Professor Li from the South China Normal University (Guangzhou, China) developed a novel column chromatography extraction method for the extraction of cordycepin from solid rice-based fermentation medium. Using this method, cordycepin is obtained at a 98% purity, with an overall recovery rate of 90% (25). Cordycepin was provided by his laboratory and was freshly prepared as stock solution in double-distilled water. It was diluted in culture medium at concentrations of 125, 250, 500, 1,000 and 2,000 μg/ml prior to experiments. Dulbecco’s modified Eagle’s medium (DMEM) and 4′, 6-Diamidino-2-phenylindole (DAPI) were purchased from Invitrogen Corporation (Carlsbad, CA, USA). Fetal bovine serum (FBS) was purchased from Gibco Industries Inc. (Big Cabin, OK, USA) and the cell apoptosis propidium iodide (PI) detection kit was purchased from Nanjing KeyGen Biotechnology Co., Ltd. (Nanjing, China). 3-(4,5-Dimethylthiazol-2-yl)-2,5-diphenyltetrazoliumbromide (MTT) and dimethyl sulfoxide (DMSO) were purchased from Sigma-Aldrich (St. Louis, MO, USA). MTT was dissolved in phosphate-buffered saline (PBS; Gibco, Carlsbad, CA, USA) and stored in the dark. Transwell chamber and Matrigel were purchased from BD Biosciences (San Jose, CA, USA). All reagents were of analytical grade, unless otherwise specified.

Human HCC cells (HepG2) and human endothelial-like immortalized cells (EA.hy926) were obtained from the Cell Bank of Type Culture Collection of Chinese Academy of Sciences (Shanghai, China). EA.hy926 and HepG2 cells were cultured in DMEM supplemented with 10% (v/v) heat-inactivated fetal calf serum, penicillin (100 U/ml) and streptomycin (100 U/ml) (both Sigma-Aldrich). Cultures were maintained at 37°C in a humidified atmosphere containing 5% CO₂ and 95% air. The medium was changed every two days.

Cell survival changes in response to cordycepin were evaluated by MTT assay (8,26). Briefly, 2×10⁴ cells in 100 μl DMEM supplemented with 2% (v/v) heat-inactivated FBS, penicillin (100 U/ml) and streptomycin (100 U/ml) were seeded into 96-well plates. Medium without cells was used as a blank control. Confluent cells were treated with various concentrations of cordycepin (125, 250, 500, 1,000 and 2,000 μg/ml) for 1, 2, 3, 4 and 5 days. The same volume of double-distilled water was used as the negative control (0 μg/ml). At the designed time points, 100 ml MTT solution in PBS was added to obtain a final concentration of 0.5 g/ml, and the incubation was continued at 37°C for 4 h. Finally, the medium was removed and replaced with 200 μl DMSO. The mixture was quantified by determining its absorbance at 540 nm using a SpectraFluor Plus Reader (Tecan AG, Hombrechtikon, Switzerland). The relative growth rate was calculated as optical density (OD)_{test group}/OD_{negative control}.

Assessment of apoptotic cells was performed according to published methods (27,28). EA.hy926 cells were exposed to various concentrations of cordycepin (0, 250, 500, 1,000 and 2,000 μg/ml). They were treated with trypsin-EDTA (Sigma-Aldrich) and collected by centrifugation at 150 × g for 10 min, then thoroughly rinsed with PBS. Pellets were resuspended in ice-cold 70% ethanol and fixed at −20°C for 24 h. Cells were then centrifuged (1,000 rpm for 15 min) and ethanol was removed by washing thoroughly with PBS. Cell pellets were resuspended in 1 ml DNA-staining reagent containing 50 μg/ml RNase, 0.1% Triton X-100, 0.1 mmol EDTA (pH 7.4) and 50 μg/ml PI which was provided with the cell apoptosis PI detection kit. Samples were stored in the dark at 4°C for 30 min. Red fluorescence (DNA) was detected through a 563–607 nm band-pass filter using a FC 500 MCL/MPL flow cytometer (Beckman Coulter, Brea, CA, USA). In flow cytometry histograms, apoptotic cells have a signal in the sub-diploid regions, which are well-separated from the normal G1 peak. A total of 10⁵ cells in each sample were analyzed and the percentage of apoptotic cell accumulation in the sub-G1 peak was calculated.

