The BT474 human breast cancer cell line was purchased from the American Type Cell Culture (ATCC; Manassas, VA, USA) and the cells were cultured in RPMI-1640 medium (Gibco-Life Technologies, Grand Island, NY, USA) supplemented with 10% fetal bovine serum (FBS; Gibco-Life Technologies) and 1% penicillin/streptomycin (Beyotime Institute of Biotechnology, Nanjing, Jiangsu, China) in the presence of 5% CO₂ at 37°C.

E2 was purchased from Sigma-Aldrich Corp. (St. Louis, MO, USA). The cells were plaed in 6-well plates at a density of 5,000 cells/well. The cells were washed and starved for 24 h in serum-free RPMI-1640 medium (Gibco-Life Technologies) after up to 60–80% confluence to eliminate the potential influence of estrogen in fetal bovine serum, and to trigger starvation-induced autophagy. The cells were then cultured in serum-free RPMI-1640 medium in the presence of 200 ng/ml E2 or 0.02% ethanol as the vehicle. The cells were exposed to E2 or the vehicle for 24, 48 and 72 h before they were harvested.

The antibodies were used were as follows: rabbit anti-caveolin 1, rabbit anti-high mobility group box 1 protein (HMGB1), rabbit anti-light chain (LC)3, rabbit anti-Beclin-1, rabbit anti-Atg12 and rabbit anti-cleaved-caspase-3 were purchased from Cell Signaling Technology (Beverly, MA, USA). Rabbit anti-GAPDH was purchased from Santa Cruz Biotechnology (Santa Cruz, CA, USA).

The human caveolin-1, human HMGB1 and negative control siRNA were designed and constructed by Guangzhou Ribio Biotech Co., Ltd. (Guangzhou, China). The sequences of caveolin-1 and HMGB1 siRNA were as follows: caveolin-1, 5′-GCAUCAACUUGCAGAAAGAdTdT-3′ and 3′-dTdTCGUAGUUGAACGUCUUUCU-5′; HMGB1, 5′-GGAGGAAGAUGAAGAAGAUdTdT-3′ and 3′-dTdTCCUCCUUCUACUUCUUCUA-5′. Twenty-four hours prior to transfection with siRNA, the medium was replaced with penicillin/streptomycin-free RPMI-1640 complete medium. The BT474 cells were then transfected with siRNA using Lipofectamine™ 2000 (Invitrogen-Life Technologies, Carlsbad, CA, USA) in OPTI-MEM (Gibco-Life Technologies) for 6 h, and then the medium was replaced with antibiotics-free RPMI-1640 complete medium. After being transfected for 48 h, the cells were then exposed to E2 for a further 24 h.

The BT474 cells were planted in 6-well plates until they were grown to 60–80% confluence and they were treated with different stimuli for the indicated periods of time. The extraction of protein was performed using an assay kit (Cell Signaling Technology), and the concentration of total protein was examined using the BCA Protein Assay kit (Beyotime Institute of Biotechnology). For western blot analysis, SDS-PAGE (Beyotime Institute of Biotechnology) was used to separated equal amounts (30 μg) of total protein and then the protein was transferred onto PVDF membranes (Millipore, Billerica, MA, USA) using transfer buffer (200 mM glycin, 40 mM Tris and 20% methanol) at 240 mA for 30–90 min, depending on the molecular weight of the detected proteins. The membranes were blocked with 5% non-fat milk (Cell Signaling Technology) in 0.1% TBST (Cell Signaling Technology) for 1 h, at 37°C and then incubated with the primary antibody overnight at 4°C. After washing in 0.1% TBST 3 times, 5 min each, the membranes were incubated in horseradish peroxidase (HRP)-conjugated anti-rabbit secondary antibody (Cell Signaling Technology) at a dilution 1:3,000 for 1 h, 37°C. The membranes were then washed in 0.1% TBST 3 times, 5 min each. The ECL Chemiluminescent Substrate Reagent kit (Cell Signaling Technology) was added to the membranes and the quantification of the band intensity of the blots was measured using Image Lab software (Bio-Rad Laboratories, Hercules, CA, USA). The internal standard was GAPDH.

The BT474 cells were seeded at sterile glass slides in 6-well plates. After they reached 50–60% confluence, the cells were treated with different stimuli as indicated. The medium was then discarded, and the cells were washed with cold PBS (Cell Signaling Technology) 3 times. The cells were fixed with 100% cold methanol at −20°C for 15 min. Following washing 3 times again in cold PBS, the slides were blocked with 1% bovine serum albumin in 0.1% PBST (Cell Signaling Technology) for 1 h at room temperature. The slides were incubated with primary antibody overnight at 4°C. FITC-conjugated goat-anti-rabbit IgG (Cell Signaling Technology) was used to detect the primary antibody for 1 h at room temperature in the dark. Subsequently, DAPI (0.3 μmol/l) was used to label the nuclei for 2 min at room temperature in the dark. The slides were then washed and images were acquired using an Olympus IX71 epifluorescence microscope (Olympus, Tokyo, Japan).

