Research ArticleExperimental Studies

BRAF Inhibitors and Radiation Do Not Act Synergistically to Inhibit WT and V600E BRAF Human Melanoma

LISA WALTER and LUCIE HEINZERLING
Anticancer Research March 2018, 38 (3) 1335-1341;

Abstract

Background/Aim: Recent evidence suggests that melanoma patients treated with BRAF inhibitors experience radiosensitization with an increased frequency of side-effects. This could also imply increased effectiveness when treating melanoma. Materials and Methods: To test whether the BRAF inhibitors dabrafenib and vemurafenib together with ionizing radiation more effectively inhibit melanoma cells, primary human melanoma tumor cell lines expressing wild-type (WT) or mutant V600E BRAF were analyzed by cell survival, cell death, and cell-cycle testing. Results: All melanoma cell lines examined were radioresistant in these assays. BRAF inhibitor treatment alone suppressed cell survival more effectively than radiation in all the mutant V600E BRAF cell lines, and vemurafenib, but not dabrafenib, also inhibited cell survival in the WT BRAF cell lines at clinically relevant concentrations. However, when cells were treated with BRAF inhibitor followed by radiation, there was no increased effect on the suppression of cell survival. Vemurafenib induced more necrosis than radiation in most melanoma cell lines, irrespective of BRAF status, but this effect was not additive with the combination treatment. BRAF inhibitors and radiation had variable, but independent effects on the induction of cell-cycle arrest. Conclusion: These results suggest that BRAF inhibitors and ionizing radiation do not act synergistically to inhibit the growth of primary human melanoma cells.

Therapeutic options for patients with melanoma have been rapidly evolving. The identification of activating point mutations in the gene encoding the serine-threonine protein kinase BRAF in over 60% of melanomas (1, 2) greatly altered the treatment landscape, as small-molecule inhibitors directed against V600 mutant BRAF were subsequently developed. Mutant BRAF constitutively activates the mitogen-activated protein kinase (MAPK) pathway, increasing cell proliferation and preventing apoptosis (1, 3). The substitution of valine by glutamic acid at codon 600 (BRAF V600E) is the most common BRAF gene mutation in cutaneous melanoma (4-7), and the BRAF V600E-selective inhibitors vemurafenib (8) and dabrafenib (9) have been shown to reduce the kinase activity of this protein.

Vemurafenib (10, 11) and dabrafenib (12) are currently used as standard treatment for patients with metastatic BRAF V600-mutated melanoma. Although overall survival is improved with BRAF-inhibitor therapy alone and in combination with mitogen-activated protein kinase kinase (MEK) inhibitors (13), drug resistance remains a major factor that limits BRAF-inhibitor clinical efficacy, and strategies to overcome this will improve clinical outcome. BRAF inhibitors have been reported to induce radiosensitization in melanoma patients, with vemurafenib increasing radiosensitivity more than dabrafenib and an increased frequency of side effects (14). Currently, there is no standard approach to the concomitant use of BRAF inhibitor therapy with radiotherapy. The aim of this study was to investigate whether a potential synergy between BRAF inhibitor therapy and radiotherapy on melanoma cells exists. Primary human melanoma cell lines expressing WT or V600E mutant BRAF were treated with BRAF inhibitors, with or without MEK inhibitors, followed by ionizing radiation, and cell survival was analyzed. Cell death and cell cycle responses were also evaluated following treatment with BRAF inhibitors and radiation.

Materials and Methods

Cell lines and BRAF mutational analyses. Primary human melanoma cells (from primary tumors) were collected in the Department of Dermatology of the University Hospital of Erlangen following approval by the institutional review board. Single cell suspensions were generated by digesting tissue samples with collagenase (Sigma, Darmstadt, Germany), hyaluronidase (Sigma, Darmstadt, Germany), and DNAse (Roche, Mannheim, Germany). Continuous cell culture was performed in RPMI (Lonza, Cologne, Germany) supplemented with 20% fetal calf serum (FCS, PAA, Freiburg, Germany), L-glutamine (2 mM, Lonza), HEPES (PAA), pyruvate (PAA), nonessential amino acids (PAA), and gentamicin (20 μg/ml, PAA) with 1 to 2 passages per week. To avoid changes in cell physiology over time, cells were used at a low passage number (<10). For experiments, cells were cultured in RPMI supplemented with 10% FCS, L-glutamine, and gentamicin. The BRAF gene in each cell line was confirmed by pyrosequencing to show the presence (V600E) or absence (WT) of the BRAF V600E mutation.

