ATRA and TGF-β (Sigma-Aldrich; Merck KGaA) were prepared as 0.4 and 50 ng/ml stock solutions in DMSO, respectively, and were stored below −20°C in the dark. ATRA and TGF-β were diluted to 10–200 µM and 1 ng/ml, respectively, in DMEM (Sigma-Aldrich; Merck KGaA) containing 10% FBS (Gibco; Thermo Fisher Scientific, Inc.) on the day of the experiment. The highest concentration of DMSO in the test solutions was 0.1%. To exclude the possibility that proliferation may be inhibited by DMSO, all cells were exposed to a final DMSO concentration of 0.1% in DMEM containing 10% FBS.

Primary HConFs (ScienCell Research Laboratories, Inc.) were cultured according to the manufacturer's instructions; three individual lots of HConFs were obtained. The HConFs were maintained and cultured at 37°C in fibroblast medium (ScienCell Research Laboratories, Inc.) containing 2% FBS, fibroblast growth supplement (ScienCell Research Laboratories, Inc.), 100 U/ml penicillin and 100 µg/ml streptomycin in a 5% CO₂ humidified incubator. The HConFs were characterized by a spindle-shaped morphology and were positively stained with anti-fibronectin antibodies.

A HConF proliferation assay was performed as previously described (17). Briefly, HConF suspensions (0.5×10⁴ cells/well) were cultured in fibroblast medium in a 96-well plate (200 µl/well) for 24 h at 37°C. ATRA (0.01–10 µM) was added to the fibroblast medium and the cells were cultured for a further 48 h at 37°C in the absence or presence of TGF-β (1 ng/ml), with 0.1% DMSO as the control. The concentrations of ATRA and TGF-β used were determined according to a previous study (15). Subsequently, each well was incubated with 10 µl Cell Counting Kit-8 solution (BestBio; Sigma) for a further 3 h at 37°C. The absorbance was measured at 450 nm using an automated microplate reader (model 3001–1387; Thermo Fisher Scientific, Inc.).

HConF apoptosis was determined using an Annexin V-FITC apoptosis kit (BestBio) as previously described (17). Briefly, the HConFs (5×10⁵ cells/well) were plated in 6-well plates and cultured for 48 h. After rinsing twice with PBS, the cells were resuspended in 400 µl 1X binding buffer [10 mM HEPES, 140 mM sodium chloride, 2.5 mM calcium chloride (pH 7.4)], into which 5 µl of Annexin V-FITC was added. After 15 min incubation at 2–8°C in the dark, 10 µl of propidium iodide (BestBio) was added to the cells prior to further incubation for 5 min at 2–8°C in the dark. Within 15 min after staining, the cells were analyzed using a flow cytometer (Cytomics FV 500) and CytExpert 2.0 software (both Beckman Coulter, Inc.). The apoptotic rate was calculated as the sum of the percentage of early + late apoptotic cells.

HConFs were seeded at a density of 5×10⁵ cells/well in 6-well plates. The culture medium for the HConFs was replaced after 24 h with serum-free medium, and then cells were incubated for a further 2 h at 37°C. Next, a sterile 20-µl pipette tip was used to scratch a line in the confluent cell monolayer, after which the cells were washed three times with PBS. The scratch wound healed after 24 h of incubation in the following conditions: 1 µM ATRA + 1 ng/ml TGF-β, 1 ng/ml TGF-β and fibroblast medium without ATRA and TGF-β. The effects on HConF migration were evaluated by measuring the area of the wound from the images captured at a magnification of ×100 at 0 and 24 h using a light microscope (Olympus Corporation); analysis was performed using ImageJ version 1.5 (National Institutes of Health).

A chemomigration assay was performed using Transwell plates (pore size, 8 µm) as previously described (18). Briefly, the cells in the upper Transwell chamber (1×10⁵) were suspended in 200 µl of DMEM, and DMEM containing 20% FBS was added to the lower chamber. Following a 12-h incubation at 37°C, the medium with non-migrated cells in the upper chamber was removed with a cotton swab. The cells that had migrated to the lower chamber were fixed with 4% paraformaldehyde for 30 min at 37°C and then stained with 0.5% crystal violet for 10 min at 37°C. The cells were counted at ×200 magnification using a light microscope in six different fields of view.

HConFs were incubated in fibroblast medium in 6-well plates for 24 h. Then, the medium was replaced with the serum-free medium. Serum-starved cells were incubated for 6 h in the presence or absence of ATRA (1 µM), and then for 48 h in the presence or absence of TGF-β (1 ng/ml). Then, cell lysates were analyzed via western blotting.

