ECL, with a purity of 93.6%, was purchased from Biopurify Phytochemicals Ltd. Cisplatin was purchased from Merck KGaA. Culture media Roswell Park Memorial Institute (RPMI)-1640, Dulbecco's modified Eagle's medium (DMEM), penicillin/streptomycin antibiotics and trypsin-ethylenediaminetetraacetic acid (trypsin-EDTA) were purchased from Thermo Fisher Scientific, Inc. Fetal bovine serum (FBS) was obtained from GE Healthcare Life Sciences. MTT was obtained from AppliChem GmbH. Muse^® Cell Cycle kit and Muse™ Annexin V & Dead Cell kit were purchased from EMD Millipore. Mammalian Protein Extraction buffer was purchased from GE Healthcare Life Sciences. Antibodies specific to AKT (product no. 9272) and phosphorylated (p)-AKT (S473; product no. 9271), NF-κB p65 (product no. 6956), p-NF-κB-p65 (S536; product no. 3033), caspase-3 (product no. 9662), cleaved caspase-3 (Asp175; product no. 9661), poly (ADP-ribose) polymerase (PARP; product no. 9542) and survivin (product no. 2808) were purchased from Cell Signaling Technology, Inc. Antibodies against Bcl-xL (product code ab32370 and β-actin (cat. no. A2066) were obtained from Abcam and Merck KGaA, respectively. Horseradish peroxidase-conjugated goat anti-rabbit (cat. no. 1706515) or goat anti-mouse (cat. no. 1706516) immunoglobulin G were purchased from Bio-Rad Laboratories, Inc. Cisplatin was dissolved in normal saline (1 mg/ml) and maintained at room temperature. ECL was dissolved in dimethyl sulfoxide (DMSO) and stored at −20°C until use. The final concentration of DMSO was <0.5% (v/v), which was also present in the corresponding controls at the same concentrations.

The human adenocarcinoma NSCLC A549 cell line was obtained from the American Type Culture Collection. The human lung squamous cell carcinoma Calu-1 cell line was purchased from the CLS Cell Lines Service. The A549 and Calu-1 cells were grown and maintained in DMEM and RPMI-1640 media, respectively. These culture media were supplemented with 10% (v/v) FBS, 100 U/ml penicillin and 100 µg/ml streptomycin. All cell lines were incubated at 37°C in a humidified atmosphere containing 5% CO₂. All cell lines were mycoplasma-free. The continuous cell lines were routinely checked every other month by PCR using a service from the Center for Veterinary Diagnosis, Faculty of Veterinary Science, Mahidol University Salaya Campus, Nakorn Pathom (Thailand).

The A549 (3,500 cells/well) and Calu-1 (6,000 cells/well) cells were seeded on a 96-well plate for 24 h and then exposed to 0, 2.5, 5, 10, 20, 40, 80 and 160 µM cisplatin or ECL for 24 and 48 h. The number of viable cells was determined by MTT assay, as previously described (24). The optical density (OD) of the formazan dye was measured at 570 nm using a microplate reader (Bio-Rad Laboratories, Inc.). The percentage of cell viability was calculated using the formula: Cell viability=(OD_treated/OD_control) ×100%. The ECL concentrations required for 20, 40 and 50% inhibition of cell viability (IC₂₀, IC₄₀ and IC₅₀, respectively) in A549 and Calu-1 cells at 24 h were then determined from the viability curves and selected for further experiments.

The antiproliferative effects of ECL on human NSCLC A549 and Calu-1 cell lines were confirmed using a colony formation assay. Briefly, the A549 (2×10⁵ cells/well) or Calu-1 (3×10⁵ cells/well) cells, were seeded on a 6-well plate and incubated for 24 h. The cells were then treated with ECL at an IC₂₀, IC₄₀ and IC₅₀ concentration for 24. Next, the cells were collected by trypsinization with 0.25% trypsin-EDTA (Gibco; Thermo Fisher Scientific, Inc.) and replated in 10-cm culture dishes at a low density of 400 cells/dish to allow colony formation for 2 weeks, with a change of the fresh growth media every 3 days. The colonies were washed with cold phosphate-buffered saline (PBS), fixed with 100% methanol for 10 min, and stained with 0.5% crystal violet for 1 h at room temperature. The colonies containing >50 cells were counted using an inverted microscope at a magnification of ×40.

