The human NPC cell line, CNE-2 (poorly differentiated), was supplied from State Key Laboratory of Oncology (Sun Yat-sen University Cancer Center, Guangzhou, China). The cell lines were maintained in RPMI-1640 with 10% fetal bovine serum (FBS). Cells in the logarithmic phase were used in the experiments. The puquitinib mesylate (XC-302; chemical structure shown in Fig. 1) was obtained from Xinchang Pharmacy Corp. and dissolved in dimethyl sulfoxide (DMSO; Sigma-Aldrich, St. Louis, MO, USA) at a storage concentration of 40 mM.

In brief, tumor cells (3×10³/100 µl/well) were plated in 96-well plates and incubated for 24 h. Culture medium containing gradient concentrations of XC-302 (16–0.125 µM) were added to each well, and 0.1% DMSO was set as the negative control. MTT (5.0 mg/l; 20 µl) was added after the cells were incubated for 68 h, followed by the addition of 150 µl DMSO into each well to dissolve the dark blue crystals. The absorbance (A) was measured at wavelengths of 570 and 630 nm, respectively (Model-550; Bio-Rad, Hercules, CA, USA). Finally, the cell viability value was calculated using the following formula: (A_sample - A_blank)/(A_control - A_blank) × 100%. All the experiments were executed independently at least three times in triplicate.

The MDC assay was used to label preliminary autophagosomes (16). Cells grown on 6-well plates were treated with XC-302 (0.5–8 µM) for 24 h, incubated with 0.05 mM MDC for 30 min at 37°C and washed with phosphate-buffered saline (PBS). Fluorescence images were captured by an Olympus IX71 fluorescence microscope (Olympus, Center Valley, PA, USA).

The presence of autophagosomes in TEM is the standard for detecting autophagy. Cells grown on 6-well plates were treated with XC-302 (4 µM) and 24 h later were trypsinized and washed with PBS prior to fixing in fixative buffer. Subsequently, cells were collected by centrifugation at 500 × g for 10 min, suspended and incubated for 2 h in 2.5% glutaraldehyde. Following fixation, cell samples were treated with 2% osmium tetroxide in 0.1 M sodium cacodylate buffer, dehydrated through a graded series of acetone and embedded in resin. Finally, the samples were sliced into 65-nm sections, which were processed for TEM (Hitachi electron microscope H-600; Hitachi, Ltd., Toyko, Japan).

The GFP-LC3 expression vector was generously provided by Professor X.F. Zhu (State Key Laboratory of Oncology). Following transfection of the GFP-LC3 expression vector with Lipofectamine 2000 (Invitrogen) for 24 h, following the manufacturer's protocol, cells were divided into groups based as follows: i) Negative control with 0.1% DMSO (4 µM); ii) XC-302 (4 and 8 µM); iii) 3-MA (5 mM); and iv) 3-MA (5 mM) + XC-302 (4 and 8 µM). Following the indicated treatment, the localization of GFP was directly observed with a laser scanning confocal microscope.

Following treatment of various concentrations of XC-302 for different times, the total protein from the CNE-2 cells was obtained by lysing in cell lysis buffer (Cell Signaling Technology, Beverly, MA, USA). The proteins were resolved by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and transferred to a polyvinylidene fluoride membrane. The membranes were subsequently blocked with skimmed milk (5%) and incubated overnight at 4°C with the following antibodies: Total AKT (1:1,000, #9916, rabbit anti-human), mTOR, phospho-AKT (S473; 1:2,000, #9916, rabbit anti-human), phospho-mTOR (1:1,000, #5536, rabbit anti-human), LC3 (1:1,000, #4599, rabbit anti-human), beclin 1 (1:1,000, #3495, rabbit anti-human), p62 (1:1,000, #8025, rabbit anti-human) and glyceraldehyde 3-phosphate dehydrogenase (GAPDH; 1:3,000, #5174, rabbit anti-human), which were purchased from Cell Signaling Technology. The samples were incubated with a secondary antibody (1:4,000, #9916, anti-rabbit IgG; CST) for 1 h at room temperature and the labeled proteins were detected using chemiluminescence reagent and automatic X-ray film. Equal loading GAPDH was assessed as the internal control for western blot analysis.

The specific siRNA oligomers against beclin 1 (forward, 5′-CAGTTTGGCACAATCAATAtt-3′) and si-control (forward, 5′-UUCUCCGAACGUGUCACGUtt-3′) were purchased from the Gene Technology Co. (Shanghai, China). The CNE-2 cells were transfected with si-beclin 1 and Lipofectamine 2000 (Invitrogen, Thermo Fisher Scientific, Waltham, MA, USA) according to the manufacturer's protocol. After incubation for 12 h, the transient transfected CNE-2 were used for the following experiments.

