17β-estradiol (E₂) was purchased from Sigma-Aldrich (St. Louis, MO, USA) and dihydrotestosterone (DHT) from Steraloids, Inc. (Newport, RI, USA), whereas hydroxyflutamide (OHF) was kindly donated by Schering-Plough Corporation (Kenilworth, NJ, USA). These compounds were dissolved in ethanol. p,p'-DDE was purchased from Cerilliant Corporation (Round Rock, TX, USA) and was dissolved in dimethylsulfoxide. Final concentrations of vehicles in the cell culture medium were 0.1% (vol/vol). Aprotinin, leupeptin, phenylmethylsulfonyl fluoride, and sodium orthovanadate were purchased from Sigma-Aldrich.

CAMA-1 and MCF-7 cells were purchased from the American Type Culture Collection (Manassas, VA, USA). MCF7-AR1 cells were kindly provided by Ana M Soto (Tufts University, Medford, MA, USA). CAMA-1 cells were maintained in phenol red-free Roswell Park Memorial Institute (RPMI) medium supplemented with 10% (vol/vol) fetal bovine serum (FBS) from Wisent Inc. (St.-Bruno, QC, Canada), 1.0 mM pyruvate, 2.0 mM L-glutamine, 0.1 μg/mL streptomycin, and 0.1 U/mL penicillin in a humidified atmosphere of 5% CO₂ at 37°C. Two thousand cells per well were seeded in 200 μL phenol red-free RPMI-10% FBS in 96-well plates (6 wells per treatment) and were incubated during 24 hours at 37°C. The complete medium was then substituted for FBS-free medium for a 24-hour period. On day 1 of the experiment, the FBS-free medium was replaced by a medium containing 10% dextran-coated charcoal-treated FBS (DCC-FBS) from Wisent Inc., the hormones, and test chemicals (or vehicles). Cells were grown over a 9-day period with a medium replacement every 3 days. The medium was then removed and nucleic acids were stained using the CyQuant^® kit purchased from Molecular Probes Inc. (now part of Invitrogen Corporation, Carlsbad, CA, USA) as described by the manufacturer. Cell proliferation for the control treatment was arbitrarily set at 1, and results were expressed as fold induction over the control.

MCF-7 and MCF7-AR1 cells were maintained in phenol red-free Dulbecco's modified Eagle's medium (DMEM) supplemented with 10% (vol/vol) FBS, 1.0 mM pyruvate, 2.0 mM L-glutamine, 0.1 μg/mL streptomycin, 0.1 U/mL penicillin, and 1 μg/mL insulin in a humidified atmosphere of 5% CO₂ at 37°C. One thousand cells per well were seeded in 200 μL of phenol red-free DMEM-10% FBS in 96-well plates (6 wells per treatment) and were incubated during 24 hours at 37°C. The complete medium was removed and cells were washed with phosphate-buffered saline (PBS). Then a medium containing 10% DCC-FBS, the hormones, and test chemicals (or vehicles) were added. Cells were grown over a 6-day period without medium replacement, and proliferation was assessed as described above for CAMA-1 cells.

Fifty thousand cells per well were seeded in 1 mL phenol red-free RPMI-10% FBS in 24-well plates and incubated during 24 hours at 37°C. The medium was replaced by FBS-free medium during 48 hours to promote G0/G1 synchronization 23. FBS-free medium was then replaced by a medium containing 10% DCC-FBS, hormones, and test chemicals (or vehicles) for a 24-hour incubation period at 37°C. Cells were harvested following trypsinization, fixed in 70% ethanol for 30 minutes at -30°C, and stained with propidium iodide (50 μg/mL) in PBS containing 40 U/mL RNase A for 1 hour at 37°C. The DNA content in each cell was determined by flow cytometry analysis using the Wallac 1420 Multilabel Counter from PerkinElmer Life and Analytical Sciences, Inc. (Waltham, MA, USA).

