Human lung A549, HCC-15 and Calu-3 cell lines (American Type Culture Collection, Manassas, VA, USA) were maintained in RPMI-1640 medium (Gibco; Thermo Fisher Scientific, Inc., Waltham, MA, USA) containing with 10% fetal bovine serum (FBS; Sigma-Aldrich; Merck KGaA, Darmstadt, Germany). During experimentation, cells were switched to RPMI containing 1% FBS.

Recombinant celastrol and chloroquine (20 µM) were obtained from Sigma-Aldrich; Merck KGaA (Darmstadt, Germany). TRAIL (200 ng/ml) was purchased from Abfrontier; Young in Frontier, Co., Ltd. (Seoul, South Korea).

A549, HCC-15 and Calu-3 cells were plated in 12-well plates and pre-exposed to celastrol (1, 2 and 4 µM) for 12 h in 37°C incubator, and were then additionally treated with TRAIL protein (200 ng/ml) for an additional 2 h. Cell morphology was assessed under a light microscope (Nikon Corporation, Tokyo, Japan, magnification, ×100), and cell viability was evaluated by a crystal violet staining method. Cells were stained with a staining solution (0.5% crystal violet in 30% ethanol and 3% formaldehyde) for 10 min at room temperature, washed four times with PBS, and were dried. Cells were then lysed with 1% SDS solution. The absorbance value was then measured at wavelength of 550 mm using a plate reader. Cell viability was expressed as relative dye intensity compared with that of the control.

Cell viability was evaluated by trypan blue exclusion assay (Sigma-Aldrich; Merck KGaA), using a hemocytometer. Following each treatment, the cells at 1.0×10⁴ cells/well in 12-well plates, were trypsinized and re-suspended in PBS. Trypan blue dye solution (0.4%) was added to the cell suspension for 5 min at room temperature. Unstained cells were viable and stained cells were dead. The total cell number and trypan blue-positive cells were counted using a light microscope in a blinded manner. The percentage of surviving cells was calculated using the formula: Number of stained cells/number of total cells ×100. Each treatment was performed in triplicate.

A549 cells (1.0×10⁴ cells/well) in 12-well plates, were pre-incubated with N-acetyl cysteine (NAC) for 1 h and then incubated with TRAIL alone or combined with CQ (10 mM). The formation of ROS was ascertained through application of the cell permeable fluorescent marker dihydroethidium (DHE). Briefly, cells were treated with 5 µM DHE for 30 min at 37°C in the dark. The fluorescence was then measured using a fluorescence plate reader at excitation and emission wavelengths of 518 and 605 nm, respectively.

The changes in ΔΨm were assessed using a cationic fluorescent marker. A549 cells were maintained on cover slips in a 24-well plate, incubated with 10 ml JC-1 at 37°C for 30 min and then washed with PBS. The cells were then mounted with DakoCytomation fluorescent mounting medium (Dako; Agilent Technologies, Inc., Santa Clara, CA, USA) and visualized under a fluorescence microscope (magnification, ×400).

A549 cells (5.0×10³ cells/well) were cultured on poly-L-lysine coated coverslips. Following differentiation and specific treatment, the cells were fixed with 4% paraformaldehyde at room temperature 15 min and permeabilized with 0.1% Triton X-100. The cells were then incubated for 60 min at room temperature with blocking solution (5% FBS in Tris-buffered saline) followed by overnight incubation at 4°C with anti-p62 (1:250; cat. no. PA5-20839; Invitrogen; Thermo Fisher Scientific, Inc.) and cleaved caspase-3 [(1:250; cat. no. 9665; Cell Signaling Technology, Inc., Danvers, MA, USA) antibodies. Subsequent to washing with PBS, the cells were incubated with secondary antibody (Alexa Fluor^® 488-conjugated donkey polyclonal anti-rabbit; 1:500; cat. no. A-21206; Thermo Fisher Scientific, Inc.; and Texas Red-X-conjugated goat polyclonal anti-mouse; 1:500; cat. no. T-6390; Thermo Fisher Scientific, Inc.) for 2 h in the dark. Finally, immunostaining was visualized under a fluorescence microscope (magnification, ×400).

