Human pancreatic cancer cell lines MIA PaCa-2 and Panc-1 were obtained from American Type Culture Collection (Manassas, VA, USA). Cells were cultured in Dulbecco’s modified Eagle’s medium (DMEM) supplemented with 10% fetal bovine serum (FBS), 1% penicillin-streptomycin at 37°C in a 5% CO₂ humidified environment.

ASP, CUR and SFN were purchased from LKT Laboratories (St. Paul, MN, USA). The chemical inhibitor U0126 was purchased from Cell Signaling Technology (Beverly, MA). Antibodies against Phospho-ERK1/2 (Thr202/Tyr204), total ERK1/2, P-p38 MAPK (Thr180/Tyr182), P-Akt (Ser474), total AKT, P-c-jun (Ser73), P-p53 (Ser15), cleaved caspase-3 (Asp175), cleaved PARP (Asp214), P-IκBα (Ser32/36) and β-actin were purchased from Cell Signaling Technology.

The cell viability assay was performed according to the manual included with the Promega CellTitre 96 Aqueous MTS reagent (Madison, WI, USA). Briefly, 5×10³ cells were seeded in 96-well plates. Test compounds ASP, CUR and SFN alone and in combination ACS were added for a period of 72 h. On the last day of the incubation period, 20% MTS and 1% of phenazine methosulfate (PMS) were added to culture medium and incubated for 3 h at 37°C and measured at 490 nm. All the assays were performed in triplicates.

The 1×10⁴ cells were seeded into the six-well plates in triplicate per data point. After 24 h of seeding, cells were treated with ASP, CUR and SFN alone and in combinations ACS. Two weeks after treatment, cells were fixed and stained with 0.5% crystal violet (Sigma) in methanol for 5 min. Then, colonies consisting of 50 or more cells were counted. The percentage cell survival was calculated (plating efficiency of non-treated cultures = 1).

The detection was performed according to Annexin V-fluorescein isothiocyanate (FITC) Vybrant Apoptosis assay kit #3 (Invitrogen, Grand Island, NY, USA). MIA PaCa-2 and Panc-1 cells (~3×10⁵) were seeded in six-well plates and treated with ASP, CUR and SFN alone and in combination ACS for 48 h. The cell suspension of 1×10⁵ cells was then subjected to 5 μl of FITC Annexin V and 1 μl of the 100 μg/ml PI followed by incubation in the dark for 15 min. The samples were analyzed using Beckman Coulter Cytomics FC500 (Brea, CA, USA).

The DNA-binding activity of NF-κB in pancreatic cancer cells was quantified by ELISA, using the TransAM NF-κB p50 transcription factor assay kit (Active Motif, Carlsbad, CA, USA). Briefly, 10 μg of total protein was incubated in 96-well plates coated with immobilized oligonucleotide for the p50 subunit. NF-κB binding to the target oligonucleotide was detected by incubation with primary antibody specific for the activated form of p50 (Active Motif), visualized and quantified at 490 nm.

MIA PaCa-2 and Panc-1 cells were treated with ASP, CUR and SFN alone and in combination for 4, 8, 24 and 48 h. Cells were lysed in RIPA buffer and were fractionated onto SDS-PAGE gels and then transferred to nitrocellulose membranes. The membranes were blocked with 2% bovine serum albumin (BSA) in Tris-buffered saline (TBS)-Tween-20 and probed with primary antibodies (1:1000 dilution) followed by horseradish peroxidase (HRP)-labeled secondary antibodies (1:5000 dilutions). The blots were probed with the Super Signal West Pico Chemiluminescent substrate (Thermo Scientific, Pittsburgh, PA, USA) to visualize the immunoreactive bands.

Results were expressed as mean ± SEM. A one-way ANOVA followed by Dunnett’s multiple comparison test post hoc analysis using Graph pad prism software (La Jolla, CA, USA) was performed to analyze and compare the results. A P-value of ≤0.05% was considered significant.

In order to evaluate the effects of ASP, CUR and SFN on pancreatic cancer cells, we treated MIA PaCa-2 and Panc-1 with various concentrations of the ACS treatment for 72 h, and measured cell growth by MTS assay. A dose-dependent reduction of the growth of MIA PaCa-2 and Panc-1 cells (Fig. 1A-C) was observed. In case of MIA PaCa-2, the IC₅₀ concentrations for ASP, CUR and SFN observed were 2.6 mM, 19.6 μM and 10.7 μM, respectively. Similarly, in Panc-1 cells, the IC₅₀ values for ASP, CUR and SFN were calculated to be 2.4 mM, 19.6 μM and 16.0 μM, respectively. Next, to examine the effect of combined regimen on cell proliferation, MIA PaCa-2 and Panc-1 cells were treated with ineffective concentrations of ASP (1 mM), CUR (10 μM) and SFN (5 μM) for 72 h.

