules, CA). The amplification reaction was by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 4 performed for 40 cycles (10s at 95 °C, 30s at 59°C, and 30s at 72 °C). B2M mRNA was used as an internal control. The fold change was determined by the 2 ΔΔCT method as described (27;28). Polysome fractionation– MDA-MB-435 cells (non-silencing control or eIFGI silenced), treated with vehicle or equol, were used for polysome profiling, as described in (36). Cells were pretreated with 100 μg/ml cycloheximide (Calbiochem), washed twice in PBS with 100 μg/ml cycloheximide, pelleted, and resuspended in 700 μl polysome isolation buffer (200 mM Tris, pH 7.5, 100 mM NaCl, and 30 mM MgCl 2 ). After 5 min incubation, 250 μl detergent buffer (1.2% Triton, 0.2 M sucrose in polysome isolation buffer) was added and cells were lysed. Clarified lysates were layered onto 10–50% sucrose gradients (Sigma-Aldrich) and sedimented at 36,000 rpm for 2 h in a SW40 rotor (Beckman Coulter) at 4°C. Gradients were collected as 15 × 750 μl fractions, by pumping 60% sucrose into the bottom of the gradient and collecting from the top using an ISCO fraction collector while simultaneously monitoring absorbance at 254 nm. RNA was isolated by extraction with phenol/chloroform. Fractions 4–12, representing polysomes, were pooled and classified as light polysome fractions (2-3 ribosomes) and heavy polysome fractions (≥ 4 ribosomes). RNA preparations from each fraction were subjected to qRT-PCR for c-MYC, CTNND1 (p120-catenin), CCND1 (cyclin D1), eIF4G, GAPDH and B2M, as described above. shRNA/siRNA transfection– eIF4GI using shRNA adenovirus (Ad) vectors were conducted as described (36). MDA-MB-435 and Hs578t cells were infected with Ad vectors twice over four days with nonsilencing (NS control) or eIF4GIsilencing (Ad) shRNA vectors at a multiplicity of infection (MOI) of 100, then treated with vehicle or 25 μM equol for 24 h. Control or c-Myc siRNAs (Santa Cruz, CA) were transfected into MDA-MB-435 and Hs578t cells using lipofectamine (Invitrogen) according to manufacturer instructions, followed by treatment with vehicle or equol for 24 h. IRES-dependent protein synthesis – MDA-MB435 cells with non-silencing control or eIF4GI siRNA were transfected with a bicistronic reporter or control plasmid containing the luciferase constructs without an IRES, using Lipofectamine 2000 (Invitrogen), as per manufacturer directions. As described (36), this plasmid contains a capdependent Renilla luciferase (RLuc) followed by a 5’UTR containing the p120 catenin IRES driving a firefly luciferase (FLuc). 24 h following transfection, cells were treated with equol for an additional 24 h. Relative IRES activity was analyzed as 570 nm FLuc/480 nm RLuc in a luminometer using a dual luciferase assay kit (Promega, Corp., Madison, WI), according to manufacturer instructions. Mammosphere formation assay ˗ Mammosphere assays were performed, as described in (42). MDA-MB-435 cells were seeded in ultra-low attachment plates (Corning) at a density of 5005000 cells/well in serum-free mammary epithelium basal medium (Lonza) supplemented with 1% penicillin/streptomycin (Lonza), B27 supplement minus vitamin A (50X, Gibco), 5 μg/mL insulin (Gibco), 1μg/mL hydrocortisone (Sigma), 20 ng/mL EGF, and 20 ng/mL fibroblast growth factor (Sigma). Mammospheres were counted using an inverted microscope after 3 days of incubation in 37 ̊C, 5% CO2. Mammosphere forming efficiency (MFE) was calculated as the number of mammospheres divided by the number of cells seeded per well and is expressed relative to cells expressing control siRNA treated with vehicle. Statistical analysis– Data was analyzed and reported as mean ± SEM of at least three independent experiments. Statistical analyses were conducted using Microsoft Excel. Differences between means were determined using Student tTest and values p≤0.05 or p≤0.01 were considered significant. RESULTS eIF4GI silencing partially rescues the pro-cancer effects of equol We recently reported that the daidzein metabolite equol, through the up-regulation of eukaryotic protein synthesis initiation factor eIF4GI, may specifically direct the synthesis of IRES-containing mRNAs that induce cell survival