Human liver caner cell lines, HCC-LM3 and SMMC-7721, were purchased from American Type Culture Collection (ATCC, USA). Human liver cancer cells of HepG2 were purchased from KeyGen Biotech (Nanjing, China). SMMC-7721 and HepG2 cells were cultured in DMEM (Gibco, USA) supplemented with 10% FBS, 100 U/ml penicillin, and 100 µg/ml streptomycin. Human HCC-LM3 cells were routinely cultured in RPMI-1640 medium (Gibco), containing 10% fetal bovine serum (FBS) (Gibco), 1% penicillin/streptomycin. MRC-5 was cultured in DMEM (Gibco) supplemented with 10% FBS, 100 U/ml penicillin, and 100 µg/ml streptomycin. All cells were cultured in a humidified atmosphere with 5% CO₂ and 95% humidity at 37°C in an incubator. All cells were cultured in a humidified atmosphere with 5% CO₂ and 95% humidity at 37°C in an incubator. Fisetin (>98% purity), used for the treatment of lung cancer, was purchased from Dayang Chem (Hangzhou, China), dissolved in DMSO and stored at −20°C, and then diluted in medium for experiments. The final DMSO concentration in our study was <0.1% (v/v) in every treatment, and bromocriptine used was purchased from Sigma-Aldrich (St. Louis, MO, USA).

Cells of HepG2 (5×10³), HCC-LM3 and SMMC-7721 were seeded into a 96-well plate (Corning, USA) per well. Bromocriptine (from 0 to 40 µM), fisetin ranging from 0–40 µM, was added to the medium. The cells were then incubated at 37°C for 24 h, and the cell viability was detected by the colorimetric MTT assay at 570 nm.

The liver cancer cells were seeded into the upper chamber of a Transwell insert pre-coated with 5 µg/ml fibronectin for migration or a BD™ Matrigel invasion chamber for invasion. Medium with 10% serum was put in the lower chamber as a chemo-attractant, and cells were then incubated for 4 h. Non-migratory cells were removed from the upper chamber with a cotton bud. The cells on the lower insert surface were stained with Diff-Quick. Cells were counted as the number of cells observed in three randomly different microscope fields of three independent inserts.

To explore the liver cancer cell proliferation, 60% liver cancer cells of HCC-LM3 and HepG2 were treated with bromocriptine and fisetin or the two drugs in combination for 24 h in growth medium. The cells were then harvested in a separate tube after incubation. Then, 500 cells/well were cultured in 6-well plate (Corning) separately with complete growth medium and grown for 2 weeks. The medium was replaced after 7 days. For incubation of 14 days, the cells were washed with phosphate-buffered saline (PBS) (Hyclone, USA). Then, cold methanol was used to fix cells for 10 min. Cells were stained with 0.5% crystal violet solution (Chemcatch, USA) in 25% methanol at room temperature. The cells were washed with water three times and air-dried for calculating through an inverted microscope.

ELISA kits for DA determination in serum and tumor tissue samples from mice were purchased from Nordhorn (Germany). DA detection was performed following the manufacturer's instructions.

After treatments under different conditions, the cells were harvested and the medium was removed. Then the cells were washed with chilled PBS three times and lysed in ice-cold lysis buffer with fresh protease inhibitor cocktail. The cell lysates were centrifuged at 12,000 g for 20 min at 4°C to collect the supernatant. BSA protein assay kit was used to detect the protein concentrations following the manufacturer's instructions (Thermo, USA). Protein extracts (40-ng) were separated by 10% SDS-PAGE and were then transferred to polyvinylidene fluoride membrane (Millipore, USA). The PVDF with proteins were blocked with 5% skim fat dry milk in 0.1% Tween-20 in Tris-buffered saline (TBS) for 2 h to block the non-specific sites on blots. The primary antibodies dissolved in blocking buffer were used to detect the target protein blots at 4°C overnight for incubation. The bands on PVDF were covered by chemiluminescence with Pierce ECL Western Blotting Substrate reagents (Thermo Scientific, IL, USA). The primary antibodies used in our study were: rabbit anti-GAPDH, caspase-3, PARP, TGF-β1, VEGFR1, ERK1/2, p-ERK1/2, p38, pJNK, E-cadherin, N-cadherin, and vimentin.

The Annexin V-FITC/propidium iodide (PI) apoptosis detection kit (KeyGen) was used to determine apoptotic cells. Liver cancer cells after different treatments were harvested and washed with chilled PBS, then incubated in a darkroom for Annexin V-FITC and PI for 15 min. Subsequently, the cells were analyzed by flow cytometry (BD Biosciences, USA).

