DPH was obtained from Sigma-Aldrich (St. Louis, MO, USA). The pan-caspase inhibitor z-VAD.fmk was purchased from Cayman Chemical (Ann Arbor, MI, USA).

Human melanoma cell lines A2058 (no. CRL-11147), A375.S2 (no. CRL-1872), MDA-MB-435S (no. HTB-129) and murine B16-F10 melanoma cell line [no. CRL-6475; all from American Type Culture Collection (ATCC), Manassas, VA, USA] were grown at 37°C and 5% CO₂ in the culture media recommended by ATTC. Primary human melanocytes were obtained from Invitrogen Life Technologies (Carlsbad, CA, USA) and grown in culture media according to the manufacturers instructions. All culture media and supplements were purchased from Invitrogen Life Technologies.

DPH-elicited cytotoxicity was evaluated by the levels of cell viability after drug treatment using an MTS assay (Promega Corp., Madison, WI, USA), which was performed according to our established protocol (11). In the present study, cells were seeded onto 96-well plates at a density of 8×10³ cells/well, followed by drug treatment and subsequent MTS assay.

Apoptosis induced by DPH was determined by Annexin V/PI dual staining assay using an ApoTarget™ Annexin V-FITC Apoptosis kit (BioSource International, Inc., Camarillo, CA, USA) following our reported protocol (11). Data acquisition and analysis were performed on FACScan flow cytometer (BD Biosciences, USA). Results are expressed as the mean ± SEM of at least three independent experiments. Cells with Annexin V-positive staining are recognized as cells undergoing apoptosis.

The open reading frames (ORF) of human MCL-1 (Genbank accession no. NM_021960) were PCR-amplified from the first-strand cDNA pools of human colon adenocarcinoma cell line HCT116 using the following primer pair: MCL-1 forward, 5-ACCggTTTTggCCTCAAAAgAAAC-3 and MCL-1 reverse, 5-CAgTAAggCTATCTTATTAgATATg-3. The ORF of the constitutive STAT3 mutant (A661C/N663C) was PCR-amplified using the plasmid pMXs-Stat3-C (plasmid #13373; Addgene, Inc., Cambridge, MA, USA) as the template. The PCR-amplified ORFs were then subcloned to the retroviral vector pBabe.puro engineered to encode an in-frame N-terminal hemagglutinin (HA) epitope (pBabe-HA). The resultant expression plasmids for MCL-1 (pBabe-HA-MCL-1) or STAT3 (pBabe-HA-STAT3-CA) were then subjected to production of retroviral particles for subsequent cell infection and puromycin selection for stable infectants according to our published protocol (11).

Immunoblotting was performed as previously described (11). Polyclonal antibodies against MCL-1, BCL-xL, BAX, HA epitope, total ERK, phospho-ERK (Thr202/Tyr204), total STAT3, phospho-STAT3 (Tyr705), and the cleaved forms of poly(ADP-ribose) polymerase (PARP), caspase-3, caspase-8 and caspase-9 were all purchased from Cell Signaling Technology (Beverly, MA, USA). α-tubulin antibody was purchased from GeneTex (Irvine, CA, USA). The signals were detected with an enhanced SuperSignal West Pico chemiluminescence kit (Pierce, Rockford, IL, USA).

The in vivo anti-melanoma effect of DPH was evaluated using the murine B16-F10 cell line-based preclinical melanoma model. Briefly, 3×10⁵ B16-F10 cells were subcutaneously injected into the ventral flank of C57BL/6 mice to allow tumor growth for 8 days until reaching the size of 10 mm³. Tumor-bearing mice were then randomized into 2 groups (n=6) and received an i.p injection of 100 µl PBS or DPH (20 mg/kg). Mice were subjected to an i.p. injection every other day. Tumor volumes were calculated with a digital caliper as length × width × thickness × 0.5 and expressed in mm³ before each treatment. Mice were euthanized when the tumor size reached <2,000 mm³ in mean diameter. All treatments were performed according to the guidelines approved by IACUC of the National Chung Hsing University.

All data from in vitro experiments were expressed as means ± standard error of the mean (SEM) from at least three independent experiments. Differences between groups were evaluated for statistical significance using a Student's t-test. A p-value <0.05 was regarded as the minimum criteria for statistical significance. As for the in vivo studies, the Kaplan-Meier method and log-rank test using GraphPad Prism software package version 5.0 (GraphPad Software, Inc., San Diego, CA, USA) were employed to compare the survival rates between vehicle controls and DPH-treated mice. Differences were considered significant at p<0.05.

