DMEM (high glucose), trypsin and FBS were purchased from Gibco; Thermo Fisher Scientific, Inc. Standardized PQ powder and LY294002 were purchased from Sigma-Aldrich; Merck KGaA. Anti-PERK (cat. no. ab229912), anti-eukaryotic initiation factor 2α (eIF2α; cat. no. ab169528), anti-phosphorylated (p)-eIF2α (cat. no. ab32157), anti-HSPA5 (cat. no. ab108615), anti-α-SMA (cat. no. ab119952), anti-PI3K (cat. no. ab32089), anti-p-PI3K (cat. no. ab182651) and anti-GAPDH (cat. no. ab8245) primary antibodies were obtained from Abcam. Anti-GSK-3β (cat. no. 12456), anti-p-GSK-3β (cat. no. 5558), anti-AKT (cat. no. 9272), anti-p-AKT (cat. no. 4060) and anti-E-cadherin (cat. no. 14472) primary antibodies were purchased from Cell Signaling Technology, Inc. HRP-labeled secondary antibody (cat. nos. A0216 and A0208) and the anti-p-PERK (Thr982; cat. no. AF5902) antibody were purchased from Beyotime Institute of Biotechnology. Highly sensitive ECL reagent and PVDF membranes were obtained from Bio-Rad Laboratories, Inc. Lipofectamine 2000^® reagent was purchased from Invitrogen; Thermo Fisher Scientific, Inc., while small interfering RNA (siRNA/si) was obtained from Shanghai GenePharma Co., Ltd.

Human lung adenocarcinoma epithelial cells (A549) and rat alveolar type II cells (RLE-6TN) were purchased from the American Type Culture Collection. A549 cells are a suitable cell model that display numerous properties in common with human alveolar epithelial cells; therefore, they are often used to research the mechanism of pulmonary fibrosis (34,35). A549 cells were cultured in DMEM (high glucose) supplemented with 10% heat-inactivated FBS, while RLE-6TN cells were cultured in F-12 medium (Gibco; Thermo Fisher Scientific, Inc.) supplemented with 10% heat-inactivated FBS. A549 and RLE-6TN cells were maintained at 37°C in a humidified incubator containing 5% CO₂. Cells were treated with PQ (800 µmol/l for A549 cells and 160 µmol/l for RLE-6TN cells; dissolved in PBS) for 24 h. The morphological alterations of cells were observed using phase contrast microscopy (Thermo Fisher Scientific, Inc.).

Following treatment with siRNA or PQ, total protein was extracted from cells using RIPA lysis buffer (Beyotime Institute of Biotechnology) and total protein was quantified using a BCA protein assay kit (Beyotime Institute of Biotechnology). Proteins (50 µg per lane) were separated via 8% SDS-PAGE and then transferred onto PVDF membranes, which were blocked with 5% non-fat milk in TBST (0.05% Tween 20) for 2 h at room temperature. The membranes were then incubated at 4°C overnight with the following primary antibodies: Anti-PERK (1:1,000), anti-p-PERK (1:1,000), anti-eIF2α (1:1,000), anti-p-eIF2α (1:1,000), anti-HSPA5 (1:1,000), anti-E-cadherin (1:500), anti-α-SMA (1:200), anti-PI3K (1:1,000), anti-p-PI3K (1:1,000), anti-AKT (1:1,000), anti-p-AKT (1:1,000), anti-GSK-3β (1:200), anti-p-GSK-3β (1:200) and anti-GAPDH (1:500). Following the primary antibody incubation, the membranes were incubated with the appropriate HRP-conjugated secondary antibody (1:3,000) at room temperature for 2 h. Protein bands were visualized using ECL reagent and densitometric analysis was performed using ImageJ software (version 1.52g; National Institutes of Health). All experiments were repeated at least three times.

A549 (2×10⁴/well) and RLE-6TN (5×10⁴/well) cells were seeded into 6-well plates and divided into four groups: i) sicontrol (transfected with scrambled RNA); ii) siPERK; iii) sicontrol + PQ; and iv) siPERK + PQ. Cells were transfected with 200 pmol siRNA (sicontrol or siPERK) using Lipofectamine 2000^® (Invitrogen; Thermo Fisher Scientific, Inc.) according to the manufacturer's protocol at 37°C in a humidified incubator containing 5% CO₂. For A549 cells, the sequence of siPERK was 5′-GAAGCUACAUUGUCUAUUU-3′ and the sequence of sicontrol was 5′-AACCACUCAACUUUUUCCCAA-3′. For RLE-6TN cells, the sequence of siPERK was 5′-AAGUAGAAGAGACCAUGCCUGCUCC-3′ and the sequence of sicontrol was 5′-ACGUGACACGUUCGGAGAATT-3′. At 48 h post-transfection, 800 µmol/l (for A549 cells) or 160 µmol/l (for RLE-6TN cells) PQ (dissolved in PBS) was added to the sicontrol + PQ and siPERK + PQ groups for 24 h at 37°C in a humidified incubator containing 5% CO₂. The doses of PQ were selected according to our previous study (14).