A Transwell chamber containing an 8-μm pore polycarbonate membrane filter was coated either with Matrigel (for invasion) or without Matrigel (for migration) and inserted in a 24-well culture plate. HepG2 cells were pre-treated with 0, 125, 250, 500 and 1,000 μg/ml cordycepin for 24 h. The cells were then detached with trypsin-EDTA and resuspended in serum-free DMEM. After filling the lower chamber with media supplemented with 10% FBS as a chemoattractant, 10⁵ cells/well in 0.2 ml serum-free DMEM were loaded in the upper chambers. The apparatus was incubated at 37°C in a humidified chamber with 5% CO₂ for 12 h (migration assay) or 24 h (invasion assay). Following incubation, the filter was removed. Cells in the upper chamber that did not migrate were scraped away with a cotton swab. The transmembrane cells were fixed in methanol for 30 min, washed twice with PBS and stained with 300 nM DAPI for 5 min. Migrating or invading cells were photographed using an inverted microscope (Axio Observer Z1; Carl Zeiss AG, Oberkochen, Germany) and were counted in five randomly selected fields per membrane, then the averages were calculated. Presented data are representative of three individual wells.

EA.hy926 cells were cultured as confluent monolayers, synchronized in 1% FBS for 24 h and wounded by removing a 300- to 500 μm-wide strip of cells across the well with a standard 200 μl pipette tip. Wounded monolayers were washed twice with PBS to remove non-adherent cells and then treated with 0, 125, 500 and 2,000 μg/ml cordycepin for 6 h. EA.hy926 cell migration was recorded under inverted microscope (Axio Observer Z1; Carl Zeiss AG). Wound healing was quantified, using Image J software (National Institutes of Health, Bethesda, MD, USA), as follows: Wound healing area (%) = [cell-free area (0 h) - cell-free area (6 h)] / cell-free area (0 h) ×100 (29).

To investigate the effect of cordycepin on angiogenic activity of EA.hy926 cells in vitro, a tube formation assay was performed following the procedure by Oikawa et al (30). Twenty-four-well cluster tissue culture dishes were coated with 500 μg/ml Matrigel and incubated for 30 min at 37°C. EA.hy926 cells were pre-treated with 0, 125, 250, 500 and 1,000 μg/ml cordycepin for 12 h and were then seeded onto solidified gels at a density of 10⁵ cells/well in 1 ml culture medium. After 24 h of incubation, the total lengths of tube-like structures in five randomly selected microscopic fields per well were determined by phase-contrast microscopy and quantified using Image J software.

Intracellular cordycepin levels were measured according to a previously published method (31). EA.hy926 cells were seeded into six-well plates at a density of 1.5–2×10⁶ cells/well. After reaching confluence, cells were pretreated with 125 μg/ml cordycepin for 0.5–3 h. In order to investigate intracellular cordycepin levels, the culture medium was removed, the cells were rinsed three times with PBS and were submitted to two freeze-and-thaw cycles, then homogenized on ice. The cell homogenate was centrifuged at 12,000 × g for 15 min at 4°C. The supernatant was stored on ice and was filtered through a 0.22-μm filter. The supernatant was finally assayed by HPLC (Dalian Elite Analytical Instruments Co., Ltd., Dalian, China) with dual P230 pumps, an UV230+ detector and analytical software. Samples were processed on an YMC-packed C18 column (5 μm, 250×4.6 mm). The mobile phase consisted of methanol:water (20:80 v/v), with a flow rate of 1.0 ml/min. The UV detector was set at 260 nm and the amount of injected sample was 10 μl. Quantitative analysis of cordycepin was determined by its peak area based on a standard curve built using 100 μg cordycepin. Cordycepin peaks in the samples were identified by the retention time and co-injection tests with the corresponding standard compound. The peak for cordycepin was shown at a retention time of 8.96 min.

