The JME/CF15 nasal epithelial cell line was obtained from The Cell Bank of Type Culture Collection of The Chinese Academy of Sciences, and cultured at 37°C (5% CO₂) in DMEM supplemented with 10% FBS (both Gibco; Thermo Fisher Scientific, Inc.) and 1% (v/v) penicillin/streptomycin (Sigma-Aldrich; Merck KGaA) at a density of 5×10⁶ cells per well.

PSO (batch no. 110739-201115; National Institutes for Food and Drug Control) was dissolved in DMSO (Sigma-Aldrich; Merck KGaA) to prepare a psoralen-conditioned medium stock solution. Then, 100, 20, 10 and 1 µM working stocks of PSO were prepared with low-glucose DMEM containing 10% FBS. After 2 h of PSO pretreatment, JME/CF15 cells were stimulated with 10 ng/ml IL-13 for 24 h at 37°C to generate a cell-based AR model. In this paper, cells were pretreated with 10 nM PMA for 24 h and 15 µl SP600125 for 24 h at 37°C, as outlined in previous studies (22,23). After giving different concentrations (1, 10 and 20 µm) of PSO, the cells were divided into the control, IL-13, 1 µM PSO + IL-13, 10 µM PSO + IL-13 and 20 µM PSO + IL-13 groups. The control group was given the same dose of DMEM. In another set of experiments, a concentration of 20 µM PSO was selected, and the cells were divided into the control, IL-13, PSO + IL-13, PMA + PSO + IL-13 and SP600125 + PMA + PSO + IL-13 groups.

According to the GEO (https://www.ncbi.nlm.nih.gov/geo/) database, the expression level of CST1 in individuals with AR was detected (GSE19187).

The CCK-8 system (Dojindo Molecular Technologies, Inc.) was used to assess cell viability. Cells were seeded into 96-well plates at a density of 5×10³ cells per well. After the relevant treatment, 10 µl CCK-8 solution was added to each well and incubated for 2 h, after which cell viability was assessed using a Benchmark microplate spectrometer (Bio-Rad Laboratories, Inc.).

Quantification of granulocyte-macrophage colony-stimulating factor (GM-CSF; cat. no. SGM00; R&D Systems, Inc.) and Eotaxin (cat. no. MME00; R&D Systems, Inc.) in cell supernatants (300 × g; 4°C; 10 min) was performed using an ELISA kit according to the manufacturer's instructions (24).

Cells (1×10³ cells/well) were cultured in 6-well plates and total RNA was extracted using TRIzol^® reagent (Invitrogen; Thermo Fisher Scientific, Inc.) according to the manufacturer's protocol. Total RNA (1 µg) was reverse-transcribed into first-strand complementary DNA using the SuperScript™ III Reverse Transcriptase kit (Invitrogen; Thermo Fisher Scientific, Inc.), according to the manufacturer's protocol, and then amplified in triplicate by qPCR (cobas Z 480 system; Roche Diagnostics) using SYBR Green (final reaction volume, 20 µl; Takara Biotechnology Co., Ltd.), according to the manufacturer's protocol. The following thermocycling conditions were used for qPCR: Initial denaturation at 95°C for 10 min; followed by 40 cycles of 95°C for 10 sec and 60°C for 60 sec. The following primers (GenScript) were used for qPCR: GM-CSF forward, 5′-CAGCCACTACAAGCAGCACT-3′ and reverse, 5′-GGGGATGACAAGCAGAAAGT-3′; Eotaxin forward, 5′-TGTCTCGTTCTCCCTCTGCT-3′ and reverse, 5′-CTCCGCTCACAGTCATTTCC-3′; IL-6 forward, 5′-GGCCCTTGCTTTCTCTTCG-3′ and reverse, 5′-ATAATAAAGTTTTGATTATGT-3′; IL-8 forward, 5′-ATGGCTGCTGAACCAGTAGA-3′ and reverse, 5′-CTAGTCTTCGTTTTGAACAG-3′; mucin 5AC (MUC5AC) forward, 5′-ATCACCGAAGGCTGCTTCTGTC-3′ and reverse, 5′-GTTGATGCTGCACACTGTCCAA-3′; and GAPDH forward, 5′-AGCCACATCGCTCAGACAC-3′ and reverse, 5′-GCCCAATACGACCAAATCC-3′. When evaluating the effects of treatment, the expression level of each control was assigned an arbitrary value of 1, and those of the treated cells were evaluated as a fold-change above the control, and calculated using the 2^−ΔΔCq method (25). GAPDH was used as the internal control gene.