by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 5 and proliferation, and increase cancer progression. In the previous study, we used 0, 1, 5, 25, or 50 μM equol and reported that the effects of equol on cell viability and upregulation of oncogenic protein expression saturated at 25 μM equol (28). Therefore, the present study was conducted with 25 μM equol, using two metastatic cancer cell lines. To investigate whether equol regulates breast cancer cell malignancy via eIF4GI, we determined the effects of equol on MDA-MB-435 and Hs578t cells with eIF4GI knockdowns. Using eIF4GI shRNA vectors, eIF4GI protein expression was silenced by ~60%, compared to cells expressing non-silenced vector controls, in both vehicle and equol-treated MDA-MB-435 and Hs578t cells (Fig. 1A). Notably, the ~1.8-fold increase in eIF4GI mRNA levels in response to equol treatment was effectively abolished by the eIF4GI targeting, resulting in a 3-fold reduction in eIF4GI mRNA in the presence and absence of equol (Fig. 1 C). Since equol upregulates expression of IRES containing oncogenic proteins (28), cells expressing control or eIF4GI knockdown were analyzed for protein expression levels of members of the eIF4F complex, as well as proteins from IRES containing mRNAs (Fig. 1 A,B). At 25 μM, equol protein expression in Hs578t and MB-435 cells, respectively increased levels of eIF4GI (~1.4, 1.6-fold), c-Myc (~1.5, 1.8-fold), Cyclin D (~1.4, 1.5-fold), Bcl-Xl (~1.3, 1.5-fold), and p120 catenin (~1.3, 1.6 fold) in a statistically significant manner, compared to control shRNA-expressing cells. Cells expressing eIF4GI shRNA demonstrated a ~50% reduction in eIF4GI in vehicle treatments and an 80~120% reduction in equol-treated cells, while the eIF4E levels remained unchanged. Knockdown of eIF4GI also caused a marked ~40-60% reduction in expression levels of proteins encoded by mRNAs with IRESs: Cyclin D, Bcl-Xl, and p120 catenin, from both vehicle and equol treated cells. Protein expression of GAPDH, JunB and Actin from mRNAs with short 5’UTRs lacking an IRES were not affected by equol treatment or eIF4GI silencing. These results suggest that elevated eIF4GI levels are essential for the significant and selectively increased level of translation of IRES-containing cancer promoting mRNAs, in response to equol treatment. Interestingly, the equol-mediated ~1.7fold increase in c-Myc, a reported IRES containing mRNA, remained elevated regardless of the eIF4GI knockdown (Fig. 1). The reason for sustained c-Myc expression is unknown but may reflect an ability to use other eIF4GI homologs such as DAP5 (45), or contribution from eIF4Emediated cap-dependent protein synthesis. To determine whether silencing eIF4GI alters transcriptional activity of the mRNAs examined in Figure 1, we quantified the mRNA levels of eIF4GI, C-MYC, CTNND1 (p120) and CCND1 (CyclinD) in MDA-MB-435 cancer cells expressing control or eIF4GI shRNAs, treated with vehicle or 25 μM equol. Figure 1C demonstrates that as previously reported by us from MDA-MB-435 mammary tumors and cells (27;28), equol increased eIF4GI transcription by ~1.8-fold. This increase was abolished in cells expressing eIF4GI shRNA, where eIF4GI expression was reduced by ~3-fold in both vehicle and equol-treated cells. The mRNA levels of CTNND1 (p120) and CCND1 (CyclinD1) were not affected by equol treatment or eIF4GI knockdown, indicating that cyclin D1 and p120 catenin expression were regulated entirely at the translational level. However, c-Myc mRNA levels increased almost 2-fold in response to equol in both control and eIF4GI silenced cells, confirming that the equol-mediated upregulation in c-Myc protein levels is independent of eIF4GI (Fig 1). As previously reported, in metastatic cancer cells, equol at 1, 5, 10, 25, or 50 μM increased cMyc protein and mRNA expression by 2-fold (28) (Fig 2 A). However, the immortalized but nontransformed mammary epithelial cell line MCF10A did not demonstrate statistically significant changes in c-Myc protein expression in response to equol treatment at 5 or 25 μM (Fig. 2 B,C). Therefore, the equol-mediated upregulation of cMyc appears to be limited to transformed cancer cells. To determine whether the elevated