Epimedium koreanum Nakai (EYK) was as described in our previous studies (7). Briefly, the dried bark of the plant was obtained from a domestic Korean market (Kyung Dong Crude Drugs Market, Seoul, Korea) and boiled in distilled water for 2.5 h at 105°C; the resultant suspension was filtered and lyophilized. The powder was stored at 4°C and the extract was dissolved in phosphate-buffered saline (PBS) and diluted with medium before each experiment.

A172, U373MG and T98G cells (human brain cancer cells; Korean Cell Line Bank, Seoul, Korea) were maintained in RPMI-1640 medium (HyClone Laboratories, Logan, UT, USA) supplemented with 10% fetal bovine serum (FBS; HyClone Laboratories) in a 5% CO₂ incubator.

We used the following primary antibodies: mouse β-actin (Santa Cruz Biotechnology, Dallas, TX, USA), mouse anti-p-IκBα (B-9, Ser32; Santa Cruz Biotechnology), rabbit anti-IκBα (Santa Cruz Biotechnology), rabbit anti-NF-κB (P65; Santa Cruz Biotechnology), PCNA (Abcam, Cambridge, MA, USA), rabbit anti-ERK (Cell Signaling Technology, Danvers, MA, USA), rabbit anti-p-ERK (Thr202/Tyr204; Cell Signaling Technology) and rabbit anti-p-NF-κB (Ser536; Cell Signaling Technology). The following secondary antibodies and dilutions were used: horseradish peroxidase (HRP)-conjugated anti-mouse and rabbit IgG (Bethyl Laboratories, Montgomery, TX, USA). Phorbol 12-myristate 13-acetate (PMA), MMP-9 inhibitor (CAS1177749-58-4) and NF-κB inhibitor (BAY 11-7085) were purchased from Sigma-Aldrich (St. Louis, MO, USA).

Western blot analysis was performed as previously described (14). Briefly, A172, U373MG and T98G cells were harvested in ice-cold lysis buffer (50 mM Tris-Cl, 150 mM NaCl, 1% NP-40) containing protease and phosphatase inhibitor (Roche Diagnostics, Indianapolis, IN, USA). Proteins from cell extracts were separated under denatured and reduced conditions using Tris-glycine polyacrylamide gel electrophoresis. Separated proteins were transferred onto polyvinylidene difluoride membrane (PVDF; EMD Millipore, Temecula, CA, USA) at 110 V for 1 h and blocked with 5% skim milk or 5% bovine serum albumin (BSA) in 0.1% TBS-T (Tris-buffered saline with 0.1% Tween-20) for 1 h at room temperature. The blots were incubated overnight at 4°C with specific primary antibodies: mouse β-actin (1:5,000; Santa Cruz Biotechnology), mouse anti-p-IκBα (Ser32, 1:500; Santa Cruz Biotechnology), rabbit anti-IκBα (1:1,000; Santa Cruz Biotechnology), rabbit anti-NF-κB (P65, 1:1,000; Santa Cruz Biotechnology), rabbit anti-ERK (Cell Signaling Technology), rabbit anti-p-ERK (Thr202/Tyr204; Cell Signaling Technology), and PCNA (1:1,000; Abcam). HRP-conjugated secondary antibody was visualized by enhanced chemiluminescence detection reagents (ECL; ATTO Corp., Tokyo, Japan) and image were captured using chemiluminescence imaging system (Vilber Lourmat Deutschland GmbH, Eberhardzell, Germany). Equal amount of protein (10 mg) were used for immunoblotting and all blot images were analyzed using either Fusion software or ImageJ.

To measure cell viability, A172, U373MG and T98G cells were seeded in 96-well plates and treated for 24 h with vehicle or EYK at various concentrations (1, 10, 100, 200, or 400 µg/ml) in the absence of serum. After 24 h, cells were treated with 0.5 mg/ml MTT and incubated for 3 h at 37°C in a 5% CO₂ incubator. Plates were read by measuring absorbance at 580 nm.

A172, U373MG and T98G cells were 80% confluence, and then the monolayer of cells was scratched using a fine pipette tip and immediately imaged (0 h). The cells were pre-treated with vehicle or PMA (75 nM) for 45 min, and then treated with vehicle or EYK (200 µg/ml) for 24 h. Images of the wound gap were acquired immediately (0 h) and 24 h after (24 h) scratching and gap width was measured using ImageJ.