Total cellular protein was extracted using RIPA buffer, and quantified using a BCA assay (both Beyotime Institute of Biotechnology). Cell lysates containing 50–100 µg protein were resolved by electrophoresis on 10% SDS-PAGE gels (Beyotime Institute of Biotechnology). The separated proteins were subsequently transferred to PVDF membranes (Thermo Fisher Scientific, Inc.), which were then blocked in 5% non-fat milk for 1 h at room temperature, and subsequently incubated overnight at 4°C in 0.25% non-fat milk containing the appropriate primary antibodies. Primary antibodies against the following targets were used in the present study: IL-6 (1:1,000; cat. no. ab6672), IL-8 (1:1,000; cat. no. ab18672), MUC5AC (1:1,000; cat. no. ab3649), phosphorylated (p)-c-Fos (1:1,000; cat. no. ab27793), c-Fos (1:1,000; cat. no. ab222699), p-c-Jun (1:1,000; cat. no. ab30620), c-Jun (1:1,000; cat. no. ab32137), CST1 (1:1,000; cat. no. ab124281) and GAPDH (1:1,000; cat. no. ab8245). All primary antibodies were purchased from Abcam. On the second day, the membranes were incubated with the secondary antibody (1:5,000; cat. no. ab150077; Abcam) for 2 h at room temperature. The protein bands were visualized using enhanced chemiluminescence reagents (Thermo Fisher Scientific, Inc.). Protein band intensity was determined using ImageJ software (version 146; National Institutes of Health).

Cellular ROS levels were detected using a fluorescent probe, 2′,7′-dichlorodihydrofluorescein diacetate (DCFH-DA; Sigma-Aldrich; Merck KGaA), which is rapidly oxidized into the highly fluorescent 2′,7′-dichlorofluorescein (DCF) in the presence of intracellular ROS. Fluorescence was monitored with a laser scanning confocal microscope (magnification, ×200; Leica Microsystems GmbH) at 488 nm. ROS levels were quantified as the relative fluorescence intensity of DCF per cell in the scanned area.

All experiments were repeated three times. The data were analyzed using SPSS version 19.0 (IBM Corp) and GraphPad 6.0 (GraphPad Software, Inc.), and are presented as the mean ± SD. Comparisons among multiple groups were analyzed using one-way ANOVA followed by Tukey's post hoc test. P<0.05 was considered to indicate a statistically significant difference.

JME/CF15 cells were induced using different concentrations of PSO (0, 1, 10, 20 and 100 µM), and cell viability was assessed using an MTT assay. As shown in Fig. 1A, normal cells exhibited marked damage following treatment with 100 µM PSO; therefore, a concentration gradient of 1, 10, and 20 µM PSO was used for subsequent experimentation. The cells were divided into the control, IL-13, 1 µM PSO + IL-13, 10 µM PSO + IL-13 and 20 µM PSO + IL-13 groups, and inflammatory responses were detected by ELISA. Compared with the control group, the expression levels of GM-CSF (Fig. 1B and C) and Eotaxin (Fig. 1D and E) were significantly increased in the IL-13 group, indicating that an inflammatory response had occurred. Compared with the IL-13 group, GM-CSF and Eotaxin expression in the 1 µM PSO + IL-13, 10 µM PSO + IL-13 and 20 µM PSO + IL-13 groups were downregulated in a dose-dependent manner. RT-qPCR (Fig. 1F) and western blotting (Fig. 1G) were used to detect the mRNA and protein expression of IL-6 and −8, and the expression trends were the same as those observed for GM-CSF and Eotaxin. Cellular ROS expression was detected using a DCFH-DA probe, and was found to be increased in the IL-13 group compared with the control group. Compared with the IL-13 group, ROS expression in the PSO-treated groups was decreased in a dose-dependent manner (Fig. 1H and I). These results indicated that PSO exerted dose-dependent inhibition of the IL-13-induced inflammatory response in JME/CF15 cells.

