Cnidium monnieri (L.) Cusson were purchased from Dong Kyung PHARM Co., Ltd. (Seoul, Korea). The 100 g of CME was soaked in 800 ml of 99.9% ethanol, and then stirring for 48 h at room temperature. The extract was filtered through filter paper (qualitative filter paper no. 1; Toyo Roshi Kaisha, Ltd., Tokyo, Japan) and concentrated with a rotary evaporator to remove the ethanol. The ethanol extracts of Cnidium monnieri (L.) Cusson (CME) was dissolved in dimethyl sulfoxide (DMSO; stock solution, 10–100 mg/ml) and refrigerated at −20°C for long storage. The final concentration of CME in the culture medium was controlled at 10–100 µg/ml. LY294002 (PI3K/Akt inhibitor) was purchased from Calbiochem (EMD Millipore, Billerica, MA, USA) and Pifithrin-α (p53 inhibitor) was purchased from Sigma-Aldrich (St Louis, MO, USA).

The human hepatocellular carcinoma cell lines HepG2 and Hep3B were obtained from the American Type Culture Collection (ATCC, Rockville, MD, USA). The cells were grown in DMEM medium (Hyclone, Laboratories Inc., Logan, UT, USA) containing 10% fetal bovine serum and 1% antibiotics (both Hyclone Laboratories Inc.) at 37°C in a 5% CO₂ atmosphere. The cells were suspended by Trypsin-EDTA (Hyclone, Laboratories Inc.) and separated at 1×10⁶ cells/ml per 100-mm plate, every 48 h.

The cells were seeded at 1×10⁴ cells/ml in 12-well plate and incubated for 24 h. Following incubation, the cells were treated with the CME (10–100 µg/ml) for 24 or 48 h at 37°C in a 5% CO₂ atmosphere. The inhibitor was pre-treated for 30 min before treating CME. The respective medium was removed, and cells were incubated with 20 µl of MTT solution (5 mg/ml) in phosphate-buffered saline (PBS) for 1 h. Converted purple formazan from MTT was solubilized in dimethyl sulfoxide (DMSO). The absorbance of the solution in each well was determined using a microplate reader (model 680, Bio-Rad Laboratories, Inc., Tokyo, Japan) at 595 nm.

The cells were seeded at 1×10⁶ cells/ml in 60-mm plate and incubated for 24 h. Following incubation, the cells were treated with the CME for 24 h at 37°C in a 5% CO₂ atmosphere. The inhibitor was pre-treated for 30 min before treating CME. Total cells were harvested by trypsinization, collected by centrifugation, washed with 3 ml of PBS (twice). The supernatant was removed and discarded. The pellet were resuspended in 1 ml of cold 70% ethanol and freezed at −20°C for at least 3 h. Ethanol-fixed cells were centrifuged at 800 × g for 5 min and washed with 1 ml of PBS. The supernatant was removed, and ethanol-fixed cells were resuspended 500 µl of PBS. The cells were stained with 4 µl of PI (5 mg/ml) and 10 µl of RNase (10 mg/ml) for 20 min at room temperature. Fluorescence intensity was analyzed using a Flow cytometry-FACS Canto (Becton-Dickinson Biosciences, Drive Frankline Lage, NJ, USA).

The cells were seeded at 1×10⁴ cells/ml in 12-well plate and incubated for 24 h after put microscope cover glass (Marlenfeld GmbH & Co., Lauda-Königshofen, Germany) into well. Following incubation, the cells were treated with the CME (20, 40, 60 µg/ml) for 24 h at 37°C in a 5% CO₂ atmosphere. After 24 h, the cells were treated with 0.7 µM Hoechst 33342 and incubated for 30 min. Cells were fixed with 3.5% formaldehyde 500 µl for 20 min and then were gently washed thrice with 150 µl of PBS for 5 min. Placed 10 µl of the mounting solution (50% glycerol) on a slide glass and covered with a cover glass. The chromatin was observed using fluorescence microscope (magnification, ×200; Axioskop 50, Carl Zeiss, Thornwood, NY, USA).