Corning Matrigel^® was loaded onto the membrane of a culture insert (Corning Transwell System; Corning Inc., Corning, NY, USA) and incubated at 37°C for 30 min in a 5% CO₂ incubator. A172 cells (1×10⁵/ml) were plated onto the Matrigel-coated insert in the upper chamber, which contained serum-free RPMI-1640, and then treated with vehicle, EYK (200 µg/ml) or PMA (75 nM). RPMI-1640 media containing 10% FBS was added to the lower chamber. After 24 h, the cells were fixed in methanol (100%) and stained with hematoxylin-eosin (Sigma-Aldrich). The membrane was cut and mounted on a glass microscope slide. Images were randomly acquired (two or three images from each sample) on aninverted microscope (Carl Zeiss, Oberkochen, Germany).

To measure MMP activity, A172 cells were pre-treated with vehicle or PMA (75 nM) for 45 min, and then treated for 24 h with vehicle or EYK (200 µg/ml). After 24 h, the conditioned medium was collected and analyzed on a 10% acrylamide gel containing 0.1% (w/v) gelatin. Following electrophoresis, the gel was washed three times for 10 min each with 2.5% Triton X-100, and then incubated overnight in zymography incubation buffer (2.5 mM CaCl₂, 200 mM NaCl, 50 mM Tris-HCl, pH 7.5). The next day, the gel was stained with 0.2% Coomassie brilliant blue solution R-250 for 1 h, and then washed three times for 10 min each in destaining buffer (10% MeOH, 10% acetic acid in distilled water). Gel images were acquired on a light box (Vilber Lourmat, Seoul, Korea) and analyzed using Image Gauge V4.0 (Fujifilm, Tokyo, Japan).

A172 cells were lysed on ice for 5 min in buffer A [10 mM HEPES (pH 8.0), 1.5 mM MgCl2, 10 mM KCl, 0.5 mM DTT, 300 mM sucrose, 0.1% NP-40 and 0.5 mM PMSF]. After 5 min, the cell lysates were centrifuged at 10,000 rpm at 4°C for 1 min, and the supernatant was collected as the cytosolic fraction. Then, the cell pellet was lysed on ice for 15 min in buffer B [20 mM HEPES (pH 8.0), 20% glycerol, 100 mM KCl, 100 mM NaCl, 0.2 mM EDTA, 0.5 mM DTT and 0.5 mM PMSF] and the cell lysates were centrifuged at 15,000 rpm at 4°C for 20 min. The supernatant was collected as the nuclear fraction.

To examine the effects of EYK on MMP-9 and TIMP-1 mRNA levels, A172 cells were pre-treated with vehicle or PMA (75 nM) for 45 min, and then treated for 24 h with vehicle or EYK (200 µg/ml). After 24 h, RNA was extracted using TRIzol (Ambion, Inc., Austin, TX, USA). RT-PCR was performed using the following primers: MMP-9: 5-CGG AGC ACG GAG ACG GGT AT and 3-TGA AGG GGA AGA CGC ACA GC; TIMP-1: 5-AGC GCC CAG AGA GAC ACC and 3-CCA CTC CGG GCA GGA TT; GAPDH: 5-GTT ACC AGG GCT GCC TTC TC and 3-GTG ATG GCA TGG ACT GTG GT. Image analyses were performed using the Fusion or ImageJ software to measure average band intensities.

A172 and U373MG cells were fixed for 8 min using ice cold 100% methanol, washed with 1X PBS, and then incubated with the following primary antibodies overnight: rabbit anti-p-NF-κB (Ser536, 1:100; Cell Signaling Technology), mouse anti-β-actin (1:200; Santa Cruz Biotechnology) in GDB buffer (0.1% gelatin, 0.3% Triton X-100, 16 mM sodium phosphate pH 7.4 and 450 mM NaCl) overnight at 4°C. The next day, cells were washed with 1X PBS three times and incubated with the following secondary antibodies in GDB solution for 1 h at room temperature: anti-rabbit-AlexaFluor 488 and anti-mouse-AlexaFluor 555 (1:200; Molecular Probes, Eugene, OR, USA) and cell covered using DAPI containing mount solution (Vector Laboratories, Burlingame, CA, USA). Images were taken on a single plane using a confocal microscope (Nikon) and analyzed using ImageJ software.