As shown in Fig. 2A, individually, the chemopreventive agents did not show significant change in cell viability at these concentrations, thereby demonstrating an ineffective profile. However, when used in combination at same concentrations, ACS showed a significant synergistic effect with a reduction in cell viability of MIA PaCa-2 cells by as much as ~70% (P<0.001). Fig. 2B demonstrated similar results with Panc-1 cells, where combinations of ACS showed a remarkable decrease of ~75% (P<0.001) in cell viability. Notably, when only dual combination studies of ASP with either CUR or SFN were conducted at the same concentration, there was no significant decrease in cell viability, with only ~20% decrease being observed from dual combinations (data not shown). Thus, the triple combination of ACS administered at low concentrations showed a significant reduction in cell viability.

To evaluate long-term efficacy of ACS on cell survival, a clonogenic assay was performed. The survival fraction of the control group was set at 1 (representing 100% cell survival) and the cell survival fraction was calculated based on individual and combination treatment. Quantitatively, an evaluation of cell survival on MIA PaCa-2 cells showed survival fractions of 0.92 (ASP), 0.89 (CUR) and 0.88 (SFN), whereas ACS combination showed significant decrease in the survival fraction of 0.06 (P<0.001) (Fig. 2C). Similar results were observed in case of Panc-1 (Fig. 2D) with low survival fractions of cells.

The induction of apoptosis was measured by flow cytometry for all individual drugs and their combinations on MIA PaCa-2 and Panc-1 cells. Individual concentrations of ASP, CUR and SFN showed minimal apoptotic cells. In case of MIA PaCa-2 cells (Fig. 3A), ASP, CUR and SFN showed approximately 8, 17 and 13% cell death, respectively. However, when mixed in combinations, the ACS combinations demonstrated ~51% cell death (P<0.01). In case of Panc-1 cells (Fig. 3B), ACS combination showed ~63% of apoptotic cells (P<0.01). Overall, our studies confirmed that ACS combinations were extremely effective in inducing apoptosis of cancer cells. Since caspase activity contributes to the overall apoptotic morphology by cleavage of various cellular substrates, we examined the effect of ACS treatment on caspase-3 activation and proteolytic cleavage of PARP using western blotting. As shown in Fig. 3C and D, there were marked increase in the levels of cleaved caspase-3 and cleaved PARP in ACS treatment compared with individual drug alone.

To gain further insight into the mechanism associated with the combination ACS, the DNA binding activity of p50 subunit of the NF-κB complex was evaluated. As shown in Fig. 4A, ~45% (P<0.01) decrease in the p50 binding activity was observed in MIA PaCa-2 cells in the presence of the ACS combination, whereas ~75% (P<0.001) decrease in NF-κB activity occurred in Panc-1 cells (Fig. 4B). These results were confirmed by checking levels of phosphorylated IκBα by Western blotting. As shown in Fig. 4C and D, MIA PaCa-2 cells and Panc-1 cells showed constitutive levels of P-IκBα, whereas treatment with ACS reduced the expression of P-IκBα. Moreover, Akt has been reported to be linked to the activation of IκBα and NF-κB (15). Thus, studies were conducted to examine if combination ACS inhibits phosphorylation of IκBα through inhibition of Akt activation. As presented in Fig. 4C and D, Akt was constitutively active in MIA PaCa-2 and Panc-1 cells respectively, and combination ACS inhibited phosphorylation of Akt, whereas levels of total Akt remained the same.

The ASP, CUR and SFN are reported to modulate ERK-MEK pathway (16–18), hence we wanted to determine whether the ERK-MEK pathway is involved in mediating growth inhibition by combination ACS, MIA PaCa-2 and Panc-1 protein lysates were analyzed by western blot analysis. We observed that incubation of MIA PaCa-2 and Panc-1 cells with combination ACS produced higher phosphorylation of ERK1/2 compared with the control and individual drugs (Fig. 5A and B). We also observed increased in phosphorylation of c-jun, p53 and p38 MAPK proteins. Next, we investigated the activation of ERK1/2 at different time intervals for 4, 8, 24 and 48 h. The expression of phospho-ERK1/2 was profoundly increased after 8 h of ACS treatment, and the ERK activation was persistent for 48 h after ACS treatment. Total ERK1/2 activity remained unchanged during all of these conditions (Fig. 5C and D).

In order to verify the involvement of ERK1/2 activation in ACS-induced apoptosis, we used MEK1/2 inhibitor, U0126, and analyzed by western blot and cell viability assay. The U0126 blocks MEK1/2 phosphorylation and subsequent activation of ERK1/2. MIA PaCa-2 and Panc-1 cells were exposed to combination ACS for 48 h after pretreatment with U0126 (10 μM) for 45 min. As shown in Fig. 6A, ACS-induced phosphorylation of ERK1/2, c-jun and p53 were dramatically blocked by U0126 pretreatment in MIA PaCa-2 cells. There was no effect of U0126 on the amount of total ERK1/2 (Fig. 6A). Similar results were observed in Panc-1 cells (Fig. 6B). These studies demonstrated that ACS activation of ERK1/2 was dependent on MEK1/2.

As U0126 was able to inhibit ERK1/2 phosphorylation induced by ACS, we next investigated whether the U0126 could attenuate ACS-induced reduction in cell viability. As shown in Fig. 6C and D, U0126 alone did not alter the cell proliferation of MIA PaCa-2 and Panc-1 cells, but pretreatment with U0126 partially attenuated ACS induced reduction in cell viability.