The A549 (2×10⁵ cells/well) or Calu-1 (3×10⁵ cells/well) cells, were seeded on a 6-well plate and incubated for 24 h. Following ECL treatment at the indicated concentrations and incubation times, cells were collected, fixed gently in 70% ethanol and stored at −20°C overnight. The fixed cells were then stained using a Muse^® Cell Cycle kit for 30 min at room temperature in the dark. The cell cycle phase distributions were determined by Muse^® Cell Analyzer and Muse^® Cell Cycle software module (version 1.0.0.0.; EMD Millipore). The cell cycle phases subG1, G1, S and G2/M were analyzed using GuavaSoft 2.7 software (EMD Millipore).

The IC₂₀ and IC₄₀ of ECL were selected to further study cisplatin co-treatment, to compare the effects of sub-cytotoxic and highly toxic concentrations of ECL on cisplatin sensitization. A549 or Calu-1 cells were treated with 0–160 µM cisplatin either alone or in combination with ECL at the IC₂₀ (2 or 10 µM, respectively) or the IC₄₀ (12 or 80 µM, respectively) for 24 h. Cell viability was then determined by MTT assay, as previously described. The CI, which reflects the nature of drug interactions in combination chemotherapy, was calculated using the Chou-Talalay Method (25) based on the following equation: CI=[(D)₁/(Dx)₁]+[(D)₂/(Dx)₂], where (D)₁ and (D)₂ represent the concentrations of compounds 1 (Cisplatin) or 2 (ECL) in the co-treatment that attains a 50% inhibition, and (Dx)₁ and (Dx)₂ represent the concentrations of compounds 1 or 2 in the co-treatment that attains a 50% inhibition when present alone (26). A CI of <0.9, 0.9–1.1 and >1.1 indicated synergistic, additive and antagonistic effects, respectively.

The A549 (2×10⁵ cells/well) or Calu-1 (3×10⁵ cells/well) cells were seeded on a 6-well plate and incubated for 24 h. The cells were then treated with ECL alone, cisplatin alone or ECL (IC₂₀ or IC₄₀) plus cisplatin for 24 h. Apoptosis was quantified by staining with Muse^® Annexin V & Dead Cell kit (EMD Millipore) for 20 min at room temperature in the dark, according to the manufacturer's instructions. The quantitative analysis of cell living, early and late apoptosis, and cell death, were obtained by the Muse^® Cell Analyzer (EMD Millipore) using the Muse^® Annexin V & Dead Cell software module (version 1.0.0.0) with a minimum of 2,000 events per sample.

Protein expression levels of p^(S473)-AKT, AKT, p^(S536)-NF-κB p65, NF-κB p65, caspase-3, PARP, Bcl-xL and survivin were measured by immunoblotting, as described in our previous study (27). Briefly, cells collected from each treatment group were lysed in a Mammalian Protein Extraction buffer. Protein concentration was determined using the Bradford assay. Protein (30 µg) from each sample was separated by 12% SDS-PAGE and electro-transferred to PVDF membranes. Primary antibodies (1:1,000 dilution) were added and incubated at 4°C overnight; after which the appropriate HRP-conjugated secondary antibody (1:5,000 dilution) was added and incubated for 2 h at room temperature. Chemiluminescence signals were detected on the X-ray film. As an internal control, the β-actin primary antibody was also probed. The normalized mean density of the immunological cross-reactive band was quantified by ImageJ software (version 1.51j8; National Institutes of Health).

Data are expressed as the mean ± standard deviation of at least three independent experiments. Significant differences among groups were analyzed and compared by one-way analysis of variance and Tukey's post hoc test using SPSS 22.0 software (IBM Corp.). P<0.05 was considered to indicate a statistically significant difference.

To determine the effect of ECL on NSCLC cell viability in vitro, human lung cancer A549 (adenocarcinoma) and Calu-1 (squamous cell carcinoma) cells were incubated with various concentrations of ECL (0–160 µM) for 24 or 48 h, and cell viability was then examined by MTT assay. As revealed in Fig. 1B and C, ECL treatment significantly reduced the cell viability of both NSCLC cell lines in a concentration- and time-dependent manner. The ECL concentrations required for a 50% inhibition of cell viability (IC₅₀) of A549 cells at 24 and 48 h (20.81±1.86 and 3.15±0.36 µM, respectively) were markedly lower compared with those required for the same inhibition of cell viability in Calu-1 cells (151.87±4.75 and 12.95±0.85 µM, respectively), indicating that ECL has a higher toxicity in A549 than Calu-1 cells. Table I summarizes the ECL concentrations at IC₂₀, IC₄₀ and IC₅₀ after 24 and 48 h of incubation. The IC₂₀, IC₄₀ and IC₅₀ concentrations of ECL at 24 h (2, 12 and 20 µM for A549 cells, and 10, 80 and 150 µM for Calu-1 cells) were used for subsequent experiments.