MDC (Sigma-Aldrich), an autofluorescent dye, is used to detect autophagy. Briefly, the BT474 cells were incubated with 50 μmol/l MDC for 15 min at 37°C to monitor autophagosomes. The cells were then washed with PBS 3 times immediately followed by image acquisition. The MDC-positive cells were observed under a fluorescence microscope (Olympus).

For the apoptosis assay, an Annexin V-FITV/PI apoptosis kit (Nanjing KeyGen Biotech, Co., Ltd., Nanjing, China) was used according to the manufacturer’s instructions. Briefly, the cells (1–5×10⁵) were isolated using EDTA-free Trypsin (Beyotime Institute of Biotechnology) and collected. The cells were then centrifuged at 5,000 × g for 5 min, and they were washed 3 times with cold PBS. The cells were resuspended in 500 μl binding buffer containing 5 μl Annexin V-FITC and 5 μl propidium iodide (PI). The apoptotic cells were detected by flow cytometry using a flow cytometer (BD Biosciences, Franklin Lakes, NJ, USA).

The BT474 cells (5×10³ cells/well) were plated in 96-well plates and cultured for the indicated periods of time. Cell viability was measured using the CCK-8 kit (Dōjindo Laboratories, Kumamoto, Japan). Briefly, the medium was removed followed by the addition of 100 μl CCK-8 in a dilution of 1:9 to each well. The cells were then incubated at 37°C for 0.5–2 h, avoiding light. The absorbance of the optical densities was measured using a microplate reader (Thermo Fisher Scientific, Waltham, MA, USA) at 450 nm.

Results obtained from 3 repeat experiments are expressed as the means ± standard deviation (SD), and analyzed using SPSS 11.0 software (SPSS, Inc., Chicago, IL, USA). The Student’s t-test was used to determine the differences between the groups. A value of P<0.05 was considered to indicate a statistically significant difference.

To investigate the involvement of E2 in the autophagy of breast cancer cells, the BT474 (ER⁺) cells were pre-incubated with serum-free RPMI-1640 medium for 24 h to induce autophagy. The cells were then treated with 200 ng/ml E2 or 0.02% ethanol as the vehicle, for various periods of time (24, 48 and 72 h). The expression of caveolin-1, HMGB1 and autophagy-related proteins (Beclin-1, LC3-II and Atg12) was detected by western blot analysis. Our results revealed that compared with the vehicle-treated group, E2 induced a time-dependent increase in the overall expression of caveolin-1, HMGB1 and autophagy-related proteins (Beclin-1, LC3-II and Atg12/5) in the BT474 cells (Fig. 1).

To further assess the association between caveolin-1 and HMGB1 and autophagy-related proteins, caveolin-1 siRNA was used to knock down caveolin-1 expression. At approximately 48 h following transfection, 200 ng/ml E2 or 0.02% ethanol were added to the medium for a further 24 h. The results revealed that caveolin-1 knockdown inhibited the E2-induced upregulation of HMGB1, LC3-II and Atg12/5, but did not affect the E2-induced upregulation of Beclin-1 (Fig. 2). These results indicate that E2-induced autophagy is regulated by cavelin-1 by affecting the expression of LC3-II and Atg12, but not Beclin-1.

As caveolin-1 siRNA also decreased HMGB1 expression, which is deeply related to autophagy, we then determined whether caveolin-1 regulates autophagy by mediating HMGB1 expression. HMGB1 siRNA was constructed and used to knock down the expression of HMGB1. We found that the knockdown of HMGB1 resulted in the inhibition of LC3-II and Beclin-1 expression (Fig. 3). However, caveolin-1 expression was not impaired by HMGB1 knockdown (Fig. 3), suggesting that HMGB1 may be involved in the E2/caveolin-1-induced LC3-related autophagy.

To evaluate autophagy, the LC3 punctate was directly detected by immunofluoresence staining for LC3, and MDC staining was further performed to detect auophagosome formation. Our results revealed that compared with the vehicle-treated group, E2 promoted the formation of both LC3 punctates (Fig. 4A-a) and autophagosomes (Fig. 4A-b). Compared with the group transfected with negative control siRNA (siCon), caveolin-1 or HMGB1 knockdown markedly decreased the E2-induced formation of LC3 punctates (Fig. 4B-a and C-a) and autophagosomes (Fig. 4B-b and C-b).

We then explored the regulation of caveolin-1 and HMGB1 knockdown in the apoptosis and E2-induced cell growth of BT474 cells. Flow cytometric analysis and immnuofluorescence staining for cleaved caspase-3 were used to assess the apoptosis of BT474 cells, and CCK-8 assay was performed in order to evaluate the viability of the BT474 cells. The results demonstrated that compared with the vehicle-treted group, E2 inhibited apoptosis and the formation of cleaved caspase-3 punctates (Fig. 5A and B-a). In addition, compared with the siCon group, caveolin-1 or HMGB1 knockdown markedly promoted apoptosis which had been inhibited by E2 (Fig. 5A and B-b). The results from the evaluation of cell viability by CCK-8 assay revealed that caveolin-1 or HMGB1 knockdown markedly suppressed the E2-induced cell growth (Fig. 5C).