The cells were grown for 24 h and subsequently treated for 6 h as follows: Groups without intervention of siRNA, i) negative control; ii) XC-302 (4 µM); iii) 3-MA (5 mM); and iv) 3-MA (5 mM) + XC-302 (4 µM); and groups with silencing of siRNA, i) si-control; ii) si-control cells with XC-302 (4 µM); iii) si-beclin 1; and iv) si-beclin 1 cells with XC-302 (4 µM). The cells were trypsinized and subsequently seeded in 6-well culture plates (500/well) for 2 weeks. The cells were washed and fixed with ice-cold methanol for 10 min, followed by the addition of 0.5% crystal violet solution for 10 min to observe the colony formation.

Briefly, the CNE-2 cells were treated with different concentrations of XC-302 (4 and 8 µM) and/or 5 mM 3-methyladenine (3-MA, M9281; Sigma-Aldrich) for 24 h. Following collection, the cells were stained with Annexin V-FITC and PI. The apoptotic cells were estimated using a Beckman-Gallios flow cytometer (Beckman-Gallios, Miami, FL, USA).

Whole data are exhibited as mean ± standard error of the mean of more than two independent experiments in each group. The variances between each group were calculated by Student's t-test and P<0.05 was considered to indicate a statistically significant difference.

To assess the effects of XC-302 on NPC cell proliferation in vitro, CNE-2 cells were treated with XC-302 at different concentrations for 72 h and subsequently evaluated by the MTT assays. Exposure to XC-302 showed a dose-dependent inhibition of cell viability. MDC is known as a specific marker of autophagic vacuoles (Fig. 2A). XC-302-treated CNE-2 cells resulted in fluorescence intensity enhanced with the increasing dose of the drug (Fig. 2B). In addition to autophagy, XC-302 treatment also induced apoptosis in the CNE-2 cells. The Annexin V-FITC/PI double staining showed that cells treated with XC-302 increased the percentage of apoptosis up to 14.2% (Fig. 2C). The TEM was adopted to further examine the autophagosomes of XC-302-treated cells. Compared with the control cells, XC-302 treatment not only resulted in a rapid increase of autophagosomes (thick arrow), but also induced the formation of autolysosomes (thin arrow) in a portion of CNE-2 cells (Fig. 2D).

Microtubule-associated protein 1 LC3 is a specific marker for autophagy. It is converted from the inactive form, LC3-I, to a cleaved form (LC3-II) during autophagy, and the LC3-II protein has been frequently used for autophagy detection. In the present study, the changes of the markers in autophagy were analyzed by western blotting analysis. The LC3-II protein levels were markedly increased by XC-302 treatment. The beclin 1 level was augmented and as a degradation product, the expression of p62 was decreased (Fig. 3A and B).

Subsequently, whether the downstream targets of PI3K could be inhibited by XC-302 was examined in the CNE-2 cell line. As shown in Fig. 3C, following exposure to XC-302 for 24 h, although the levels of AKT and mTOR did not exhibit significant changes, the phosphorylation levels of AKT and mTOR protein were attenuated when treated by XC-302 in a dose-dependent manner.

3-MA is a known specific inhibitor of autophagy, which is frequently used to detect the role of autophagy under various treatments. Thus, the effects of 3-MA was investigated on the apoptosis, autophagy, proliferation and clone formation of XC-302-treated CNE-2 cells. The apoptosis rate of cells were markedly decreased in cells co-treated with various concentrations of XC-302 and 3-MA, compared with those treated with XC-302 alone (P<0.05) (Fig. 4A and B). To detect the formation of autophagosomes specifically, cells were transfected with the GFP-LC3 plasmid transiently. Following treatment with XC-302, cells showed increased LC3 punctures compared with the control in a dose-dependent manner (Fig. 4C), visualized by fluorescence microscopy. In addition, there was a significant degradation of green fluorescence in XC-302 (8 µM) and 3-MA co-treated cells. These results corroborate the observation that XC-302 induced autophagy, as well as 3-MA decreased the accumulation of autophagosomes, in XC-302-exposed CNE-2 cells. The proliferation of the CNE-2 cells was inhibited by XC-302 and could be reversed by exposure to 3-MA after 24 or 48 h, as revealed by the MTT assay (P<0.05) (Fig. 5A). Subsequently, clone formation assays were used to further ensure that 3-MA reduced the sensitivity of the cells to XC-302. The group combining 5 mM 3-MA with 4 µM XC-302 formed more colonies compared with the individual use of XC-302 (P<0.05) (Fig. 5B and C). These results clearly reveal that autophagy contributes to XC-302-induced cell death in CNE-2 cells.

Beclin 1 is a critical regulator of autophagy, which can specifically suppress the autophagy pathway by knockdown of it. The beclin 1 gene was further knocked down using siRNA and the efficiency of the knockdown was confirmed by western blotting (Fig. 6A). Using the MTT assay, similar to the effect of 3-MA, the knockdown of beclin 1 resulted in a higher vital rate following exposure to XC-302 (P<0.05) (Fig. 6B). Additionally, clone formation is markedly increased in beclin 1 knockdown cells compared with the scramble control cells following the treatment of XC-302 (Fig. 6C and D). Taken together, these results revealed that the inhibition of autophagy by beclin 1 knockdown promoted proliferation and clone formation of CNE-2 cells that were exposed to XC-302.