Subsequently, the anti-proliferative effect of ECL on the A549 and Calu-1 cells was confirmed by the inhibition of colony formation, as revealed in Fig. 1D and E. The indicated cells were treated with ECL at the IC₂₀, IC₄₀, and IC₅₀ concentrations for 24 h before the cells were replated (300 cells/plate) and allowed to form colonies. The numbers of the colonies formed proportionally reflect the IC₂₀, IC₄₀ and IC₅₀ concentrations of ECL.

To investigate the mechanism through which ECL inhibits cell growth, cell cycle distribution was analyzed by flow cytometry following 24 h of ECL treatment with the IC₂₀, IC₄₀ and IC₅₀ concentrations. As revealed in Fig. 2A and C, ECL caused cell cycle arrest at the G2/M phase in A549 cells. In Calu-1 cells, ECL caused the S phase arrest when treated with IC₂₀, IC₄₀ or IC₅₀ concentrations (Fig. 2B and D) and induced both S and G2/M phase arrest when treated with the IC₂₀ concentration. Such arrest in both NSCLC cells was associated with a concomitant decrease in the percentage of cells at the G1 phase. Moreover, the accumulation of a sub-G1 population, which comprised apoptotic cells containing only fractional DNA content, was observed in a dose-dependent manner in the A549 and Calu-1 cells. These results indicated that ECL could induce NSCLC cell death following the induction of cell cycle arrest.

The effect of ECL on the NSCLC cell apoptosis was confirmed using Annexin V-FITC/7-AAD double-staining, followed by flow cytometry (Fig. 3A and B). Following the 24-h ECL treatment, the apoptotic rates of A549 (Fig. 3C) and Calu-1 (Fig. 3D) cells in the ECL-treated group were significantly increased in a dose-dependent manner, when compared with the control group. Next, the expression of apoptosis regulators, including the pro-apoptotic caspase-3 and PARP proteins, and the anti-apoptotic Bcl-xL and survivin proteins, was determined by immunoblotting in the A549 and Calu-1 cells (Fig. 3E and F, respectively). The expression levels of active caspase-3 and active PARP (cleaved form) were both markedly induced, while that of Bcl-xL and survivin were significantly decreased following treatment with various concentrations of ECL for 24 h, when compared with the control group. These results confirmed that ECL could trigger apoptotic cell death in NSCLC cells.

The inhibitory effect of ECL on the viability of NSCLC cells by triggering apoptotic cell death prompted us to investigate the AKT/NF-κB signaling pathway, which participates in not only multiple steps of lung cancer progression, but also the resistance to chemotherapy (28,29). Phosphorylation at serine 473 (S473) in the C-terminal hydrophobic motif of AKT is involved in AKT activation (30), and phosphorylation at the serine 536 (S536) position of the NF-κB p65 subunit is required for the activation and nuclear translocation of NF-κB (31). ECL significantly inhibited the expression levels of p^(S473)-AKT, total AKT, p^(S536)-NF-κB p65 and total NF-κB p65 in both A549 (Fig. 4A) and Calu-1 (Fig. 4B) cells. In fact, ECL downregulated the expression of p^(S473)-AKT and total AKT in both A549 and Calu-1 cells when normalized to β-actin (Fig. S1). Likewise, the significant depletion of both p^(S536)-NF-κB p65 and total NF-κB p65 levels when normalized to β-actin was observed in the NSCLC cells treated with ECL (Fig. S2). Notably, the ratio of p^(S473)-AKT/AKT and p^(S536)-NF-κB p65/NF-κB p65 were also significantly decreased in the A549 (Fig. 4C) and Calu-1 (Fig. 4D) cells, supporting the involvement of AKT/NF-κB inactivation in ECL-induced apoptosis in the NSCLC cells.