All investigations were conducted with at least three independent experiments, each performed in triplicates. Data are expressed as the mean ± standard deviation and were evaluated for statistical significance using one-way analysis of variance followed by Duncan’s multiple range tests. GraphPad Prism 5.0 (GraphPad Software Inc., San Diego, CA, USA) was used to perform statistical analysis. P<0.05 was considered to indicate a statistically significant difference.

To investigate whether cordycepin affects cell proliferation in HCC cells, we performed MTT assays in EA.hy926 and HepG2 cells. As shown in Fig. 1A and B, the relative growth rates were markedly decreased in the presence of high doses of cordycepin exceeding 500 μg/ml, indicating that cordycepin inhibited EA.hy926 and HepG2 cell proliferation in a dose- and time-dependent manner.

To assess whether cordycepin affects apoptosis of endothelial cells, we incubated EA.hy926 cells with 0, 250, 500, 1,000 and 2,000 μg/ml cordycepin for 24 h and performed a flow cytometry assay. As shown in Fig. 2A and B, 250 μg/ml cordycepin had no detectable effect on cell apoptosis, while 500, 1,000 and particularly 2,000 μg/ml cordycepin caused a marked increase in the percentage of apoptotic cells, compared with the negative control (0 μg/ml) (all P<0.05).

In HCC development and metastatic spread, cell migration and invasion are essential processes. To detect antitumor activities of cordycepin on HepG2 cells, Transwell migration and invasion assays either without or with precoated Matrigel were performed following treatment with cordycepin at doses of 0, 125, 250, 500 and 1,000 μg/ml. HepG2 migration was significantly suppressed by cordycepin in a dose-dependent manner (all P<0.05; Fig. 3A and B). The numbers of migrating cells following treatment with cordycepin at doses of 0, 125, 250, 500 and 1,000 μg/ml were 97±5, 80±3, 79±2, 62±3 and 58±3, respectively.

Similarly, HepG2 cell invasion was markedly inhibited in a dose-dependent manner (all P<0.05; Fig. 3C and D). The numbers of invading cells following incubation with 0, 125, 250, 500 and 1,000 μg/ml cordycepin were 51±4, 25±3, 23±3, 9±1 and 7±1, respectively. These results demonstrate that cordycepin significantly reduced the potential of HepG2 cells to migrate and invade.

To explore whether cordycepin affects the angiogenic potential of HCC cells, we examined cell migration and angiogenesis by wound healing and tube formation assays in EA.hy926 cells. The wound healing assay demonstrated that the migration of EA.hy926 cells incubated with cordycepin was significantly decreased compared with the negative control (0 μg/ml) (all P<0.05). After treatment with various concentrations of cordycepin for 24 h, the percentage of wound healing area was 85.48±0.84% in the negative control cells, 63.50±1.08% in 125 μg/ml-treated cells, 40.81±1.76 in 500 μg/ml-treated cells and 3.45±0.29% in 2,000 μg/ml-treated cells (Fig. 4A and B).

As shown in Fig. 5A, EA.hy926 cells in the negative control aligned to form tube-like structures and crossing tubes with multicentric junctions. EA.hy926 cells treated with various concentrations of cordycepin tended to form fewer tubes, as well as fewer and weaker junctions. The total lengths of tubular structure after incubation with 0, 125, 250, 500 and 1,000 μg/ml cordycepin for 24 h were 936±56, 536±126, 395±31, 292±88 and 107±39 μm (Fig. 5B). The results revealed that cordycepin significantly inhibited migration and angiogenesis of endothelial cells.

Based on the standard curve of cordycepin, the stability of intracellular cordycepin is shown in Fig. 6A. EA.hy926 cells were incubated with the culture medium (DMEM plus 10% FBS) containing 125 μg/ml cordycepin from 0.5 to 3 h (Fig. 6B–D). The cytosol of EA.hy926 cells without cordycepin is shown in Fig. 6E. The cellular content was assayed by HPLC. Under the chromatographic conditions used, cordycepin had a retention time of 8.96 min. The results demonstrated that cordycepin was able to permeate the cell membrane of EA.hy926 cells and was stable during the 3 h of incubation.