To evaluate the volatile compounds present in P. quercetorum, DTD followed by analysis with comprehensive two-dimensional gas chromatography-time-of-flight/mass spectrometry (GCxGC-TOF/MS) was performed. The plant was directly loaded into the system. A GCxGC-TOF/MS system was used together with a dual stage commercial thermal desorption injector, which incorporated a thermal desorption unit (TDU) connected to a programmable-temperature vaporization injector [Cooled Injection System (CIS)-4 Plus; Gerstel, Mülheim an der Ruhr, Germany], using a heated transfer line. The injector was equipped with a MultiPurpose Sample (Gerstel). Empty glass thermodesorption tubes were conditioned at 400°C for 2 h prior to each use. Approximately 20–30 mg sample was placed into the thermodesorption tubes using tweezers to ensure no contamination of the sample. The initial desorption of the sample was conducted by heating the TDU from 40°C (initial time, 0.2 min) to 150°C at a rate of 120°C/min with a final hold time of 10 min under a helium flow of 1.5 ml/min in splitless mode. Volatile analytes released from this heating were cryo-focused at −40°C in the CIS, which was cooled with liquid nitrogen prior to injection. The CIS was then heated at a rate of 10°C/sec to a final temperature of 150°C. Analytes were transferred splitless to the GC column during the CIS temperature ramp.

The GCxGC-TOF/MS system consisted of a 6890 GC (Agilent Technologies, Inc., Santa Clara, CA, USA) and a Pegasus III TOF-MS system (LECO Corporation, Saint Joseph, MI, USA). The modulator between the first and second GC columns was based on a LECO liquid nitrogen two-stage cold jet system. Helium was used as a carrier gas at a constant flow of 1.0 ml/min. The first column was a non-polar BPX5 (30 mx0.32 mm i.d. ×0.25 µm film thickness), while the second column was a BPX50 (1.5 mx0.10 mm i.d. ×0.10 µm film thickness), both from SGE Analytical Science (Victoria, Australia). The combination of separations produced the overall two-dimensional chromatogram. Peak identification was performed using TOF/MS with electron ionization.

Non-small cell lung cancer cell lines A549, H1299 (Dr Donner, Walther Oncology Center, Indiana University School of Medicine, Indianapolis, IN, USA) and PC3 (Dr Yokota, National Cancer Center Research Institute, Division of Genome Biology, Tokyo, Japan) were cultured in RPMI-1640 (Lonza Bioscience, Verviers, Belgium) medium supplemented with L-glutamine (Gibco^®; Thermo Fisher Scientific, Inc., Waltham, MA, USA), 10% fetal bovine serum (Lonza Bioscience), penicillin G (100 U/ml) and streptomycin (100 µg/ml) (HyClone; GE Healthcare Life Sciences, Logan, UT, USA) at 37°C in a humidified atmosphere containing 5% CO₂. According to the American Type Culture Collection (Manassas, VA, USA), PC3 is often known as a prostate cancer cell line (CRL1435), but in the present study, it represents a non-small cell lung cancer cell line derived from the Japanese Collection Research Resources Bank (Osaka, Japan; JCRB, JCRB0077).

The lyophilized P. quercetorum extract (PQE) was dissolved in dimethyl sulfoxide (DMSO; Sigma-Aldrich, St. Louis, MO, USA) at a concentration of 100 mg/ml as a stock solution, aliquoted and stored at −80°C. PQE was used at different concentrations ranging from 3.13 to 100 µg/ml, and the dilutions were made in culture medium.

The ATP assay, a highly sensitive luciferin:luciferase-based assay, was performed to determine the level of cellular ATP as an indirect marker of the number of alive cells present in the sample (30). A549, PC3 and H1299 cells were seeded at a density of 1×104 cells/well in a 96-well plate in 200 µl medium. Cells were incubated either alone (as control) or in the presence of PQE for 48 h. The untreated/control cells received vehicle only (0.1% DMSO) without any drugs (which represented the maximum viability). Each experiment was conducted at least twice in triplicates. At the end of the treatment period (48 h), cell viability was determined by ATP assay with an ATP bioluminescent somatic cell assay kit (Sigma-Aldrich), according to the manufacturer's protocol with a slight modification, as explained previously (31). Morphological changes of cells were also observed under a phase-contrast microscope (CKX41; Olympus Corporation Tokyo, Japan).