Western blot analysis was performed as described previously (39). Briefly, immunoprecipitation assay buffer (Qiagen, Inc, Valencia, CA, USA) was used to extract total protein in A549 cells. The supernatant was collected by centrifugation (13,282 × g; 4°C; 10 min). The protein concentration was determined using the Pierce Bicinchoninic Protein Assay kit (Thermo Fisher Scientific, Inc.). Proteins (30 µg) were separated on 10% SDS-PAGE gels and blotted onto polyvinylidene fluoride membranes. Membranes were blocked with 5% non-fat dried milk at 25°C for 1 h, followed by incubation with primary antibodies overnight at 4°C. Antibodies against β-actin were purchased from Sigma-Aldrich; Merck KGaA, and those against cleaved caspase-8 were obtained from BD Pharmingen (BD Biosciences, Franklin Lakes, NJ, USA). Cleaved caspase-3 and LC3 antibodies were purchased from Cell Signaling Technology, Inc., and p62 antibodies were purchased from EMD Millipore (Billerica, MA, USA). Membranes were incubated with horseradish peroxidase conjugated secondary antibody (cat. no. 4410; 1:2,000; Cell Signaling Technology, Inc.) at 25°C for 1 h. The immune-reactive protein bands were visualized using an enhanced chemiluminescence detection system (GE Healthcare Life Sciences, Chalfont, UK). Densitometry of the signal bands was conducted using the Bio-1D densitometer (Vilber Lourmat, Eberhardzell, Germany). Images were examined using a Fusion-FX7 imaging system (Vilber Lourmat).

Statistical analysis was performed using GraphPad Prim (version 5.03; GraphPad Software, Inc., La Jolla, CA, USA). All experiments were performed in triplicate, and the data are expressed as the mean ± standard error. Significant differences between control and treated samples were analyzed using one-way analysis of variance followed by Duncan's post hoc test.

Alterations in cell morphologies were examined under a light microscope. Treatment with either celastrol or TRAIL alone did not or only marginally induced cell death (Fig. 1), and no morphological changes were observed. However, a combined regimen of TRAIL and different concentrations of celastrol markedly increased the number of apoptotic cell deaths compared with celastrol or TRAIL alone (Fig. 1A-D). These data indicate that celastrol promoted TRAIL-initiated apoptosis in A549 cells.

LC3-II and p62 expression increased following celastrol treatment (Fig. 2A-C). Immunofluorescence staining also demonstrated that varying doses of celastrol increased p62 protein levels (Fig. 2D). The combined regimen of TRAIL and celastrol increased active (Ac)-caspase 3 and Ac-caspase 8 levels (Fig. 2E-G). Immunofluorescent staining results also suggested that Ac-caspase 3 levels of combined celastrol and TRAIL treatment were increased than only TRAIL treatment (Fig. 2H), indicating that autophagy flux was inhibited by celastrol.

The cell morphology results indicated that increased apoptosis was achieved by co-treatment of TRAIL and celastrol or CQ (Fig. 3A). The combined regimen of CQ and TRAIL markedly increased cell death and attenuated cell viability (Fig. 3B and C). These results suggested that celastrol sensitized TRAIL-initiated cell death by attenuating autophagy flux.

LC3-II and p62 expression were markedly increased in A549 cells treated with celastrol or CQ alone, confirming that celastrol inhibits autophagy flux (Fig. 4A-C). Immunofluorescence staining results also demonstrated that p62 protein levels were increased (Fig. 4D). The combined regimen of TRAIL and CQ increased Ac-caspase 3 and Ac-caspase 8 protein levels (Fig. 4E-G). The immunofluorescent staining results also demonstrated that Ac-caspase 3 expression was increased (Fig. 4H). These results also indicated that the promotion of the TRAIL-initiated apoptotic mechanism by celastrol was due to the attenuation of autophagy flux.

As demonstrated in Fig. 5A, ROS levels were increased in cells treated with celastrol combined with TRAIL or CQ. These increases were effectively attenuated when the cells were pre-incubated with N-acetyl cysteine (NAC) for 1 h. Green fluorescence observed in the cells treated with celastrol combined with TRAIL or CQ suggested decreased ΔΨm values compared with that from the TRAIL alone treatment, but treatment with NAC restored these ΔΨm values (Fig. 5B). These data suggest that celastrol-mediated autophagy flux attenuation increased TRAIL-initiated apoptosis via increases in ROS generation and decreasing ΔΨm.

Celastrol or TRAIL treatment alone did not, or only marginally affected, the cell viability of Calu-3 and HCC-15 cells (Fig. 6). Nevertheless, the combined TRAIL and celastrol regimen significantly decreased the cell viability of Calu-3 and HCC-15 cells (Fig. 6A-F). These results suggested that celastrol significantly increased TRAIL-initiated apoptosis in Calu-3 and HCC-15 cells.