Five breast carcinoma cell lines (T-47D, SK-BR-3, MDA-MB-231, MCF7 and BT-474) were purchased from the Chinese Academy of Science Cell Bank (Shanghai, China). Esophageal squamous cell carcinoma (EC-109), human cervical adenocarcinoma (HeLa), prostate cancer (PC1) and MCF10A cells were kindly provided by the Central Laboratory, Tongji University Affiliated People's 10th Hospital (Shanghai, China). All cells except MCF10A were cultured with 10% fetal bovine serum (FBS; Gibco-BRL/Life Technologies, Paisley, UK) in high-glucose Dulbeccos modified Eagles medium (DMEM; HyClone Laboratories, Inc., Logan, UT, USA) and supplemented with antibiotics (100 U/ml penicillin and 100 mg/ml streptomycin; Gibco-BRL, Grand Island, NY, USA) at 37°C with 5% CO₂ in a humidified incubator. The MCF10A was maintained in complete media [DMEM/F12 (50:50 mix) supplemented with 5% horse serum, 10 mg/ml 10 mM HEPES, insulin, 20 ng/ml epidermal growth factor, 0.5 mg/ml hydrocortisone and 100 ng/ml cholera toxin]. Thirty-eight pair-matched breast tissue samples were obtained from the Department of Breast and Thyroid Surgery, Tongji University Affiliated People's 10th Hospital (Shanghai, China). All samples were obtained surgically and immediately snap- frozen and stored in liquid nitrogen until use. The Institutional Review Board approved the tissue procurement protocol used in the study, and the appropriate informed consent was obtained from the patients.

Total RNA was isolated by TRIzol reagent according to the manufacturers protocol (Invitrogen, Carlsbad, CA, USA). cDNA was performed using 1000 ng of total RNA as the template with looped primers and using a PrimeScript RT reagent kit (RR037A; Takara Bio, Inc., Shiga, Japan). Quantitative real-time PCR was performed in a 96-well plate according to the protocol of the KAPA SYBR FAST Universal qPCR kit (KK4601; Kapa Biosystems, Wilmington, MA, USA). An ABI 7900HT PCR sequencer (Applied Biosystems, Foster City, CA, USA) was used for the data measured, and gene expression was calculated using the ∆∆Ct method for relative quantitation using 18S or U6 as endogenous reference genes. The sequences of specific primers are 5-GAGAGGAACA AGCTGGCTGC-3 and 5-GCTTCTCCTTCTCCTTCTGC-3 for FOSL2; 5-CGTACAGCATCCTGGAGATA-3 and 5-CC TTCAGCTTACAGTCATTG-3 for FGF10; 5-CTGAGCTC TCTGAGTGCAAC-3 and 5-GGTCTGAGCTGTATCGC TGC-3 for EGFR; 5-GCAAGACTCCAGCGCCTTCT-3 and 5-CTCATCTTCTTGTTCCTCCTC-3 for MYC; 5-CCTGG ATACCGCAGCTAGGA-3 and 5-GCGGCGCAATACGAA TGCCCC-3 for 18S RNA; 5-ACACTCCAGCTGGGTGTG TCACTCGATGAC-3 and 5-TGGTGTCGTGGAGTCG-3 for miR-597; 5-CTCGCTTCGGCAGCACA-3 and 5-AACGCT TCACGAATTTGCGT-3 for U6.

Cell proliferation was detected using MTT assay, 1,000 cells transfected with synthesized oligonucleotides were seeded in 96-well plates. At 0, 48, 72 and 96 h, 100 µl of 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) solution (0.5 mg/ml) (Sigma-Aldrich, St. Louis, MO, USA) was added to each well, after incubated for another 4 h the medium was removed, and 150 µl of dimethyl sulfoxide (DMSO) was added. The plates were read at a wavelength of 490 nm. Cell migration was detected by the wound-healing assay, an artificial wound was created by a 200 µl pipette tip. To visualize migrated cells and wound healing, images were taken at 0 and 36 h. Cell invasion was detected using a Transwell chamber (Millipore, Billerica, MA, USA) with Matrigel (BD Biosciences, San Jose, CA, USA). Cells (1×10⁵) were cultured in the top chamber of Transwell coated with Matrigel. Cells were cultured in medium with no fetal bovine serum (FBS) in the upper chamber and added with FBS-DMEM in the lower chamber. After 36 h, invasive cells on the lower chamber were fixed in 95% ethanol and stained with 0.5% crystal violet, the numbers were determined using ImageJ software (National Institutes of Health, Bethesda, MD, USA).

A total of 5×10⁵ transfected cells were seeded into 6-well plates and incubated in 0.2% serum medium for cell synchronization. Subsequently, the cells were incubated with complete medium for 48 h. The cells were stained with propidium iodide (PI) (550825; BD Biosciences, San Diego, CA, USA) and ~1×10⁵ cells were examined with a FACS flow cytometer and analyzed with ModFit software (BD Biosciences, San Jose, CA, USA).

A total of 1.5×10⁵ transfected cells were plated into 6-well plates, and the assay performed according to the manufacturers protocol of a Cell-Light™ EdU Apollo^® 488 In Vitro Imaging kit (C10310-3; Guangzhou RiboBio, Co., Ltd., Guangzhou, China). Finally, cells were visualized and counted using a fluorescence microscope (Leica Microsystems, Wetzlar, German).