levels of eIF4GI as found in highly transformed cells in response to equol treatment might be necessary for efficient translation of IRES-containing mRNAs, we performed dual luciferase assays that measure both cap-dependent and p120 catenin IRESdependent protein synthesis in MDA-MB-435 cells expressing control or eIF4GI shRNA, treated with vehicle or equol. Data shown in Figure 3 demonstrates that equol increased IRES-dependent by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 6 mRNA translation in cells expressing control shRNA by ~1.7-fold, while this increase was reduced by half when eIF4GI was silenced, effectively abolishing the effect of equol. Vehicle treatment of cells with eIF4GI knockdown did not statistically decrease IRES activity (data not shown). Thus, the elevated protein synthesis of mRNAs with IRESs can be attributed to the increased levels of eIF4GI in response to equol. To investigate whether translation initiation is sensitive to the reduction in eIF4GI levels, we performed polysome profiling for control and eIF4GI-silenced MDA-MB-435 cells treated with vehicle or equol. The ribosome content on mRNA is an established surrogate for translation activity. As previously reported (28), figure 4A shows that equol increased the total mRNA associated with the polysomal fractions compared with vehicle alone, a manifestation of increased eIF4GI levels. In equol-treated MDA-MB-435 cells with eIF4GI knockdown, total RNA associated with polysomes was only very slightly decreased, again indicative of a selective reduction in translation of specific mRNAs rather than a global decrease. As expected in vehicle treated cells, in the absence of equol, eIF4GI knockdown resulted in a general decreased association of RNA with both light and heavy polysomal fractions. To identify specific mRNAs differentially associated with polysome fractions in control or eIF4GI silenced cells, real-time quantitative (q) RT-PCR was performed to measure IREScontaining mRNAs: CTNND1, CCND1, EIF4G, C-MYC, and the non-IRES containing housekeeping genes GAPDH and B2M. Figure 4B demonstrates that in MDA-MB-435 cells expressing control shRNA, equol treatment increased the association of eIF4GI with both light and heavy polysomal fractions (~1.7-fold), while the association of C-MYC, CTNND1, and CCND1 with the heavy polysomal fraction was increased by ~1.5-1.8-fold. Equol therefore promoted a greater increase in the translation of these mRNAs by increasing their polysome content, a hallmark of increased initiation. In the MDA-MB-435 cells expressing eIF4GI shRNA, a ~2.5-fold reduction in eIF4GI levels was reflected in decreased polysome association of CTNND1 and CCND1, by ~1.2 fold in the light fractions and by ~1.4 fold in the heavy fractions. However, the equolstimulated C-MYC mRNA levels remained increased by 1.4 and 1.7 fold in the light and heavy fractions compared with vehicle controls, even in the cells with eIF4GI knockdown. The IRES-negative GAPDH mRNA was also not affected by eIF4GI silencing or equol treatment. These data are consisted with the protein abundance levels shown earlier under identical conditions. The observed down-regulation of equol-mediated CyclinD and p120 catenin protein expression (Fig. 1A, B) and decreased polysome association of their mRNAs in cells silenced for eIF4GI (Fig. 4B), indicates a dependence on increased eIF4GI abundance to enable preferential translation of some IRES-containing mRNAs in equol-treated cells. c-Myc knockdown reduces eIF4GI levels and abrogates the effects of equol on cell viability and mammosphere formation Our results show that equol upregulates mRNA and protein levels and the polysomal association of the key transcription factor and oncogene c-Myc, independent of eIF4G (Figs.1, 4). Therefore, we tested the effect of reducing cMyc expression in Hs578t and MDA-MB-435 cells to investigate the importance of its elevated expression in equol action. To achieve this, cellular c-Myc levels were only partially reduced by carefully titrated c-Myc siRNA. This strategy enabled us to specifically determine the physiological relevance of elevated c-Myc in response to equol. Cells transfected with c-Myc siRNA demonstrated a ~40% reduction in c-Myc protein expression compared to control siRNA cells. The 1.5-fold increase in equol-mediated cMyc protein expression in cells expressing the control siRNA was completely abolished in both Hs578t and MDA-MB-435 cells expressing c-Myc siRNA. This result indicates that the siRNA targeting of c-Myc is sufficient to inhibit the de novo protein synthesis of c-Myc in response to equol, without affecting its basal levels (Fig. 5A). Protein expression of eIF4GI and cyclin D were both also significantly downregulated in c-Myc silenced cells, indicating that increased c-Myc abundance promotes increased eIF4GI mRNA expression by c-Myc. Interestingly, the levels of Bcl-Xl and p120 catenin proteins were not altered by c-Myc silencing. Rather, a statistically significant increase in Bcl-Xl and p120 catenin was demonstrated in response to equol in cells by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 7 with control or c-Myc siRNA in the MDA-MB435 cells. In the Hs578t cell line, protein expression of eIF4GI, cyclin D, and Bcl-Xl were downregulated following c-Myc knockdown, while p120 catenin expression remained unchanged. When eIF4GI was silenced, we observed a statistically significant decrease in p120 catenin and cyclin D1 expression while the other oncogenes tested, including c-Myc, remained unchanged. Therefore, to investigate the relative roles of eIF4GI and c-Myc on cell viability, Hs578t and MDA-MB-435 cancer cells expressing control, eIF4GI shRNA, or c-Myc siRNA were treated with vehicle or 25μM equol, and subjected to cell viability analysis by MTT assay. Although the increase in eIF4GI levels in response to equol was effectively abolished by eIF4GI siRNA targeting (Fig. 1), the 1.4-1.7 fold increase in cell viability in response to 25 μM equol remained constant in MDA-MB-435 and Hs578t cells, despite eIF4GI silencing (Fig. 6A). These results indicate that the equol effect on cell viability is not eIF4G dependent. In contrast, Figure 6B (Fig. 6B) demonstrates that knockdown of c-Myc reduced the viability of MDA-MB-435 cells by 50% in control treated cells and 50-80% in equol treated cells. To further investigate a role for c-Myc in regulating the effects of equol on cancer malignancy, non-adherent seeding of spheroids (mammosphere assays), which measure tumor initiating cell capacity, were performed in response to vehicle or equol using MDA-MB-435 cells expressing control or c-Myc siRNA. Our results show that equol increases the size and number of mammospheres formed by the MDAMB-435 cell line by 1.5-fold compared to controls. Knockdown of c-Myc expression (as determined by western blotting, data not shown) abolished the equol-mediated increase in mammosphere forming efficiency (Fig. 7). Therefore, the breast cancer promoting effects of equol appear to be dependent on its ability to increase c-Myc expression. DISCUSSION Dysregulation of translational control can have oncogenic consequences by altering global control of protein synthesis as well as selective translation of a subset of mRNAs important for cell growth, survival, metastasis and proliferation (29;46). Accordingly, eIF4F complex members eIF4E and eIF4GI are overexpressed in advanced cancers. Upregulation of eIF4GI in aggressive breast cancers may preferentially enhance capindependent and non-canonical means of initiation such as IRES-mediated translation; especially, when the cap-dependent scanning mechanism of translation initiation is compromised by stress conditions (47-49). Therefore, our finding that eIF4GI is upregulated by the dietary soy isoflavone equol in MDA-MB-435 human metastatic cancer cell tumors in immune-impaired mice, as well as in human metastatic breast cancer cells in vitro, has implicated the equol-stimulated eIF4GI in selective translational control (27;28). We also showed that equol treatment of breast cancer cells results in increased IRES-dependent mRNA translation, increased protein expression and increased polysome association of a number of mRNAs with IRES elements coding for proteins that regulate cancer cell survival, proliferation, and invasion (27). In this study, we tested the hypothesis that elevated levels of eIF4GI in response to equol