The translocation of phosphatidylserine (PS) molecules from the inner to the outer side of the cell membrane is one of the earlier events of apoptosis (32). Annexin-V-FITC is able to bind to PS, thus allowing the apoptotic cells to become visible. Propidium iodide (PI) is normally used as a second dye to distinguish between early and late apoptosis as well as necrosis (33). In addition, a nucleus-staining fluorescent dye, Hoechst 33342 (200 µg/ml, 1:40; AppliChem GmbH, Darmstadt, Germany) was used in the present study to detect apoptosis on the basis of nuclear morphology. Hoechst 33342 dye stains all types of cells (alive and dead) (34). While early apoptotic cells are considered only Annexin-V-FITC-positive, late apoptotic cells (or secondary necrotic cells) are considered both Annexin-V-FITC- and PI-positive, with the presence of pyknotic nuclei and/or condensed chromatin (33,34). Briefly, A549, PC3 and H1299 cells were seeded in a 96-well plate at a density of 1×104 cells/well, and treated for 12 and 24 h with PQE at a dose of 100 µg/ml. Upon treatment, cells were stained with Annexin-V-FITC and PI using the Annexin-V-FLUOS Staining kit (Roche Diagnostics GmbH, Mannheim, Germany), according to the manufacturer's protocol. The cells were then visualized under a fluorescence microscope.

Intact cytokeratin 18 (CK18, also known as M65) and caspase-cleaved CK18 (also known as M30) were measured using M30-Apoptosense^® and M65 EpiDeath^® enzyme-linked immunosorbent assay (ELISA) kits (Vivalavida AB, Nacka, Sweden). The M30-Apoptosense^® ELISA kit measures the levels of M30 produced during apoptosis, while the M65 EpiDeath^® ELISA kit measures the levels of both caspase-cleaved and intact CK18, which is released from cells undergoing necrosis (35). A total of 1×10⁴ A549, PC3 or H1299 cells were seeded per well in a 96-well plate in 200 µl culture medium in triplicates. After 24 h, cells were treated with PQE (100 µg/ml) for 48 h. At the end of the treatment period, cells were lysed with 10% NP-40 (Sigma-Aldrich) for 10 min on a shaker to perform the M30 assay, while the supernatants were collected for the M65 assay, according to the manufacturer's protocol. The absorbance was determined with an ELISA reader at 450 nm (FLASH Scan S12^®; Analytik Jena AG, Jena, Germany).

A549, PC3 and H1299 cells were seeded in 25-cm² flasks, and treated with PQE (100 µg/ml) for 24 h when the cells reached 70% confluency. Additionally, cisplatin (20 µM) for A549 and PC3 cells, and etoposide (5 µM) for H1299 cells, were used as positive controls for cleaved-poly (adenosine diphosphate-ribose) polymerase (PARP) (36–38). Cells were lysed in radioimmunoprecipitation assay lysis buffer (Santa Cruz Biotechnology, Inc., Dallas, TX, USA), containing protease inhibitors. Equal amounts of protein (20 µg protein/lane) were subjected to 12% sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and then transferred to a nitrocellulose membrane (Thermo Fisher Scientific, Inc.). Western blotting was performed using rabbit anti-β-actin and anti-PARP monoclonal antibodies at 1:1,000 dilution (catalog nos., 4970 and 9532, respectively; Cell Signaling Technology, Inc., Danvers, MA, USA) in 5% (w/v) bovine serum albumin (Amresco, LLC, Solon, OH, USA). Horseradish peroxidase (HRP)-linked anti-rabbit immunoglobulin G antibody (1:2,000 dilution; catalog no., 7074; Cell Signaling Technology, Inc.) was used to detect anti-β-actin and anti-PARP antibodies. Secondary antibody detection was performed according to the instructions of Phototope^®-HRP Western Blot Detection System (Cell Signaling Technology, Inc.). Stripping was performed according to the manufacturer's reprobing protocol (Cell Signaling Technology, Inc.). Bound antibodies were visualized on a FUSION-FX7 imaging device (Vilber Lourmat, Marne-la-Vallée, France).

All statistical analysis were performed using SPSS 20.0 statistical software (IBM SPSS, Armonk, NY, USA). The significance was calculated using one-way analysis of variance. Significant differences in the M30 and M65 assays were determined using the Student's t test. P<0.05 was considered to indicate a statistically significant difference. The results were expressed as the mean ± standard deviation.