Two million cells were seeded into 10-cm dishes in 10 mL of phenol red-free RPMI-10% FBS and were incubated during 24 hours at 37°C. The complete medium was then substituted for FBS-free medium for a 24-hour period. The FBS-free medium was subsequently replaced by a medium containing 10% DCC-FBS, the hormones, and test chemicals (or vehicles), and cells were grown over a 24-hour period. Duplicate cell cultures were used for each treatment: one dish was used for RNA and the other for total cell extracts. RNA was isolated with TRIzol^® from Gibco (now part of Invitrogen Corporation) as described by the manufacturer and diluted in 40 μL of diethyl pyrocarbonate-treated H₂O. mRNAs were reverse-transcribed by Super Script II™ using Oligo(dt) primer from Invitrogen Corporation as described by the manufacturer in a final volume of 50 μL. An amount of 500 ng of total RNA was included as template for each reaction. The amount of cDNA used for polymerase chain reaction (PCR) was adjusted for each target gene. To assess ESR1 mRNA (forward primer: 5'-AATTCAGATAATCGACGCCAG-3'; reverse: 5'-GTGTTTCAACATTCTCCCTC-CTC-3'; annealing temperature (Tm) = 58°C; 344 base pairs [bp]) 24, a 10-μL aliquot of cDNA was used compared with 1 μL for β-actin (forward primer: 5'-CGTGACATTAAGGAGAAGCTGTGC-3'; reverse: 5'-CTCAGGAGGAGCAATGATCTTGAT-3'; Tm = 58°C; 375 bp) 25, while 10 and 5 μL of amplified product were loaded on an 8% polyacrylamide gel for ESR1 and β-actin, respectively. To evaluate mRNAs for CCND1 (forward primer: 5'-CGGAGGAGAACAAACAGATC-3'; reverse: 5'-GGGTGTGCAAGCCAGGTCCA-3'; Tm = 55°C; 350 bp) 26 and AR (forward primer: 5'-GTCAAAAGCGAAATGGGCCCC-3'; reverse: 5'-CTTCTGGGTTGTCTCCTCAGT-3'; Tm = 60°C; 420 bp) 27, we used 5-μL aliquots of cDNA for both genes and a 2-μL aliquot for β-actin while 10 μL of amplified products was loaded on the gel. To evaluate mRNAs for TFF1 (forward primer: 5'-TTTGGAGCAGAGAGGAGGCAATGG-3'; reverse: 5'-TGGTATTAGGATAGAAGCACCAGGG-3'; Tm = 58°C; 240 bp) 28, we used 2-μL aliquots of cDNA and a 2-μL aliquot for β-actin while 10 μL of amplified products was loaded on the gel. Taq DNA polymerase and deoxynucleotides (Roche Diagnostics, Basel, Switzerland) were used as described by the manufacturer in a 50-μL final volume. The PCR settings were adjusted to complete each reaction within the linear portion of amplification. PCR conditions were one 5-minute cycle at 95°C, 25 (β-actin) or 30 cycles (target mRNAs) each comprising a 30-second step at 95°C, followed by a 30-second step at primer-specific Tm and a 45-second step at 72°C, and one last cycle of 7 minutes at 72°C. Negative controls were included for each reaction. PCR products were stained with ethidium bromide and captured with a 16-bit camera. Densitometry was determined by Quantity One 1-D Software Analysis from Bio-Rad Laboratories, Inc. (Hercules, CA, USA) and normalized with β-actin.

Floating cells were recovered with the medium and pooled with the adherent cells that were harvested by scraping in 2 mL of ice-cold PBS, centrifuged, and resuspended in 600 μL of lysis buffer containing 50 mM Hepes, pH 7.5; 1 mM EGTA (ethylene glycol tetraacetic acid), pH 8; 150 mM NaCl; 1.5 mM MgCl₂; 10 mM sodium pyrophosphate; 200 μM sodium orthovanadate; 100 mM NaF; 1% Triton X-100; 10% glycerol; and a protease inhibitor cocktail from EMD Biosciences, Inc. (San Diego, CA, USA). Insoluble material was removed by centrifugation (10 minutes at 13,000 g). Thirty micrograms of the cellular extract was resolved on PROTEAN^® II (Bio-Rad Laboratories, Inc.) 10% SDS-polyacrylamide gels. The proteins were electroblotted onto 0.45-μM polyvinyl difluoride membranes purchased from Millipore Corporation (Billerica, MA, USA). Membranes were blocked at room temperature for 1 hour in PBS containing 5% (wt/vol) dried milk and incubated 2 hours at 37°C with the specific antibody diluted in PBS containing 1% (wt/vol) dried milk. Antibodies against ERα, AR, and cyclin D1 were purchased from Santa Cruz Biotechnology, Inc. (Santa Cruz, CA, USA), and anti-actin was from Cedarlane Laboratories Limited (Burlington, ON, Canada). Membranes were washed in PBS containing 0.1% (vol/vol) Tween 20 followed by a 1-hour incubation with specific immunoglobulin G horseradish peroxidase-conjugated antibodies from Jackson ImmunoResearch Laboratories, Inc. (West Grove, PA, USA) and then incubated in Immun Star HRP Substrate (Bio-Rad Laboratories, Inc.) as described by the manufacturer. Signals were analyzed as described above for reverse transcription-polymerase chain reaction and were normalized for actin within the same membrane according to the method of Liao and colleagues 29.

