The human NPC cell lines HONE-1 and CNE-1 were grown in RPMI-1640 medium (Gibco, USA) supplemented with 10% fetal bovine serum (FBS) (Hyclone, Logan, UT, USA). All cells were cultured in a 5% CO₂ incubator at 37°C. The working stock of RAD001 (Selleck Chemicals, USA) was diluted to 20 mM using dimethyl sulfoxide (DMSO) and stored at −20°C. The concentration of DMSO in the final solution did not exceed 1% (v/v). 3-Methyladenine (3-MA, #M9281) from Sigma-Aldrich was dissolved in hot water (70°C) to 30 mg/ml before use. Caspase inhibitor z-VAD-fmk (#sc-3067, 0.5 mg/0.1 ml) was purchased from Santa Cruz Biotechnology, Inc., Santa Cruz, CA, USA).

The cells were dispensed in 96-well, flat-bottom microtiter plates at a density of 2×10³ cells/well and incubated with RAD001 at various dilutions for 20, 44 and 68 h followed by an additional 4 h treatment with WST-1 (Roche, Germany). The cleavage of WST-1 to formazan by metabolically active cells was quantified by scanning the plates in a microtiter plate reader at 440 and 620 nm (reference wavelength). The test medium was used as the background control. Three independent sets of experiments that were performed in triplicate were evaluated. The viability of the treated cells was normalized to the untreated control cells.

Twenty-four hours prior to drug treatment, the cells were seeded directly into 6-well culture plates at a density of 1×10⁵ cells/well. The cells were then treated with various concentrations of RAD001 (0, 20 or 40 μM) for 24 h, stained with DAPI, mounted, and analyzed using an inverted microscope (IX71; Olympus).

The cytotoxicity assay was performed using the Cytotoxicity Detection Kit^PLUS LDH (#04744926001; Roche) according to the manufacturer’s instructions. This assay is based on the measurement of lactate dehydrogenase (LDH) activity released from the cytosol of damaged cell. Three controls are included: background control (assay medium), low control (untreated cells) and high control (maximum LDH release). To determine the experimental absorbance values, the average absorbance values of the triplicate samples and controls were calculated and subtracted from the absorbance values of the background control. The percent cytotoxicity was determined using the following equation: Cytotoxicity (%) = (exp. value − low control)/(high control − low control) × 100.

Cells (1×10⁵ cells/ml) seeded in a 6-well plate were treated with RAD001 for 24 h. For analysis of apoptosis, staining was performed using the Annexin V-FITC/PI Apoptosis Detection kit (#PF032; Merck) according to the manufacturer’s instructions. Both cell cycle distribution and apoptosis were analyzed using flow cytometry (FC500; Beckman Coulter, Brea, CA, USA), and the results were displayed as histograms.

Lysates were prepared from 4×10⁵ cells by dissolving the cell pellets in 100 μl of cell lysis buffer (#9803; Cell Signaling Technology) for 30 min on ice. The lysates were centrifuged at 12,000 × g for 20 min and the supernatant was collected. The protein content was determined using the Pierce BCA Protein Assay (#23225; Thermo Scientific). A total of 30 μg of protein was loaded into each well of an 8–15% SDS-PAGE gel. The resolved proteins were electrophoretically transferred to PVDF membranes and incubated sequentially with primary and secondary antibodies [anti-rabbit IgG, HRP-linked antibody (#7074P2) or anti-mouse IgG, HRP-linked antibody (#7076P2; both from Cell Signaling Technology)]. After washing, the bound antibody complex was detected using LumiGLO reagent (#7003; Cell Signaling Technology) and XAR film (XBT-1; Kodak) as described by the manufacturers. The following primary antibodies were used: caspase-3 antibody (#9662; Cell Signaling Technology); poly(ADP-ribose) polymerase (PARP) antibody (sc-7150; Santa Cruz Biotechnology, Inc.); LC3 antibody (NB100-2220; Novus Biologicals); and glyceraldehyde 3-phosphate dehydrogenase antibody (#32233; Santa Cruz Biotechnology, Inc.).

All experiments were repeated three times. The results of multiple experiments are presented as the mean ± SD. Statistical analyses were performed using the SPSS 17.0 statistical software. The P-values were calculated using a one-way analysis of variance (ANOVA). A P-value of <0.05 was considered to indicate a statistically significant result.

We first examined the viability of the two NPC cell lines in the presence of different concentrations of RAD001 (0–100 μM) using the WST-1 assay. CNE-1 cells were more sensitive, with a 50% growth inhibition (GI₅₀) of 30.0±1.0 μM at 72 h compared to the GI₅₀ of HONE-1, which was 56.9±13.1 μM (Fig. 1A and Table I).

To examine the lethal effect of RAD001 in CNE-1 and HONE-1 cells, both cell lines were treated with different concentrations of RAD001 (0, 20 and 40 μM) for 24 h. Cellular apoptosis was determined using DAPI staining. Chromatin condensation and cell shrinkage were clearly observed after RAD001 treatment (Fig. 1B).

To identify whether mTOR inhibition induces apoptosis, the treated cells were stained with Annexin V-FITC/PI and the apoptotic cell population was analyzed using flow cytometry. RAD001 treatment significantly increased the proportion of apoptotic cells (Fig. 2). In the control group, 3.1±1.1% cells were positive for Annexin V-FITC staining, and the 20, 40 and 80 μM RAD001 treatments resulted in Annexin V-FITC-positive rates of 3.5±0.9, 15.0±4.7 and 27.0±15.3%, respectively, in the CNE-1 cells treated for 24 h. At 48 h post-treatment, the apoptotic rates increased to 3.8±0.8% for the control and to 9.5±6.3, 52.3±11.8 and 96.5±2.2%, respectively, for the above-mentioned treatment groups. Similar results were observed in HONE-1 cells (Fig. 2 and Table II).