Total RNA was extracted from A549 and RLE-6TN cells using RNAiso Plus reagent (Takara Biotechnology Co., Ltd.) according to the manufacturer's protocol. The concentration of total RNA was determined using an ultraviolet spectrophotometer. Total RNA was reverse transcribed into cDNA using a HiScript II Q RT SuperMix for qPCR (Vazyme Biotech Co., Ltd.) according to the manufacturer's instructions. qPCR was subsequently performed using a ChamQ™ SYBR qPCR Master mix (Vazyme Biotech Co., Ltd.) on an ABI ViiA™ 7 Real-Time PCR system (Applied Biosystems; Thermo Fisher Scientific, Inc.). The following thermocycling conditions were used for qPCR: 95°C for 2 min, 60°C for 30 sec and 72°C for 30 sec. The following primer pairs for β-actin and PERK were provided by Sangon Biotech Co., Ltd.: Human PERK forward, 5′-GGACCTCAAGCCATCCAACA-3′ and reverse, 5′-TCCTGGTCCATTGCAGTCAC-3′; human β-actin forward, 5′-CTGGAACGGTGAAGGTGACA-3′ and reverse, 5′-AAGGGACTTCCTGTAACAATGCA-3′; rat PERK forward, 5′-GGAAACGAGAGCCGGATTTATT-3′ and reverse, 5′-ACTATGTCCATTATGGCAGCTTC-3′; and rat β-actin forward, 5′-AGGATGCAGAAGGAGATTACTGC-3′ and reverse, 5′-AAAACGCAGCTCAGTAACAGTGC-3′. mRNA expression levels were quantified using the 2^−ΔΔCq method (36).

A549 (5×10⁵/well) cells were incubated with anti-E-cadherin (1:50) or anti-α-SMA (1:50) primary antibodies at 4°C overnight, washed with TBST (0.05% Tween-20) for 5 min at room temperature thrice, fixed with 4% paraformaldehyde (Beyotime Institute of Biotechnology) for 10 min at room temperature, blocked with 5% BSA (Beyotime Institute of Biotechnology) for 2 h at room temperature and incubated with fluorescent secondary antibodies (Alexa Fluor 488-labeled Goat Anti-Mouse IgG and Alexa Fluor 647-labeled Goat Anti-Mouse IgG; 1:200) in a humidified chamber for 2 h at 37°C. The cell nuclei were stained with 4′,6-diamidino-2-phenylindole at room temperature for 5 min. Stained cells were visualized using a laser confocal microscope (Leica TCS SP8; Leica Microsystems GmbH).

A549 (2×10⁴/well) were cultured in 6-well plates and transfected with siPERK. After 48 h, PQ (800 µmol/l) was added to treat the cells in the corresponding groups for 24 h at 37°C in a humidified incubator containing 5% CO₂. At 70% confluence, a scratch was then made in the center of the cell monolayer with a 10-µl Eppendorf pipette tip. The culture medium was replaced with FBS-free medium and cells were visualized under a light microscope. The change in the width of the scratch was photographed at 0 and 24 h using an EVOS cell imaging system (Thermo Fisher Scientific, Inc.).

LY294002 (Selleck Chemicals), a PI3K inhibitor, was used to block the PI3K/AKT signaling pathway (37). Briefly, 20 µM LY294002 was dissolved with 0.1% DMSO and added into the cell culture medium of both cell lines (2×10⁴/well for A549 and 5×10⁴/well for RLE-6TN) seeded into 6-well plates, while cells exposed to the corresponding concentration of DMSO (0.1%) were used as the control at 37°C. Following 24 h of LY294002 or DMSO incubation, the cells were treated with PQ (800 µmol/l for A549 and 160 µmol/l for RLE-6TN) for 24 h at 37°C. Subsequently, cells were collected by digestion with trypsin followed by centrifugation at 1,000 × g for 3 min at 4°C.

Statistical analysis was performed using SPSS 16.0 software (SPSS, Inc.). All data are presented as the mean ± SD of three independent experiments. Statistical comparisons between two groups were performed using an unpaired Student's t-test. Multigroup comparisons were performed using a one-way ANOVA followed by a Bonferroni's correction post hoc test. P<0.05 was considered to indicate a statistically significant difference.