All data were analyzed by either two-tailed t-test or ANOVA using the GraphPad Prism 4 software. Post hoc analyses were completed with the Tukeys multiple comparison test with P<0.05 considered to represent significance (P<0.05, P<0.01, P<0.001).

To test the effects of EYK on cell viability in malignant human tumor cells, we treated U373MG, T98G and A172 cells with vehicle or EYK (1, 10, 100, 200 or 400 µg/ml) for 24 h and then conducted MTT assays. In U373MG cells, EYK did not influence cell viability at any doses (Fig. 1A). In T98G cells, EYK slightly decreased cell viability at the highest doses, by 13 and 23% at 200 and 400 µg/ml, respectively (Fig. 1B, P<0.01; two-tailed t-test). In A172 cells, EYK caused no toxicity up to a concentration of 200 µg/ml, but had some toxicity at 400 µg/ml (Fig. 1C, P<0.01; two-tailed t-test). Based on these findings, we selected a working concentration of 200 µg/ml for the following experiments.

To determine whether EYK can regulate PMA-induced brain tumor cell migration, we initially optimized the dose and timing for treatment with PMA, a cancer inducer (15), in our culture system. For these experiments, U373MG, T98G and A172 cells were grown in a monolayer, scratched with a pipette tip, and treated with vehicle or PMA (25, 50, 75, 100 or 125 nM) for 24 h. At 0 h (i.e., immediately after scratching) and 24 h, we acquired images of the wound gap at both time-points and measured the proportion of cells migrated from 0 h to 24 h at different PMA concentrations. Subtracting the surface area at 0–24 h with vehicle treatment were listed as 100%, and difference between the areas at 0–24 h at various PMA concentrations were compared with vehicle treatment. PMA dramatically increased cell migration relative to the vehicle at all doses tested in U373MG (Fig. 2A and D, P<0.01; P<0.001; ANOVA with post hoc Tukeys test), T98G (Fig. 2B and E, P<0.001, ANOVA with post hoc Tukeys test), and A172 cells (Fig. 2C and F, P<0.01, P<0.001, ANOVA with post hoc Tukeys test), with an optimal concentration at 75 nM in all three cell lines.

To determine the optimal time for PMA treatment, we treated U373MG, T98G and A172 cells with vehicle or PMA at various times (15, 30, 45 and 60 min) and performed western blotting to detect anti-p-ERK and total ERK, an important signaling for cancer migration (16). PMA significantly increased p-ERK at all time-points in U373MG (Fig. 2G and H, P<0.01, P<0.001, ANOVA with post hoc Tukeys test), T98G (Fig. 2I and J, P<0.05, ANOVA with post hoc Tukeys test), and A172 cells (Fig. 2K and L, P<0.05, ANOVA with post hoc Tukeys test). Based on our findings and literature, we selected a dose of 75 nM and a duration of 45 min for PMA treatment in the following experiments (15).

To determine whether EYK can alter cell migration in human malignant cells, we performed wound healing assays on U373MG, T98G and A172 cells pre-treated with PMA (75 nM) or vehicle for 45 min, and then treated with EYK (200 µg/ml) or vehicle for 24 h. As expected, PMA alone significantly increased cell migration in all three cell lines (Fig. 3A-F). EYK did not alter PMA-induced cell migration in comparison with PMA in U373MG or T98G cells (Fig. 3A-D, P<0.001; ANOVA with post hoc Tukeys test). By contrast, EYK significantly suppressed PMA-mediated cell migration in A172 cells (Fig. 3E and F, P<0.001; ANOVA with post hoc Tukeys test).

Next, we performed Transwell assays to investigate whether EYK can regulate cell invasion. To this end, A172 cells were pre-treated with PMA or vehicle for 45 min, treated with vehicle or EYK (200 µg/ml) for 24 h, and then subjected to cell invasion assays. PMA increased cell invasion in comparison with vehicle (Fig. 3G and H, P<0.05; ANOVA with post hoc Tukeys test, CON vs. PMA, P=0.057; two-tailed t-test). However, EYK inhibited PMA-induced cell invasion (Fig. 3G and H). Together, these data indicate that EYK can inhibit PMA-mediated cell migration and invasion, at least in monomorphic malignant human glioma cells.