Concentration-response relationships were tested using linear regression analysis. Group means were compared using an analysis of variance (ANOVA) with specific contrasts or an ANOVA followed by the Bonferroni post hoc test. One-tail tests were performed for cell proliferation experiments because of a priori hypotheses regarding treatment effects (that is, inhibition for androgens and induction for antiandrogens). All other tests were two-sided. All statistical analyses were performed using the SPSS for Windows software (version 11.5.0; SPSS Inc., Chicago, IL, USA).

Figure 1 displays the relative levels of ERα and AR in CAMA-1, MCF7-AR1, and wild-type MCF-7 cells. CAMA-1 and MCF7-AR1 cells expressed, respectively, 6.5-fold (P < 0.01) and 7.5-fold (P < 0.01) more AR proteins compared with wild-type MCF-7 cells, whereas ERα expression levels were not different among the cell lines. Because of their high levels of expression of ERα and AR, CAMA-1 and MCF7-AR1 cells were used to investigate the capacity of p,p'-DDE to disrupt the estrogen-androgen balance and increase cell proliferation.

Before testing the effect of the environmental antiandrogen p,p'-DDE on cell growth, we first assessed the proliferative response of CAMA-1 cells in the presence of estrogens and androgens in the cell culture medium over a 9-day period. Figure 2a shows the concentration-response relationship for E₂-induced proliferation of CAMA-1 cells. We used a 100-pM concentration of E₂, which generates near maximal proliferation, in combination with increasing concentrations of DHT and observed an inverse dose-response relationship between androgen concentrations (log-transformed) and cell proliferation (regression coefficient [β] = -0.887; P < 0.001) (Figure 2b). Combined treatment with 100, 500, or 1,000 pM DHT reduced the E₂-induced proliferative response by 27% (P < 0.05), 54% (P < 0.001), and 60% (P < 0.001), respectively.

To investigate the potential of p,p'-DDE to increase the proliferation of CAMA-1 cells cultivated in the presence of endogenous estrogens and androgens, increasing concentrations of p,p'-DDE were added to the cell culture medium together with E₂ and DHT. p,p'-DDE induced concentration-related increases in CAMA-1 cell proliferation in the presence of 100 pM E₂ and DHT added at a concentration of 100 pM (β = 0.674, P < 0.001; Figure 3a), 500 pM (β = 0.629, P < 0.001; Figure 3b), or 1,000 pM (β = 0.663, P < 0.001; Figure 3c). Concentrations of p,p'-DDE as low as 2 μM caused a statistically significant increase in cell proliferation compared with the E₂+DHT treatment (P < 0.01; Figure 3a,b); the 5-μM concentration completely abolished the inhibitory effect of DHT on cell proliferation. In the absence of sex steroid hormones, p,p'-DDE added to the cell culture medium induced only a slight proliferative response (1.3-fold induction at 10 μM, P < 0.01; Figure 3d).

The capacity of p,p'-DDE to increase breast cancer cell proliferation in the presence of sex steroids was also tested in MCF7-AR1 cells. Szelei and colleagues 30, who genetically engineered these cells that overexpress the AR, previously reported that DHT added together to E₂ decreased the proliferation of MCF7-AR1 cells compared with treatment with E₂ alone. We observed that p,p'-DDE induced a concentration-related increase in MCF7-AR1 proliferation in the presence of 10 pM E₂ and 100 pM DHT (β = 0.513, P = 0.01; Figure 4a). A 2-μM concentration of p,p'-DDE caused a 2-fold increase in cell proliferation compared with the E₂+DHT treatment (P < 0.05). In the absence of sex steroid hormones, p,p'-DDE added to the cell culture medium also induced a significant proliferative response (2.9- and 3.6-fold induction at 5 and 10 μM, respectively, P < 0.001; Figure 4b).