Our previous study indicated that the expression levels of HSPA5, an ER stress-marker protein, were significantly upregulated following 2 h of PQ poisoning (24). To validate whether ER stress-related signals exerted a role in PQ-induced lung injury, the present study performed western blotting to analyze the expression levels of proteins involved in ER stress in PQ-treated A549 and RLE-6TN cells. The results revealed that the expression levels of HSPA5 were significantly upregulated following PQ treatment compared with the control group in both cell lines (Fig. 1A, B, D and E). In addition, the protein expression levels of PERK, p-PERK/PERK and p-eIF-2α/eIF-2α, which are all involved in ER stress-related signaling (38,39), were all significantly upregulated in the PQ group compared with the control group in both cell lines (Fig. 1A-E). These results suggested that PERK signaling in ER stress was activated during PQ poisoning.

A previous study indicated that ER stress may be involved in cell differentiation and apoptosis (40). To evaluate whether PQ induced pulmonary fibrosis through the PERK-mediated signaling of ER stress, the present study blocked PERK signaling by transfection with siPERK in both cell lines. The expression levels of PERK mRNA in the siPERK group were significantly decreased compared with those in the sicontrol group. The mRNA expression levels of PERK were significantly downregulated in the siPERK + PQ group compared with the sicontrol + PQ group in both cell lines (Fig. 2A and B). In addition, the protein expression levels of PERK and p-PERK/PERK were significantly downregulated in the siPERK + PQ group compared with the sicontrol + PQ group (Fig. 2C and D). In A549 cells, the expression of p-eIF-2α/eIF-2α was downregulated in the siPERK + PQ group compared with the sicontrol + PQ group. Meanwhile, in the siPERK + PQ group, the protein expression levels of E-cadherin (an epithelial marker) were upregulated, while the protein expression levels of α-SMA (a mesenchymal marker) were downregulated compared with the sicontrol + PQ group (Fig. 2C and D). Similar results were obtained for RLE-6TN cells (Fig. 2F-H). Immunofluorescence analysis revealed that the expression levels of E-cadherin were markedly upregulated in the siPERK + PQ group compared with the sicontrol + PQ group, wheras the expression levels of α-SMA were notably downregulated at 24 h in A549 cells in the siPERK + PQ group compared with the sicontrol + PQ group (Fig. 3A). A549 and RLE-6TN cells were observed to undergo transition from a polygonal to a fusiform morphology in the sicontrol + PQ group compared with the sicontrol group under phase contrast microscopy; however, this change was attenuated in the siPERK + PQ group compared with the sicontrol + PQ groups (Fig. 3B). The results of the wound healing assay demonstrated that cell migration in the sicontrol + PQ group was increased compared with the sicontrol group, while cell migration in the siPERK + PQ group was markedly decreased compared with the sicontrol + PQ group (Fig. 3C). These data indicated that PQ-induced EMT may be regulated by PERK signaling, which is an ER stress-regulated signaling pathway.

The results of our previous study demonstrated that PERK-regulated ER stress had a significant effect on PQ-induced EMT; however, the underling mechanism remained unclear (24). The expression levels of proteins associated with the PI3K/AKT/GSK-3β signaling pathway were subsequently determined via western blotting following the knockdown of PERK and PQ poisoning. The total proteins of GSK-3β, AKT and PI3K in each group displayed no significant differences (Fig. 4A and B). The results revealed that PERK silencing significantly downregulated the protein expression levels of p-GSK-3β/GSK-3β, p-AKT/AKT and p-PI3K/PI3K in the siPERK + PQ group compared with the sicontrol + PQ group in both cell lines (Fig. 4A and C). Thus, it was suggested that PQ may induce EMT through the PERK-mediated PI3K/AKT/GSK-3β signaling pathway.

A recent study indicated that the PI3K/AKT/GSK-3β signaling pathway, which can mediate survival, migration and apoptosis, also played an important role in TGF-β1-induced EMT (41). Therefore, the present study investigated the expression levels of proteins related to the PI3K/AKT/GSK-3β signaling pathway in A549 and RLE-6TN cells following treatment with a PI3K-specific inhibitor, and investigated its role in PQ poisoning. The total proteins of GSK-3β,AKT and PI3K in each group displayed no significant differences (Fig. 5A, B, D and E). The present results revealed that the protein expression levels of p-PI3K/PI3K, p-AKT/AKT and p-GSK-3β/GSK-3β were significantly upregulated in the DMSO + PQ group compared with the DMSO group in A549 (Fig. 5A and C)and RLE-6TN cells (Fig. 5D and F). To verify the role of the PI3K/AKT/GSK-3β signaling pathway in PQ-induced EMT, the PI3K-specific inhibitor, LY294002, was used to block PI3K/AKT signaling. The results revealed that LY294002 partially reversed the PQ-induced upregulation in p-GSK-3β, p-AKT and p-PI3K expression levels in both cell lines (Fig. 5A, C, D and F). In addition, LY294002 + PQ group partially alleviated the downregulated E-cadherin expression levels and upregulated α-SMA expression levels compared with the DMSO + PQ group (Fig. 5A, B, D and E). These results indicated that the PI3K/AKT/GSK-3β signaling pathway may regulate PQ-induced EMT.