contribute to breast cancer malignancy. As shown by our results comparing metastatic cancer cells and non-cancer cells, the increased cMyc and eIF4G expression in response to equol is a cancer cell-specific effect. This may be due to the complex deregulation of c-Myc expression in cancer that would be more responsive to the effects of equol (50). Our strategy in this study was to achieve only a partial silencing of eIF4GI levels in equol treated cells; thus, reducing it to levels found in untreated cells. In so doing, we found that the increased viability of metastatic cancer cells in response to equol was insensitive to eIF4GI knockdown. This result corroborates previous reports of eIF4GI depletion, which found only a small reduction in overall protein synthesis, cell viability, and only slightly impaired cell proliferation (35;36). Nevertheless, similarly partial eIF4GI silencing has been shown previously to decrease the translation of the IRES-containing mRNAs such as p120 catenin, which has been implicated in cancer cell invasion (36). Confirming this report, we found eIF4GI knockdown in metastatic breast cancer cells to by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 8 result in a significant reduction in the equolmediated increase in protein expression of p120 catenin, Cyclin D1, and Bcl-Xl, without affecting their mRNA levels. These mRNAs all contain an IRES in their 5’UTR and have been shown to be under eIF4GI regulation during cancer progression (36;51-53). Their decreased IRES-dependent translation and the associated polysome association also validates the mechanism that equol increases expression of eIF4GI, which in turn favors the increased translation of certain IRES-containing, cancer promoting mRNAs. When eIF4GI was silenced by 50-60%, we observed a parallel 50-60% decrease in the translation of these IRES-containing mRNAs. The eIF4GI knockdown was sufficient to reduce 100% of the equol-mediated increases in Cyclin D1, BclXl, and p120 catenin, proteins that were specifically dependent on elevated eIF4GI levels. A central finding from our research is that equol increases mRNA and protein levels of eIF4GI and c-Myc, selectively in cancer cells. Intriguingly, c-Myc and eIF4E protein levels were not affected by silencing eIF4GI. The oncogenic transcription factor c-Myc regulates a large variety of cellular functions including cell cycle progression, protein synthesis, metabolism, apoptosis, and genomic stability through several signaling pathways. Accordingly, c-Myc is increased in many human cancers, including breast cancer, and is regulated via direct and indirect mechanisms (38;54-57). We found that reducing the levels of eIF4GI was not sufficient to downregulate the equol increased levels of c-Myc nor to abolish the increase in cell viability in response to equol. Therefore, equol may activate c-Myc transcription independently of eIF4GI upregulation. Overall, c-Myc appears to be a major player in the cancer promoting effects of equol in MDAMB-435 and Hs578t metastatic cancer cells. Both eIF4E and eIF4GI are reported to be transcriptionally regulated by c-Myc (41;58). Accordingly, we found a significant reduction in eIF4GI and a trend toward eIF4E reduction in cMyc silenced cells. C-Myc knockdown resulted in a significant decrease in Cyclin D1 levels, which were also reduced in cells with eIF4GI knockdown. c-Myc is an established transcriptional regulator of Cyclin D1, which likely explains the decreased Cyclin D1 expression and cell viability we observed in breast cancer cells expressing c-Myc siRNA. However, c-Myc knockdown did not affect Bcl-Xl and p120 catenin proteins. Since elevated Bcl-Xl and p120-catenin levels in equol treated cells were inhibited by partial eIF4GI silencing, as well as with c-Myc knockdown, this result indicates that equol mediated c-Myc upregulation leads to the transcriptional activation of eIF4GI. The resultant elevated eIF4GI protein levels are predicted to stimulate preferential cap-independent synthesis of IRES-containing mRNAs such as Cyclin D1, BclXl, and p120 catenin. However, when c-Myc is silenced and the equol-elevated eIF4GI is abolished, cap-dependent protein synthesis may account for the