To better characterize the proliferative response induced by p,p'-DDE on CAMA-1 cells, we measured cell transition from the G0/G1 to the S phase after a 24-hour treatment with p,p'-DDE in the presence of sex steroid hormones and compared the results to those obtained with the potent antiandrogen OHF. Adding 1 nM DHT in combination with 1 nM E₂ reduced by more than 50% (P < 0.05) the percentage of cells in the S phase observed in the presence of 1 nM E₂ alone (Figure 5a). The addition of either 10 μM p,p'-DDE or 1 μM OHF to the cell culture medium completely abolished the androgen-mediated decrease in the percentage of CAMA-1 cells entering the cell cycle (P < 0.05 versus E₂+DHT treatment). Treatment-induced changes in the percentage of cells in G0/G1 were of similar magnitude to those observed for the S phase but in the opposite direction (Figure 5b). The proportion of cells in the G2/M phase was slightly increased by the 1-nM E₂ treatment (P < 0.05), but adding DHT and antiandrogens in combination with E₂ did not modify the E₂-induced response (Figure 5c).

To further elucidate the mechanism underlying the induction of CAMA-1 cell proliferation by p,p'-DDE, we studied the effect of a 24-hour treatment with p,p'-DDE on the expression of sex-hormone-sensitive genes at the mRNA level, in the presence of E₂ and DHT, and compared the results with those obtained by treating the cells with OHF in combination with the endogenous hormones. The mean cyclin D1 mRNA level was increased by 50% (P < 0.01) in E₂-treated cells compared with that of the control cells (Figure 6a), whereas 1 nM DHT significantly reduced this estrogenic effect (P < 0.01 versus E₂ alone). Treatment with either 10 μM p,p'-DDE or 1 μM OHF partly abolished the inhibition of cyclin D1 mRNA expression induced by DHT, resulting in mean expression levels that are not significantly different from that induced by E₂ alone. Although E₂ alone did not modulate ERα mRNA expression, the E₂+DHT treatment appeared to decrease the mean expression level compared with that induced by E₂ alone (Figure 6b), whereas p,p'-DDE or OHF partly offset this downregulation. However, differences between treatments did not reach statistical significance. AR mRNA mean expression level was decreased by 27% following DHT treatment compared with E₂ treatment (P < 0.01; Figure 6c), whereas treatment with either 10 μM p,p'-DDE or 1 μM OHF completely antagonized this inhibition (P < 0.01 versus E₂+DHT). pS2 mRNA mean expression level was increased by 50% (P < 0.01) following E₂ treatment compared with the control (Figure 6d). The E₂+DHT treatment induced a slightly lower expression of pS2 mRNA compared with that caused by E₂ alone, but the difference was not statistically significant. p,p'-DDE added together with E₂ and DHT induced a greater pS2 mRNA expression than did the E₂+DHT treatment (P < 0.05).

We also evaluated the modulation of cyclin D1, ERα, and AR protein expression levels by p,p'-DDE treatment in CAMA-1 cells in the presence of endogenous sex steroids. Cyclin D1 level was increased by 80% (P < 0.01) in cells treated with 1 nM E₂ compared with the vehicle-treated cells (Figure 7a), whereas adding 1 nM DHT in combination with E₂ blocked this increase (P < 0.01 versus E₂ alone). The addition of either 10 μM p,p'-DDE or 1 μM OHF to the cell culture medium together with E₂ and DHT completely abolished this DHT-mediated inhibition of cyclin D1 expression (P < 0.01 versus E₂+DHT). Whereas E₂ alone was without effect, the combined E₂+DHT treatment markedly decreased ERα protein level (more than 50%) as compared with that observed following E₂ treatment or control (P < 0.05; Figure 7b). p,p'-DDE or OHF treatment again abolished this androgen-mediated inhibition (P < 0.01 versus E₂+DHT). A different response pattern was observed for AR protein expression (Figure 7c). E₂ treatment decreased by 28% (P < 0.05) the mean AR protein expression level compared with control, whereas AR protein level was significantly increased following the combined E₂+DHT treatment compared with the value noted following E₂ treatment alone (P < 0.01). The androgen-mediated increase in AR protein level was antagonized by adding OHF in the incubation medium (P < 0.05 versus E₂+DHT) but not p,p'-DDE (Figure 7c).