To determine whether EYK regulates activity and expression of MMPs, which are involved in cell migration and invasion (15,17), we pre-treated A172 cells with PMA (75 nM) or vehicle for 45 min, treated with EYK (200 µg/ml) or vehicle for 24 h, and then conducted gelatin zymography assays. PMA significantly increased MMP-9 activity compared to vehicle (Fig. 4A and B, P<0.001; ANOVA with post hoc Tukeys test). EYK significantly decreased PMA-induced MMP-9 activity (Fig. 4A and B).

In order to examine the effects of EYK on MMP-9 and TIMP-1 mRNA levels, we conducted RT-PCR under the same conditions as described above. We found that PMA significantly increased MMP-9 and TIMP-1 mRNA levels compared to vehicle (Fig. 4C-F). EYK significantly decreased PMA-mediated MMP-9 mRNA levels (Fig. 4C and D, P<0.001; ANOVA with post hoc Tukeys test), but had no effect on TIMP-1 mRNA levels (Fig. 4E and F). These data suggest that EYK can regulate PMA-induced MMP-9 activity as well as its mRNA levels.

We then investigated whether EYK requires MMP-9 activity to alter cell migration. For this purpose, A172 cells were pre-treated with vehicle or PMA (75 nM), treated with CAS1177749-58-4 (an MMP-9 inhibitor, 5 µM) for 1 h, exposed to vehicle or EYK (200 µg/ml) for 24 h, and then subjected to the wound healing assay. Consistent with our findings above, PMA significantly increased cell migration but EYK significantly decreased PMA-induced cell migration (Fig. 4G and H, P<0.001; ANOVA with post hoc Tukeys test). In addition, pretreatment with PMA, MMP-9 inhibitor, and EYK treatment further decreased cell migration compared to treatment with PMA and EYK (Fig. 4G and H). Moreover, we found that treatments with PMA, MMP-9 inhibitor, and EYK significantly reduced MMP-9 activity compared to PMA and EYK treatment (Fig. 4I and J; P<0.001; ANOVA with post hoc Tukeys test, PMA+CAS vs. PMA+CAS+EYK; two-tailed t-test).

A transcriptional factor NF-κB plays an important role in cell migration and invasion by regulating MMP activity (18). Hence, we initially investigated whether EYK could alter PMA-induced NF-κB levels in the cytosol vs. the nucleus. For these experiments, A172 cells were pre-treated with PMA (75 nM) or vehicle for 45 min, treated with EYK (200 µg/ml) or vehicle for 45 min, and then subjected to subcellular fractionation. PMA treatment showed a trend toward increased p-IκBα and NF-κB levels, but decreased IκBα levels in the cytosol (Fig. 5A-D; P<0.01; ANOVA with post hoc Tukeys test). EYK did not alter PMA-induced p-IκBα and IκBα levels, but significantly decreased PMA-mediated NF-κB levels in the cytosol (Fig. 5A-D). In addition, EYK did not alter the PMA-induced NF-κB levels in the nucleus (Fig. 5E and F, P<0.01; ANOVA with post hoc Tukeys test).

We then asked whether EYK could alter NF-κB subcellular localization when administered for longer periods of time. To answer this question, A172 cells were pre-treated with PMA (75 nM) or vehicle for 45 min, treated with EYK (200 µg/ml) or vehicle for 24 h, and then subjected to subcellular fractionation. EYK slightly decreased PMA-induced p-IκBα and NF-κB levels, but did not alter IκBα levels in the cytosol (Fig. 5G-J, P<0.001; ANOVA with post hoc Tukeys test). In addition, EYK significantly decreased PMA-mediated NF-κB levels in the nucleus (Fig. 5K and L, P<0.05; P<0.001; ANOVA with post hoc Tukeys test).

To examine whether EYK can alter PMA-induced p-NF-κB levels in the nucleus, A172 cells were pre-treated with PMA (75 nM) or vehicle for 45 min, treated with EYK (200 µg/ml) or vehicle for 24 h, and then immunostaining were performed. PMA significantly increased p-NF-κB levels in the nucleus (Fig. 5M and N, P<0.001; ANOVA with post hoc Tukeys test). EYK significantly decreased PMA-induced p-NF-κB levels in the nucleus (Fig. 5M and N). These data suggest that EYK can alter NF-κB nuclear translocation between subcellular compartments.