increased Bcl-Xl and p120 expression. Validating the role of c-Myc in control of cell viability in multiple cancers (59;60), knockdown of c-Myc to basal levels of expression as in nonequol treated (control) Hs578t and MDA-MB-435 cells, completely abolished the increase in cell viability in response to equol. Furthermore, knockdown of c-Myc expression abolished the effect of equol on enhanced mammosphere formation. Mammosphere assays have been used to identify stem cell-like properties of self-renewal and tumorigenesis in aggressive cancer cell populations (42;43;61). Enhanced c-Myc expression and the associated increase in translation initiation have been implicated with mammary stem cell amplification and tumorigenic potential (62-64), especially in human growth factor receptor 2 (HER2)-amplified breast cancers, such as the MDA-MB-435 HER2++ cell line used in this study (65). Therefore, collectively, our data suggests that equol-mediated amplification of cMyc and eIF4G may direct increased cancer stem cell-like and tumorigenic properties. At present, the mechanism by which equol upregulates c-Myc transcription is not known. Equol is structurally similar to estrogen with 80 times more ERβ affinity than their precursor, daidzein (66). c-Myc is a recognized estrogen and estrogen mimetics regulated oncogene. However, unlike other estrogen stimulated genes, the mechanism by which c-myc is regulated is not completely understood (56). c-Myc transcription is regulated by cell surface receptors that include Wnt/β-catenin and growth factor or signaling pathways that activate transcription factors such as by gest on July 5, 2017 hp://w w w .jb.org/ D ow nladed from Equol increases cancer potential via c-Myc upregulation 9 TCF/LEF and AP-1, known to regulate c-Myc expression in breast cancer (37;56;67). Although the role of equol in Wnt signaling is not yet established, equol has been implicated in enhanced AP-1 activity (68). In our study, we used ERbreast cancer cell lines, however these cells still expresses steroid receptors and may even express estrogen related receptors (66;69). Moreover, MDA-MB-435 cells have been shown to express splice variants of the ER that may still be responsive to phytoestrogens (70). Therefore, equol may regulate c-Myc transcription via a variety of mechanisms, some of which may involve estrogen receptor related pathways and crosstalk with growth factor receptor signaling. c-Myc is highly amplified in human cancers (37). c-Myc regulates approximately 15% of the human genome, and can also control multiple stages of ribosome biogenesis including the expression of translation initiation factors that are important for both cap-dependent and capindependent translation (71;37). Since equol did not significantly affect c-Myc or eIF4G levels in non-transformed cells, equol is not expected to affect the function of normal cells. However, in cancer cells that already have amplified c-Myc, the 2-fold upregulation of c-Myc may have a profound effect on cancer potential. Increased c-Myc and eIF4G levels can promote the selective translation of mRNAs that use non-canonical eIF4Eindependent modes of initiation; thus, enhancing the survival of cancer cells in the nutrient-deprived and hypoxic conditions that exist in solid tumors. Moreover, the equol-mediated c-Myc upregulation may enhance the stem cell-like properties of a subset of cancer cells. This action is also expected to increase the potential for malignant properties such as therapy resistance and survival during nutrient deprivation. Taken together, this study demonstrates that equol possesses pro-cancer properties and may influence cancer potential via upregulation of cMyc transcription leading to both c-Myc dependent and -independent eIF4G-mediated translation initiation of oncogenes and increased cancer cell survival. Thus, this study contributes to an understanding of the possible mechanisms by which soy isoflavones can affect breast cancer by demonstrating a key role for c-Myc upregulation. Acknowledgements– We wish to thank Dr. Deborah Silvera (NYU School of Medicine) for providing the eIF4G shRNA constructs.

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تاریخ انتشار 2014