To demonstrate whether RAD001 treatment results in increased activation of caspases, we analyzed both the cleavage of PARP-1, a substrate cleaved by caspases during apoptosis, and the activated cleavage of caspase-3. Our western blotting results determined that procaspase-3 was cleaved to yield a 17 kDa fragment and PARP-1 was cleaved to an 89 kDa fragment following treatment in both cell lines (Fig. 3). These results further confirmed that RAD001 induced caspase-3-dependent cell death in these two nasopharyngeal carcinoma cell lines. RAD001-treated NPC cells displayed typical signs of apoptotic cell death including chromatin condensation, cell shrinkage, cleavage of PARP and activation of caspase-3.

mTOR is well known as a major negative regulator of autophagy and acts as a central regulator of the PI3K/Akt pathway, which can induce autophagy when inhibited. The membrane-associated light chain 3 protein (LC3, Atg8) is a key marker of autophagy. After the induction of autophagy, LC3-I is converted to LC3-II, which is most likely conjugated to phosphatidylethanolamine (PE) and tightly bound to the autophagosomal membranes, forming ring-shaped structures in the cytoplasm. The amount of PE-conjugated LC3 (LC3-II) correlates well with the number of autophagosomes. Therefore, we examined LC3-I/II expression using western blotting. RAD001 treatment caused the levels of LC3-II to increase in a dose- and time-dependent manner in both cell lines (Fig. 3).

Since RAD001 induced both apoptosis and autophagy in CNE-1 and HONE-1 cells, we aimed to identify which mechanism of cell death was dominant. We first inhibited autophagy by combining RAD001 with the autophagy inhibitor, 3-MA. 3-MA is used to inhibit and study the mechanism of autophagy (lysosomal self-degradation). It inhibits autophagy by blocking autophagosome formation via the inhibition of type III PI3K. RAD001 of 40 and 80 μM resulted in decreased survival rates of 34.9±2.4 and 19.9±0.9% compared with the control group (100.0%) in the CNE-1 cells (Fig. 4A). Furthermore, there was extensive growth inhibition in the combined treatment group. A survival rate of 17.3±0.5% (P<0.05) and 3.9±0.2% (P<0.05) was noted when 40 and 80 μM RAD001 was combined with 10 mM 3-MA in CNE-1 cells. Similar results were observed in the HONE-1 cells (Fig. 4A).

We next examined whether the combination was effective at inducing cellular apoptosis. As displayed in Fig. 4B, 3.4±1.3% of the cells were positive for Annexin V-FITC staining in the CNE-1 cell control group. Treatment with 40 or 80 μM RAD001 resulted in Annexin V-FITC-positive staining rates of 6.0±0.7 and 15.2±3.6% at 24 h. When 40 or 80 μM RAD001 was combined with 3-MA, the Annexin V-FITC-positive staining rates were 9.0±1.8% (P<0.05) and 34.5±4.7% (P<0.01), respectively. The combination treatment significantly increased the proportion of apoptotic cells compared to this proportion following RAD001 treatment (80 μM) alone (P=0.0024). Regarding the HONE-1 cells, RAD001 of 40 or 80 μM resulted in the Annexin V-FITC-positive staining rates of 4.6±2.0 and 28.6±3.8% compared with the control group (2.7±0.8%) at 24 h. When 40 or 80 μM RAD001 was combined with 10 mM 3-MA, the Annexin V-FITC-positive staining rates were 11.4±3.7% (P<0.05) and 51.5±9.0% (P=0.0076), respectively (Fig. 4B).

We next combined RAD001 with the caspase-3 inhibitor z-VAD-fmk to determine whether inhibition of apoptosis decreases RAD001-induced cell death. Using an LDH assay we determined that the growth inhibition effect was markedly reduced in both CNE-1 and HONE-1 cells. As shown in Fig. 5A, 40 and 80 μM RAD001 resulted in increased cytotoxicity rates of 37.1±4.3 and 51.8±1.7% compared with the control group (0.0%) in CNE-1 cells. When 40 or 80 μM RAD001 was combined with 20 μM z-VAD-fmk, the cytotoxicity rates were decreased to 12.5±5.9% (P<0.01) and 23.8±1.7% (P<0.01), respectively. Similar results were observed in HONE-1 cells (Fig. 5A).

Furthermore, using flow cytometry we examined whether the combination of RAD001 and z-VAD-fmk was effective at reducing cellular apoptosis. As shown in Fig. 5B, 1.2±1.3% of the cells were positive for Annexin V-FITC staining in the CNE-1 cell control group. In regards to the CNE-1 cells, treatment with 40 or 80 μM RAD001 resulted in Annexin V-FITC-positive staining rates of 4.7±3.6 and 61.5±12.5% at 24 h. When 40 or 80 μM RAD001 was combined with 20 μM z-VAD-fmk, the Annexin V-FITC-positive staining rates were reduced to 2.9±2.0% (P>0.05) and 39.1±6.5% (P<0.05), respectively. For HONE-1 cells, RAD001 of 40 or 80 μM resulted in Annexin V-FITC-positive staining rates of 3.2±2.1 and 60.2±9.6% when compared to the rates in the control group (1.7±1.4%) at 24 h. When 40 or 80 μM RAD001 was combined with z-VAD-fmk, the Annexin V-FITC-positive staining rates were reduced to 2.3±0.6% (P>0.05) and 30.7±10.3% (P<0.05), respectively (Fig. 5B).