Sixty, 6-week old male, athymic BALB/C nude mice were purchased from the Animal Center of Nanjing Medical University (Nanjing, China) and cultured in a 25±2°C temperature and 50±10% humidity-controlled environment with a standard 12-h light and dark cycle with food and water in cages under germ-free conditions. All processes were in line with the Institutional Animal Care and Use Committee of the second Xiangya Hospital of Central South University. Briefly, athymic BALB/C nude mice were implanted orthotopically with liver cancer HCC-LM3 cells (3×10⁶ cells). All tumor-bearing mice were divided into 4 groups randomly: i) control; ii) Fis (20 mg/kg); iii) Fis (40 mg/kg); iv) Fis (80 mg/kg) daily through i.p. After 7 weeks of treatment, the mice were sacrificed for the following experiments. The blood from mouse was obtained through the eyeball, and then was centrifuged at 15,000 g for 15 min. Fisetin was dissolved in DMSO and diluted in distilled water for further use.

The tissue in each group were fixed with 10% buffered formalin, embedded in paraffin and sliced into 4–5-µm thick sections. Tumor tissues also were subjected to immunohistochemical (IHC) staining for the analysis of VEGFR1 and Ki-67 expression. The immunfluorescent analysis was carried out as described previously (18). The cells or tissue samples were incubated with TGF-β1, as the primary antibody, overnight at 4°C. The slides were then washed with cold PBS and incubated with anti-rabbit secondary antibody (KeyGen). The histological examination was performed following the standard procedures described previously (19).

Data were expressed as mean ± SEM. Statistical analyses were carried out with GraphPad PRISM (version 6.0; Graph Pad Software). A P-value <0.05 was considered statistically significant.

In order to explore whether fisetin could perform as DR2 agonist showing important role in regulating liver cancer cell prolifreration, the cell viability of liver cancer cells of HCC-LM3, HepG2 and SMMC-7721 was calculated. As shown in Fig. 1B, fisetin at different concentrations (0, 1, 2.5, 5, 10, 20, 40 and 80 µM) was administered to HCC-LM3 cells. Fisetin showed significantly inhibitory role in HCC-LM3 proliferation >10 µM. Similarly, the death receptor 2 agonist of bromocriptine markedly suppressed HCC-LM3 cell proliferation in a dose-dependent manner. Consistently, in HepG2 cells, fisetin also displayed suppressive effects on cell proliferation, which was in line with the role of bromocriptine in HepG2 regulation (Fig. 1C). Fisetin also exhibited inhibitory role in SMMC-7721 cells. Of note, bromocriptine, as DR2 agonist, reduced the liver cancer cell viability (Fig. 1D). Taken together, the results above indicated that fisetin shows similar role with bromocriptine, reducing liver cancer cell lines proliferation, which might be an essential therapeutic strategy for liver cancer treatment and linked with the DR2 signal.

In this regard, we investigated the effects of fisetin and bromocriptine treatment on liver cancer cell proliferation, migration and invasion. Whether the treatment of fisetin and bromocriptine influenced the clonogenic growth of HCC-LM3 and HepG2, colony-forming analysis was also carried out. In Fig. 2A and B, the invasion of liver cancer cells were apparently reduced due to fisetin and bromocriptine treatment in HCC-LM3 cells. Notably, fisetin and bromocriptine co-treatment could further downregulate the number of invaded cells, suggesting that fisetin might share similar molecular mechanism with bromocriptine to regulate liver cancer progression. Also, in HepG2 cells, fisetin and bromocriptine reduced cell invasion, which was further enhanced for fisetin and bromocriptine combination (Fig. 2A and C). Next, fisetin and bromocriptine obviously reduced HCC-LM3 cell migration. Also, intensively suppressive role of fisetin and bromocriptine co-treatment in cell migration inhibition was observed (Fig. 2D and E). In addition, fisetin and bromocriptine could considerably downregulate HepG2 cell migration, which was promoted for fisetin and bromocriptine in combination (Fig. 2D and F). Finally, colony formation assays showed that fisetin and bromocriptine monotherapy significantly reduced the colony number of cancer cells compared to the control ones. Notably, combination of fisetin and bromocriptine markedly decreased the clonogenic growth of lung cancer cells of HCC-LM3 and HepG2 (Fig. 2G-I). The results illustrate the capability of fisetin and bromocriptine to suppress liver cancer cell invasion migration, and proliferation is apparently stronger than the effect of fisetin and bromocriptine separately performed in the present experiments, and fisetin, at least partly, could perform as bromocriptine in controlling liver cancer progression.