We used the pGL3-reporter luciferase vector to construct the pGL3-FOSL2 3UTR or pGL3-FOSL2 3UTR-mut vectors. The pGL3-FOSL2 3UTR-mut vector was obtained using a KOD-Plus-Mutagenesis kit (F0936K; Toyobo, Co., Ltd., Osaka, Japan). The Luciferase activity of NC and miR-597 were measured whit the Dual-luciferase reporter assay system (Promega Corp., Fitchburg, WI, USA) after transfection for 36 h. Firefly luciferase activity was normalized to Renilla luciferase activity for each transfected well. The sequences of specific primers are 5-AT ACTCGAGAGCACCTTCAAGCGCTCCAG-3 and 5-GG AAGCTTCTGCTGCTTGGATTCATCTC-3 for FOSL2-3UTR, 5-ATACTCGAGATGTACCAGGATTATCCCGG-3′ and 5-GCGGAATTCTTACAGAGCCAGCAGAGTGG-3 for FOSL2-CDS.

Protein lysates were separated by sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis and transferred to nitrocellulose membranes (Millipore, Billercia, MA, USA). The primary antibodies were incubated overnight after blocking with 5% fat-free milk for 1 h and the primary antibodies were β-actin (Santa Cruz Biotechnology, Inc., Santa Cruz, CA, USA), FOSL2 (ab124830; Abcam, Cambridge, UK), MMP-2 and MMP-9 (13132, 13667; Cell Signaling Technologies, Beverly, MA, USA) and then incubated with their corresponding secondary antibodies (LI-COR Biosciences, Lincoln, NE, USA). Odyssey LI-CDR scanner (BD Biosciences) were used for the membranes.

All statistical analyses were performed using the SPSS version 20.0 (SPSS, Inc., Chicago, IL, USA). The data are presented as the mean ± SD. The statistical significance is shown as P<0.05, P<0.01.

In order to ascertain the expression of miR-597 in breast cancer, qRT-PCR was performed in 38 pairs of breast cancer and non-cancerous tissues. As shown in Fig. 1A, the results demonstrated that miR-597 was significantly downregulated in breast cancer tissues (Fig. 1A). Human breast cancer cell lines T-47D, SK-BR-3, MDA-MB-231, MCF7 and BT-474, and normal breast cell line MCF10A were also detected by qRT-PCR. As shown in Fig. 1B, the expression levels of miR-597 were also downregulated in the five breast cancer cell lines (Fig. 1B). Since MDA-MB-231 and SK-BR-3 cells exhibited the lowest miR-597 expression among the five breast cancer cell lines, these two cell lines were chosen for mature miR-597 mimic transfection and for further studies.

Subsequently, to evaluate the function of miR-597 in tumorigenesis, we transfected miR-597 mimics into MDA-MB-231 and SK-BR-3 to increase the levels of ectopic miR-597. As a result, the elevation of miR-597 significantly inhibited the growth rate of MDA-MB-231 and SK-BR-3 from the third day (Fig. 2A and B; P<0.01). The cell proliferation process was modulated by the cell cycle, thus, an EdU assay was performed. The result showed that the miR-597 subclone incorporated less EdU compared with the NC subclone (Fig. 2C and D; P<0.01), indicating that miR-597 reduced cells into S-phase. In addition, flow cytometry revealed that cells with miR-597 overexpression had a 20–30% higher proportion at the G0/G1 phase and a 20% lower proportion at the S phase compared with NC groups (Fig. 2E and F). All results suggested that miR-597 inhibited cell proliferation by modulating the G1-S phase of the cell cycle.

To investigate the effect of miR-597 on the migration and invasion of breast cancer cells, miR-597 mimic or its negative control were transfected into MDA-MB-231 and SK-BR-3 cells, respectively. The wound healing assay was performed, the results showed that the migration ability of MDA-MB-231 and SK-BR-3 cells in the miR-597 group was lower than NC groups at 36 h post-wounding (Fig. 3A and B; P<0.01). The cell invasion assay showed similar results, in the miR-597 group, there was ~50% reduction in the average number of cells penetrating the Transwell membrane and Matrigel compared with NC group (Fig. 3C and D; P<0.01). By detecting and analyzing with western blot analysis, we found that the expression levels of invasion-related proteins MMP-2 and MMP-9 were reduced (data not shown). Thus, the above results suggest that miR-597 plays an important part in the cell migration and invasion.

In order to find the targets of miR-597, we used TargetScanHuman 6.2 and GeneCoDis3 to predict the targets of miR-597 and we found that four genes (FGF10, EGFR, FOSL2 and MYC) had functions that oppose miR-597 in breast cancer. By performing qRT-PCR, we only found FOSL2 markedly inhibited by miR-597 (Fig. 4A and B; P<0.01). In addition, the expression of FOSL2 protein in the miR-597 subclone was lower than that in the NC subclone (Fig. 4C). The luciferase reporter assays also demonstrated that miR-597 mimics significantly reduced the activity of FOSL2 3-UTR, while there was no change in the mutant group (Fig. 4D). These data suggested that FOSL2 is a direct target of miR-597.

To test the hypothesis that miR-597 regulates cell proliferation and invasion by targeting FOSL2, we co-transfected miR-597 mimics and FOSL2-expressing vector into MDA-MB-231 and SK-BR-3 cells. The western blot result showed that the level of FOSL2 decreased by miR-597 could be rescued by overexpression of FOSL2 in cells (data not shown). As shown in Fig. 5, FOSL2 reintroduction reversed the anti-proliferation and anti-invasion roles of miR-597, suggesting that the effect of miR-597 on cell growth and invasion were largely mediated by its downregulation of FOSL2.

In order to determine the expression levels of FOSL2 in breast cancer, the real-time PCR analysis was performed in 38 pairs of breast cancer and adjacent non-cancerous tissues. The results demonstrated that the FOSL2 mRNA were higher in tumor samples compared with the adjacent normal tissues (Fig. 6A). Finally, analyzing with Pearson correlation the expression of FOSL2 and miR-597 (Fig. 1A) in these 38 tumor samples, we found a negative correlation between the two (Fig. 6B, R=−0.5979; P=0.0082).