To observe their cisplatin sensitivity, the A549 and Calu-1 cells were treated with cisplatin at various concentrations for 24 h, and cell viability was determined by MTT assay. As revealed in Fig. 5A, the A549 cells displayed a 2-fold greater sensitivity to cisplatin than the Calu-1 cells, when comparing their IC₅₀ values. Next, it was determined whether cisplatin treatment (at IC₂₀) could stimulate AKT/NF-κB signaling in the NSCLC cells using immunoblotting of p^(S473)-AKT, total AKT, p^(S536)-NF-κB p65 and total NF-κB p65. The results in Fig. 5B revealed that the levels of p^(S473)-AKT and p^(S536)-NF-κB p65 were markedly increased in the A549 and Calu-1 cells following cisplatin treatment. The highest levels of p^(S473)-AKT and p^(S536)-NF-κB p65 were detected at 30 min and 24 h, respectively, following cisplatin treatment in both NSCLC cell lines. Therefore, the activation of AKT and NF-κB was responsive to cisplatin treatment in the NSCLC cells.

Next, it was examined whether the combination of ECL and cisplatin exerts a lethal enhancement in NSCLC cells. Following co-treatment with the IC₂₀ or IC₄₀ concentrations of ECL and various concentrations of cisplatin for 24 h, MTT assays were performed. As demonstrated in Fig. 6A and B, the co-treatment significantly reduced the viability of both NSCLC cells when compared with cisplatin alone. Table II summarizes the IC₅₀ values of cisplatin in the co-treatment with ECL (IC₂₀ or IC₄₀); the CI values were calculated to define the drug interaction of cisplatin and ECL, when administered in combination, as synergistic, additive or antagonistic effects. Co-treatment with ECL led to the positive dose (IC₅₀) reduction of cisplatin in both NSCLC cell lines. The CI values of cisplatin combined with ECL at the IC₂₀ and IC₄₀ concentrations in the A549 cells were 0.66±0.06, indicating synergistic effects, and 0.91±0.04, indicating additive effects (Fig. 6C). Moreover, the CI values of cisplatin plus ECL at the IC₂₀ and IC₄₀ concentrations in the Calu-1 cells were 0.60±0.04 and 0.73±0.03, respectively, indicating their synergistic effects (Fig. 6D).

Since the effect of ECL on potentiating cisplatin sensitivity was found in the A549 and Calu-1 cells, the mechanisms of ECL on the enhancement of cisplatin cytotoxicity were further investigated by examining the induction of apoptosis. The flow cytometric results presented in Fig. 7A and B revealed that co-treatment of cisplatin at the IC₂₀ value with ECL at the IC₂₀ or IC₄₀ concentrations significantly induced a higher number of A549 cells to undergo apoptosis compared with either cisplatin or ECL alone. Similar results were obtained in Calu-1 cells (Fig. 7C and D). The effect on apoptosis was confirmed by immunoblotting of pro-apoptotic and anti-apoptotic proteins. As revealed in Fig. 7E and F, caspase-3 cleavage was induced by either ECL or cisplatin as a single agent, whereas the co-treatment resulted in a higher increase of cleaved caspase-3, with a corresponding decrease in the pro-form of caspase-3. By contrast, the co-treatment of cisplatin with ECL markedly decreased the expression of anti-apoptotic Bcl-xL and survivin proteins, when compared with cisplatin alone. These findings demonstrated that the combination of cisplatin and ECL treatment further induced apoptosis in the NSCLC cells more effectively than cisplatin alone.

To understand the cisplatin sensitization mechanisms of ECL, our attention turned to the cisplatin resistance-related AKT/NF-κB signaling pathway, as ECL alone could suppress AKT/NF-κB activation in the NSCLC cells, as demonstrated in the previous results (Fig. 4). The expression of p^(S473)-AKT, total AKT, p^(S536)-NF-κB p65 and total NF-κB p65 was therefore detected by western blotting in the A549 (Fig. 8A) and Calu-1 (Fig. 8B) cells following treatment with ECL or cisplatin alone, or in combination. ECL alone could significantly suppress the ratio of p^(S473)-AKT/AKT (Fig. 8C and D) and p^(S536)-NF-κB p65/NF-κB p65 (Fig. 8E and F) in the A549 and Calu-1 cells, when compared to the non-treatment control. On the other hand, cisplatin alone significantly increased the ratio of p^(S473)-AKT/AKT and p^(S536)-NF-κB p65/NF-κB p65 in both tested NSCLC cells, indicating that cisplatin could induce AKT and NF-κB activation. Notably, the co-treatment of ECL with cisplatin significantly decreased the ratio of p^(S473)-AKT/AKT and p^(S536)-NF-κB p65/NF-κB p65, when compared to cisplatin alone. In combination, ECL sensitized the cisplatin-induced cytotoxicity in NSCLC cells at least partially by inhibiting the activation of the AKT/NF-κB signaling pathway.