To comprehensively explore the anti-melanoma activity of DPH, we started by testing the in vitro cytotoxic effect of DPH on a panel of melanoma cell lines, including murine B16-F10 cells (BRAF wild-type) and human A2058, A375.S2 and MDA-MB-435S cells (all carrying the BRAF^V600E mutation) in addition to normal human melanocytes. As shown in Fig. 1A, DPH was cytotoxic against all melanoma cell lines tested; in contrast, normal human melanocytes were refractory to DPH-elicited cell death. Additionally, we found that DPH treatment led to a marked increase in Annexin V-positive (apoptotic) cells in both the A2058 (from 8.96±0.49 to 33.10±2.12%, p<0.001) and A375.S2 (from 8.65±0.49 to 30.36±2.68%, p<0.001) cell lines (Fig. 1B), illustrating the induction of apoptosis. Immunoblotting further revealed that DPH induced a dose-dependent increase in the levels of caspase-dependent cleavage of PARP in addition to the proteolytic processing and thus activation of caspase-9, caspase-8 and caspase-3 (Fig. 1C). These results thus confirmed the proapoptotic effect of DPH on melanoma cells. Noteworthy, pre-treatment with the pan-caspase inhibitor z-VAD.fmk significantly rescued A2058 and A375.S2 cells from DPH-induced cell death (Fig. 1D). Altogether, our results established the anti-melanoma effect of DPH through the induction of apoptosis-dependent cytotoxicity.

We next addressed whether the in vitro cytotoxicity of DPH accounts for its in vivo anti-melanoma effect. Using the well-established B16-F10 melanoma mouse model, we found that i.p. administration of DPH (20 mg/kg) evidently suppressed tumor growth compared to the vehicle control (Fig. 2A and B). Furthermore, the tumor volume was decreased to nearly 30% of the vehicle control 19 days after DPH administration (from 1750±176 to 610±209 mm³, p<0.001). It is also noteworthy that DPH markedly prolonged the survival of the B16-F10-bearing mice (Fig. 2C). Overall, these results validated the in vivo anti-melanoma effect of DPH.

The mechanism underlying the proapoptotic action of DPH was further investigated. We started by testing the effect of DPH on the expression of proteins responsible for the control of apoptosis initiation, including proapoptotic BAX and antiapoptotic BCL-xL and MCL-1. It is noteworthy that only MCL-1 was markedly reduced by DPH in both the A2058 and A375.S2 cells (Fig. 3A). Given that MCL-1 is fundamental for melanoma progression, relapse and drug resistance (12–14), the role of MCL-1 downregulation in DPH-elicited anti-melanoma activity was further examined in the A2058 and A375.S2 clones stably overexpressing MCL-1. We found that MCL-1 overexpression potently rescued cells from DPH-evoked cell death (Fig. 3B and C). Immunoblotting further revealed noticeable reduction in DPH-induced PARP cleavage in the MCL-1 stable clones (Fig. 3D and E), suggesting that MCL-1 overexpression blunts DPH-elicited apoptosis. Collectively, we conclude that downregulation of MCL-1 is integral to the proapoptotic action of DPH.

We next explored how DPH downregulates MCL-1. It has been shown that oncogenic BRAF^V600E-initiated persistent ERK signaling upregulates MCL-1 (15). However, immunoblotting showed limited alteration in the levels of phospho-ERK (Thr202/Tyr204) following DPH treatment (Fig. 4A), suggesting that DPH failed to inhibit ERK signaling to decrease MCL-1. Alternatively, we tested the effect of DPH on the activation of STAT3 [revealed by phosphorylation of tyrosine 705 (p-Y705-STAT3)], considering that MCL-1 is a known transcriptional target of STAT3 (16). In addition, constitutive activation of STAT3 is associated with melanoma tumorigenesis, progression and chemoresistance through the upregulation of the transcription of genes promoting cell proliferation, survival, angiogenesis and metastasis (12,17,18). Our results indicated that DPH impeded constitutive STAT3 activation, as evidenced by the decrease in the levels of p-Y705-STAT3 in both the A2058 and A375.S2 cells (Fig. 4A). Furthermore, overexpression of a constitutively active STAT3 mutant (HA-STAT3-CA) effectively protected cells from DPH-induced cell death (Fig. 4B and C), likely through the reduction of apoptosis (Fig. 4D), thus illustrating an essential role of STAT3 blockage in the proapoptotic action of DPH. Moreover, HA-STAT3-CA-expressing cells displayed an increase in the basal levels of MCL-1 but also markedly restored MCL-1 expression levels following DPH treatment (Fig. 4E), indicating that DPH downregulates MCL-1 by impairing STAT3-mediated induction of MCL-1. Overall, we conclude that DPH likely blocks the STAT3-MCL-1 survival signaling pathway to induce apoptosis in melanoma cells.