The cells were seeded at 1×10⁵ cells/ml in 6-well plate and incubated for 24 h. Then, the cells were treated with the concentration of CME for 24 h at 37°C in a 5% CO₂ atmosphere. The inhibitor was pre-treated for 30 min before treating CME. The cells were then rinsed twice with ice-cold PBS and scraped with RIPA lysis buffer (50 mM Tris-HCl pH 8.0, 150 mM NaCl, 1% NP-40, 0.5% sodium deoxycholate, 1 mM PMSF) and subjected to western blot analysis. Protein quantification was performed by Bradford assay. 30 µg of protein was loaded per lane. The Nitrocellulose membranes (0.45 µm; cat. no. 10600003; GE Healthcare Life Science, Freiburg, Germany) were blocked with 2% bovine serum albumin (BSA, Bovogen, Melbourne, Australia) in 1X TBST (24.7 mM Tris-HCl, pH 8.0, 137 mM NaCl, 0.05% Tween-20) for 1 h 30 min and incubated overnight at 4°C with primary antibodies targeting mouse monoclonal-p-Akt (Ser473) (1:2,000; cat. no. 4051), rabbit monoclonal-Akt (1:1,000; cat. no. 4685), rabbit monoclonal-GSK-3β (1:1,000; cat. no. 9315), rabbit monoclonal-Bax (1:1,000; cat. no. 5023), rabbit monoclonal-Bak (1:1,000; cat. no. 6947), rabbit monoclonal-caspase-3 (1:1,000; cat. no. 9665), rabbit polyclonal-Bcl-2 (1:2,000; cat. no. 2876), and rabbit polyclonal-β-actin (1:2,000; cat. no. 4967); all purchased from Cell Signaling Technology, Inc. (Beverly, MA, USA) and rabbit polyclonal-p-MDM2 (Ser166) (1:3,000; cat. no. ab131355), rabbit monoclonal-MDM2 (1:3,000; cat. no. ab178938), rabbit monoclonal-p21 (1:3,000; cat. no. ab109520), mouse monoclonal-cyclin E (1:3,000; cat. no. ab3927), rabbit monoclonal-p-cdk2 (Tyr15) (1:3,000; cat. no. ab76146), and rabbit monoclonal-p-cdk2 (Thr14) (1:3,000; cat. no. ab68265); all purchased from Abcam Inc. (Cambridge, MA, USA) and rabbit polyclonal-p-GSK-3β (Ser9) (1:1,000; cat. no. sc-11757-R), and mouse monoclonal-p53 (1:1,000; cat. no. sc-126) were purchased from Santa Cruz Inc. (Santa Cruz, CA, USA). After primary antibody incubation, the membranes were washed 4 times for 5 min each with 1X TBST at room temperature. Following the addition of the secondary antibody; goat polyclonal-anti-mouse antibody conjugated with HRP (1:10,000; cat. no. PA1-30126; Thermo Scientific Rockford, IL, USA) and goat anti-rabbit antibody conjugated with HRP (1:10,000; cat. no. 166-2408; Bio-Rad Laboratories, Inc., Tokyo, Japan), the membrane were reacted for 1 h 30 min at room temperature with gentle agitation. After secondary antibody incubation, the membranes were washed 4 times for 10 min each with 1X TBST at room temperature. Proteins were detected using SuperSignal West Pico Chemiluminescent Substrate (cat. no. PI34080; Thermo Scientific Rockford, IL, USA) and visualized on CP-BU new X-ray film (Agfa HealthCare, Inc., Mortsel, Belgium).

MTT assay were statistically analyzed using an unpaired an independent sample t-test (IBM SPSS Statistics 20.0, SPSS Inc., Chicago, IL, USA). A value of P<0.05 was considered to indicate a statistically significant difference.

To determine the anti-proliferative effect of CME, we performed MTT assay after treatment with various concentrations of CME (10–100 µg/ml) for 24 and 48 h in HepG2 cells. As shown in Fig. 1A, CME inhibited cell proliferation in a dose-dependent manner (IC50 value=88.76 µg/ml in 24 h and 30.93 µg/ml in 48 h). Also, we observed the cell morphology change after treatment with CME for 24 h. As shown in Fig. 1B, cell morphology was changed by CME in a dose-dependent manner. Cell shrinkage and loss of proliferation potential were increased when cells were treated with CME (20–100 µg/ml). Furthermore, we confirmed that the number of cells that were detached from the cell culture plate was increased. These characteristics were observed during the process of apoptosis. These results indicated that CME has anti-proliferative and cell morphology change-inducing effects in HepG2 hepatoma cells.