To determine whether EYK requires NF-κB to suppress cancer cell migration, we performed wound healing assays on A172 cells pre-treated with PMA (75 nM) or vehicle for 45 min, treated with BAY 11–7085 (10 µM, a NF-κB inhibitor) or vehicle for 1 h, and then treated with EYK (200 µg/ml) or vehicle for 24 h (Fig. 6A and B, P<0.05; P<0.001; ANOVA with post hoc Tukeys test). Treatments with PMA, NF-κB inhibitor, and EYK significantly inhibited cell migration in comparison with treatments with PMA and EYK, suggesting that NF-κB is necessary for EYK to regulate cell migration.

Next, we examined the effects of EYK on MMP-9 activity by treating cells with PMA and NF-κB inhibitor and found that inhibition of NF-κB in combination with EYK treatment further decreased PMA-induced MMP-9 activity in comparison with PMA and EYK treatments (Fig. 6C and D, P<0.05; P<0.01; P<0.001; ANOVA with post hoc Tukeys test).

To determine whether pre-treatment with EYK can modulate cell migration, we performed wound healing assays on A172 cells pre-treated with vehicle or EYK (200 µg/ml) for 45 min, treated with PMA (75 nM) or vehicle for 24 h, and then wound healing assays were conducted. PMA significantly increased cancer cell migration, but this effect was suppressed by pre-treatment with EYK (Fig. 7A and B, P<0.001; ANOVA with post hoc Tukeys test).

Next, we performed the Transwell assays to investigate the effects of pre-treatment with EYK on cell invasion and found that PMA significantly increased cell invasion while pre-treatment with EYK significantly inhibited PMA-induced cell invasion (Fig. 7C and D, P<0.05; ANOVA with post hoc Tukeys test).

We then investigated whether pre-treatment with EYK could alter MMP-9 activity and found that pre-treatment with EYK significantly decreased PMA-induced MMP-9 activity (Fig. 7E and F, P<0.001; ANOVA with post hoc Tukeys test). Moreover, pre-treatment with EYK significantly decreased PMA-induced MMP-9 mRNA levels, but had no effect on TIMP-1 mRNA levels (Fig. 7G-I, P<0.05; P<0.001; ANOVA with post hoc Tukeys test).

To determine whether pre-treatment with EYK can regulate PMA-induced NF-κB subcellular translocation, we pre-treated A172 cells with EYK (200 µg/ml) or vehicle for 45 min, treated with PMA (75 nM) or vehicle for 24 h, and then performed subcellular fractionation. Pre-treatment with EYK followed by PMA treatment showed a trend toward decreased p-IκBα levels and did not alter IκBα and NF-κB levels in the cytosol (Fig. 8A-D, P<0.05; ANOVA with post hoc Tukeys test). In the nuclear fraction, pre-treatment with EYK significantly decreased PMA-induced NF-κB levels (Fig. 8E and F, P<0.01; P<0.001, ANOVA with post hoc Tukeys test). Moreover, pre-treatment with EYK significantly decreased PMA-induced p-NF-κB levels in the nucleus (Fig. 8G and H, P<0.001; ANOVA with post hoc Tukeys test).

We then investigated whether pre-treatment with EYK could alter cell migration via NF-κB pathways. To test this, we performed wound healing assays on A172 cells pre-treated with vehicle or BAY11-7085 (10 µM, an NF-κB inhibitor) for 1 h, treated with EYK (200 µg/ml) or vehicle for 45 min, and then treated with PMA 75 nM) or vehicle for 24 h. Pre-treatment with EYK decreased PMA-induced cell migration (Fig. 8I and J, P<0.05; P<0.001, ANOVA with post hoc Tukeys test; EYK+PMA vs. BAY+EYK+PMA, two-tailed t-test). In addition, pre-treatment with NF-κB inhibitor followed by treatments with EYK and PMA further inhibited cell migration in comparison with treatments with EYK and PMA (Fig. 8I and J). Based on these findings, we conclude that EYK could be used as a drug to prevent cancer cell migration by decreasing the nuclear localization of NF-κB and MMP-9 activity in A172 cells (Fig. 8K).