Cellular expression of MUC5AC, a representative mucus-producing protein, was also detected to determine whether PSO was able to influence IL-13-induced mucus production. Compared with the control group, MUC5AC expression was significantly increased in the IL-13 group, and decreased in a dose-dependent manner following treatment with different concentrations of PSO (Fig. 2A and B). The results confirmed that IL-13 induced mucus production in JME/CF15 cells, which was subsequently inhibited by PSO.

In the present study, phosphorylation levels of the AP-1 pathway-associated proteins c-Fos and c-Jun were found to be abnormally altered. Compared with the control group, the levels of p-c-Fos and p-c-Jun were significantly increased in the IL-13 group, indicating that the AP-1 pathway had been activated. After the addition of PSO, the levels of p-c-FOS and p-c-Jun were decreased in a dose-dependent manner, compared with those in the IL-13 group (Fig. 3A). Subsequently, the AP-1 pathway activator PMA and the pathway inhibitor SP600125 were used to further assess whether the regulatory effects of PSO on AR were achieved through the AP-1 pathway. A concentration of 20 µM PSO was selected, and the cells were divided into the control, IL-13, PSO + IL-13, PMA + PSO + IL-13 and SP600125 + PMA + PSO + IL-13 groups. Western blot analysis was used to detect the expression of AP-1 pathway proteins. Compared with the PSO + IL-13 group, the levels of p-c-Fos and p-c-Jun were significantly increased in the PMA + PSO + IL-13 group (Fig. 3B), and the expression of GM-CSF and Eotaxin were also increased (Fig. 4A-D). Furthermore, the expression levels of IL-6 and −8 (Fig. 4E and F), ROS (Fig. 4G and H) and MUC5AC (Fig. 5A and B) were all increased. These results indicated that PMA reversed the inhibitory effects of PSO on p-c-FOS, p-c-Jun, IL-13-induced inflammation and mucus production in JME/CF15 cells. Compared with the PMA + PSO + IL-13 group, the levels of c-Fos and c-Jun phosphorylation in the SP600125 + PMA + PSO + IL-13 group were reduced (Fig. 3B), and the expression of GM-CSF, Eotaxin (Fig. 4A-D), inflammatory cytokines IL-6 and IL-8 (Fig. 4E and F), ROS (Fig. 4G and H) and MUC5AC (Fig. 5A and B) were all decreased. These results suggested that PSO suppressed inflammation and mucus production in IL-13-induced JME/CF15 cells by inhibiting the AP-1 signaling pathway.

CST1 is a targeted regulator of the AP-1 pathway (6). In the present study, the expression of CST1 in IL-13-induced cells was significantly increased compared with that in the control group. Compared with the IL-13 group, the expression of CST1 in the PSO + IL-13 group was decreased, indicating that PSO inhibited the expression of CST1. Furthermore, compared with the PSO + IL-13 group, CST1 expression was increased in the PMA + PSO + IL-13 group, and compared with the PMA + PSO + IL-13 group, CST1 expression was decreased in the SP600125 + PMA + PSO + IL-13 group (Fig. 6). Collectively, these findings indicated that PSO downregulated the expression of CST1 by inhibiting the AP-1 signaling pathway, thus suppressing the IL-13-induced inflammatory response and mucus production in nasal mucosal epithelial cells.