To identify whether CME-induced effects on cell growth and morphology were caused by apoptosis, we performed Hoechst 33342 staining and western blot analysis. As a result, the apoptotic DNA fragmentation was increased by CME in a dose-dependent manner (Fig. 2A). Also, the expression levels of apoptosis-associated proteins, Bax and Bak, were increased and the levels of procaspase-3 and anti-apoptotic protein Bcl-2 were decreased by CME (Fig. 2B-D).

To confirm whether the reduced cell viability was due to cell cycle arrest, we analyzed the cell cycle after treatment with various concentrations of CME (20–60 µg/ml) for 6 h. As indicated in Fig. 3, the percentage of G1 phase in HepG2 cells was increased to 54.87% (control group), 57.94% (20 µg/ml), 61.17% (40 µg/ml) and 65.41% (60 µg/ml).

We examined the effect of CME on the expression levels of cell cycle-related proteins by CME using western blot analysis. The results showed that the expression levels of p-Akt, p-GSK-3β, p-MDM2 and cyclin E were decreased, while the levels of p53, p21, p-CDK2 (T14) and p-CDK2 (Y15) were increased in a dose-dependent manner (Fig. 4).

CME-induced apoptosis and cell cycle arrest were occurred through regulation of Akt/GSK-3β signaling pathway in a p53-independent manner. To determine the association between CME-induced apoptosis and cell cycle arrest and the Akt/p53 signaling pathway, we used specific inhibitors such as LY294002 (PI3K/Akt inhibitor) and pifithrin-α (p53 inhibitor). We co-treated the cells with LY294002 or pifithrin-α and CME and performed the MTT assay. As shown in Fig. 5A, cell viabilities in the CME-treated group and the LY294002-treated group were decreased compared to that in the control group. Also, the cell viability in the CME/LY294002 co-treated group was decreased more than that in the CME-treated group. Furthermore, cell viabilities in the CME/pifithrin-α co-treated group and the CME-treated group did not differ. To confirm whether CME-induced anti-proliferative and apoptotic effects occur in a p53-independent manner, we performed the MTT assay, Hoechst 33342 staining and western blot analysis in Hep3B (p53-null) cells. As a result, CME suppressed Hep3B cell proliferation (Fig. 5B) (IC50 value=64.46 µg/ml in 24 h and 46.32 µg/ml in 48 h), and induced apoptotic DNA fragmentation in a dose-dependent manner (Fig. 5C). Also, the expression levels of apoptosis-associated proteins were regulated by CME in Hep3B cells (Fig. 5D). In the cell cycle analysis, treatment with CME or LY294002 induced cell cycle arrest at G1 phase and co-treatment with CME/LY294002 and CME/pifithrin-α also induced G1 arrest in HepG2 cells (Fig. 5E). Moreover, the percentage of G1 phase was increased by CME in Hep3B cells (Fig. 5F). These results supported the claim that CME induces apoptosis and G1 cell cycle arrest in a p53-independent manner.

To investigate whether the CME-induced cell cycle arrest occurred through p53-independent pathway, we performed western blot analysis after treatment with LY294002 (PI3K/Akt inhibitor) and pifithrin-α (p53 inhibitor). As a result, the expression levels of p-Akt, p-GSK-3β, p-MDM2 and cyclin E were decreased in the CME-treated group compared to the control group and the expression levels in the CME/LY294002 co-treated group were also decreased (Fig. 6A). Especially, when we co-treated cells with CME and pifithrin-α, the expression levels of p-Akt, p-GSK-3β, p-MDM2 and cyclin E were decreased and the expression levels of p53, p21, p-CDK (T14) and p-CDK (Y15) were increased by CME although pifithrin-α-treatment was performed. Additionally, the expression levels of cell cycle-related proteins were regulated by CME in Hep3B (p53-null) cells (Fig. 6B).