Western blot analysis was performed as previously described (17,19,20). Cells were washed with pre-cooled PBS and lysed with RIPA buffer (Nanjing KeyGen Biotech Co., Ltd.) containing the protease inhibitor phenylmethylsulfonyl fluoride and the phosphatase inhibitor sodium orthovanadate (Nanjing KeyGen Biotech Co., Ltd.) on ice for 30 min. Subsequently, the cells were gently scraped from the plate and centrifuged at 1,500 × g for 12 min at 4°C. Protein concentrations were measured using the bicinchoninic acid method. A total of 20 µg/sample of protein was separated via 6–15% SDS-PAGE and then transferred onto PVDF membranes. Membranes were blocked with 5% non-fat dry milk for 1 h at 37°C before overnight incubation at 4°C with mouse monoclonal anti-collagen I (1:2,500; cat. no. ab88147; Abcam), rabbit polyclonal anti-fibronectin (1:1,500; cat. no. ab137720; Abcam), mouse antibodies against PI3K p85α (1:500; cat. no. sc-1637), phosphorylated (p)-PI3K p85α (1:500; cat. no. sc-12929), AKT (1:500; cat. no. sc-5298) and p-AKT (1:500; cat. no. sc-293125; all from Santa Cruz Biotechnology, Inc.), and mouse monoclonal anti-GAPDH (1:1,000; cat. no. A01020; Abbkine Scientific Co., Ltd.). Each membrane was incubated with anti-rabbit (1:5,000; cat. no. A0208) or anti-mouse (1:5,000; cat. no. A0216) horseradish peroxidase-conjugated secondary antibodies (both from Beyotime Institute of Biotechnology) for 1 h at room temperature. The blots were visualized using ECL reagent (Beyotime Institute of Biotechnology) and the bands were analyzed using ImageJ software.

HConFs were incubated in fibroblast medium in 6-well plates for 24 h, then the medium was replaced with serum-free medium. Serum-starved cells were incubated with 10 µM LY294002 (Calbiochem; Merck KGaA) for 1 h at 37°C. Subsequently, the cells were treated with 1 ng/ml TGF-β for 48 h at 37°C. The effects of the PI3K inhibitor on the TGF-β-induced expression of collagen I and fibronectin in HConF were investigated via western blot analysis.

Data analysis was performed using SPSS version 19.0 (IBM Corp.). The data are presented as the mean ± SD. Each experiment was repeated at least three times. Statistical analysis was performed using Student's t-test or one-way ANOVA; following ANOVA, the least significant difference test was used for pairwise comparisons between groups. P<0.05 was considered to indicate a statistically significant difference.

The effect of ATRA on HConF proliferation was examined. The cells were incubated for 48 h with 0.01–10 µM ATRA in the absence or presence of 1 ng/ml TGF-β with 0.1% DMSO as the control. ATRA was revealed to inhibit HConF proliferation in a concentration-dependent manner (P<0.05; Fig. 1A). HConFs were divided into three treatment groups: The ATRA group (1 µM ATRA + 1 ng/ml TGF-β), the TGF-β group (1 ng/ml TGF-β) and the control group (0.1% DMSO). ATRA inhibited TGF-β-induced HConF proliferation by 77.50±1.88% (P<0.01 vs. TGF-β; Fig. 1B).

The effect of ATRA on HConF apoptosis was examined using flow cytometry. A significantly increased number of apoptotic HConFs were observed in the ATRA group compared with the control group (53.25±1.2 vs. 22.5±1.1%, respectively; P<0.01). The TGF-β group showed a significantly decreased apoptotic rate compared with the control group (14.75±1.4%; P<0.01; Fig. 2).

The migratory ability of the HConFs was evaluated using in vitro wound healing and Transwell assays. Similar results were observed for the two assays. The ATRA group exhibited a ~30% reduction in wound healing compared with the control group (48.9±1.34 vs. 71.30±1.55%, respectively; P<0.05). Wound healing was increased in the TGF-β group compared with the control group (90.50±1.22%; P<0.05; Fig. 3A). Reduced HConF migration was observed for the ATRA group (14.85±1.13 cells; P<0.01), whereas significantly increased migration was noted for the TGF-β group compared with the control group (135.55±1.12 cells vs. 28.65±1.02 cells, respectively; P<0.01; Fig. 3B) in the Transwell migration assays.

The effect of ATRA on TGF-β-induced ECM production was investigated. Western blotting analysis and densitometric analysis revealed that exposure of HConFs to 1 ng/ml TGF-β for 48 h induced the production of collagen I and fibronectin, whereas 1 µM ATRA inhibited TGF-β-induced synthesis of collagen I and fibronectin by HConFs (P<0.01; Fig. 4).

The effect of ATRA on TGF-β-induced PI3K and AKT phosphorylation in HConFs was examined (Fig. 5). Western blotting analysis and densitometric analysis revealed that the exposure of HConFs to 1 ng/ml TGF-β for 48 h induced the phosphorylation/activation of PI3K and AKT. Treatment with 1 µM ATRA inhibited TGF-β-induced PI3K and AKT phosphorylation, indicating that ATRA inhibited the TGF-β-induced PI3K/AKT signaling pathway (P<0.05; Fig. 5).

The effect of the PI3K inhibitor LY294002 on the TGF-β-induced expression of collagen I and fibronectin in HConF was investigated. Cells were incubated with 10 µM LY294002 for 1 h before treatment with 1 ng/ml TGF-β for 48 h. Western blotting analysis and densitometric analysis revealed that LY294002 significantly inhibited TGF-β-induced expression of collagen I and fibronectin in HConFs (P<0.05; Fig. 6). The TGF-β-induced expression of collagen I and fibronectin in HConFs was inhibited by 27 and 47% in the presence of LY294002, respectively. The inhibitor had no effect on collagen I and fibronectin expression in the absence of TGF-β (data not shown).