Apoptosis induction is known as a key mechanism, contributing to cell death, which is widely used to explore and find new therapeutic strategy (20). In this study, the flow cytometric results exhibited that the fisetin and bromocriptine significantly upregulated the apoptotic liver cancer cells HCC-LM3 and HepG2. Interestingly, fisetin and bromocriptine combination caused an obvious upregulation of apoptotic cells compared to the control ones (Fig. 3A-C). Next, the caspase activation of cancer cells after fisetin and bromocriptine and the co-treatment were determined through western blot analysis. As shown in Fig. 3D, fisetin markedly induced high cleavage of caspase-3 in a dose-dependent manner. Consequently, PARP was activated and apoptosis was induced. Significantly, fisetin at the highest concentration resulted in an obvious more intensive caspase-3 (Fig. 3E) and PARP (Fig. 3F) cleavage in liver cancer cells of HCC-LM3. Significantly, HCC-LM3 treated by bromocriptine at different concentrations could also stimulate caspase-3 and PARP cleavage, which was performed in a dose-dependent manner (Fig. 3G-I). The results above show that caspase signaling pathway activation is involved in fisetin- and bromocriptine-induced apoptosis, which might be a possible molecular mechanism by which fisetin and bromocriptine exhibits strong antitumor effects.

EMT is known to play an important role in cancer metastasis (21). Essentially, TGF-β1 has been well reported to induce the process of EMT (22). Fig. 4A shows western blot analysis of TGF-β1 downregulated significantly compared to the control in HCC-LM3 cells after fisetin treatment, dose-dependently (Fig. 4C). In addition, vimentin (Fig. 4A and D), E-cadherin (Fig. 4A and E) and N-cadherin (Fig. 4A and F) were apparently reduced due to fisetin administration, which was in line with TGF-β1 expression. Importantly, bromocriptine indicated similar role in suppressing TGF-β1 (Fig. 4B and G), vimentin (Fig. 4B and H), E-cadherin (Fig. 4B and I) and N-cadherin (Fig. 4B and J) in HCC-LM3 cells. Furthermore, immunofluorescence analysis proved that TGF-β1 could be reduced in fisetin and bromocriptine treatment (Fig. 4K and L). The data above suggested that fisetin could ameliorate liver cancer progression via EMT inhibition through TGF-β1 signaling pathway.

To explore the role of fisetin and bromocriptine on VEGFR1 expression and to investigate the underlying molecular mechanism, VEGFR1, ERK1/2, p38 and pJNK expression levels were determined through western blot assays. As shown in Fig. 5A, we found that VEGFR1 (Fig. 5A and C), p-ERK1/2 (Fig. 5A and D), p38 (Fig. 5A and E) and Pjnk (Fig. 5A and F) expression levels in HCC-LM3 cells after fisetin treatment were downregulated markedly compared to the control ones. Also, in bromocriptine-treated HCC-LM3 cells, reduced protein levels of VEGFR1 (Fig. 5B and G), p-ERK1/2 (Fig. 5B and H), p38 (Fig. 5B and I) and pJNK (Fig. 5B and J) were observed. The data above indicated that fisetin could perform as bromocriptine, showing suppressive role in liver cancer progression via VEGFR1 and EMT-related signaling pathway inhibition.

In this regard, the role of fisetin i.p. injection in vivo study was evaluated. As shown in Fig. 6A and B, fisetin administration significantly reduced the weight of tumors, isolated from mice with orthotopically implanted tumors. Also, survival analysis showed that fisetin treatment significantly prolonged the survival time of mice with orthotopically implanted tumors in comparison to the control ones (Fig. 6C). Finally, DA levels were measured via ELISA kits. In the serum (Fig. 6D) and tumor tissue (Fig. 6E) from mice with orthotopically implanted tumors, DA was expressed highly, which was downregulated significantly after fisetin treatments in a dose-dependent manner.

Next, immunohistochemical analysis was used to detect Ki-67, and VEGFR1 levels from tumor specimens. As shown in Fig. 7A and B, Ki-67 was significantly downregulated due to fisetin administration, which was dose-dependent. Similarly, VEGFR1 was also impeded in fisetin-treated group, which was in line with the results in vitro (Fig. 7C and D). TGF-β1 was reduced in tumor tissue samples isolated from fisetin-treated mice through immunofluorescent analysis (Fig. 7E and F). The data above indicated that fisetin could suppress liver cancer development, which was related to death receptor signaling.