View this table:
Table I.

Clinically relevant human plasma concentrations and experimental concentrations used in the present study for BRAF inhibitors vemurafenib and dabrafenib and MEK inhibitors trametinib and cobimetinib.

Drug treatments and radiation. Drugs were purchased from Hoelzel Diagnostika (Cologne, Germany). Stock concentrations of the BRAF inhibitors vemurafenib (100 mM) and dabrafenib (10 mM) and the MEK inhibitors trametinib (10 mM) and cobimetinib (10 mM) were prepared in dimethylsulfoxide (DMSO) and stored at −80°C. Cells were treated with either drug or vehicle (DMSO) for the indicated times at the concentrations listed. Ionizing radiation (2, 6, or 10 Gy) was generated by a General Electric Isovolt 160 with a dose rate of 4 Gy/min.

Cell survival. Cell survival assays were performed in duplicate wells in 96-well flat-bottom plates. Four hours following seeding, cells were treated with drug or vehicle, and the WST-1 assay (Roche, Mannheim, Germany) was executed at the indicated time points. Plates were read at a wavelength of 450 nm with a Wallac Victor 2 plate reader operated by Wallac 1420 Manager software. For radiation experiments, cells were irradiated 20 hours following drug treatment, and the WST-1 response was measured the following day.

Cell death. For analyses of cell death, cells were cultured in 6-well plates and treated with drugs 4 hours later. After 20 hours, cells were irradiated, and, after an additional day, harvested with trypsin. Early apoptotic cell death was measured by annexin V (eBioscience, Darmstadt, Germany) single-positive staining, and necrotic death was measured by propidium iodide (eBioscience, Darmstadt, Germany) positive staining according to the manufacturer's instructions. Cells were measured with a BD FACS Canto II flow cytometer operated with BD FACS Diva software. All flow cytometry analyses were performed with FlowJo Version 10 software with gating on singlet events.

Cell cycle. For cell cycle analyses, cells were treated and harvested as per the cell death analyses, but instead washed in PBS, fixed in 70% ethanol on ice for 20 min, washed twice in PBS, and stained with propidium iodide (50 μg/ml) in PBS containing RNase (20 μg/ml, Qiagen, Hilden, Germany). Cells were measured in a linear range with a BD FACS Canto II flow cytometer operated with BD FACS Diva software. Singlet events were gated with FlowJo Version 10 software.

Statistics. All statistical analyses were performed with IBM SPSS Statistics 20 software.

Results

Dabrafenib and vemurafenib rapidly inhibited primary human mutant V600E BRAF melanoma cells at clinically relevant concentrations. Primary human melanoma cell lines expressing wildtype BRAF (TZ05, TZ07, and TZ08) or mutant V600E BRAF (TZ02, TZ03, TZ04, and TZ06) were treated for 2 days with dabrafenib, vemurafenib, or vehicle (DMSO) at concentrations equivalent to the published plasma concentrations of melanoma patients treated with these drugs (Table I) as well as lower concentrations, which may better correspond with the amount of drug that reaches the tumor cells in vivo. Responses in the WST-1 cell survival assay showed that the mutant V600E BRAF cell lines were more sensitive to dabrafenib than the WT BRAF cell lines in the range of 10 nM to 3 μM (Figure 1A). Vemurafenib inhibited all the cell lines tested at a concentration of 60 μM, with all 4 mutant V600E BRAF cell lines sensitive to concentrations as low as 1 μM (Figure 1B). For further experiments, the clinically relevant concentrations of 1 μM for dabrafenib and 60 μM for vemurafenib were used.

Subsequently, a time course of melanoma cell line responses to BRAF inhibitors was established. Whereas the mutant BRAF cell lines were inhibited by dabrafenib at all time points examined, the WT BRAF cell lines showed minimal or no response (Figure 1C). The mutant V600E BRAF cell lines were also inhibited by a single treatment of vemurafenib by day 1, and this inhibition was sustained at days 2, 3, and 4 (Figure 1D). The WT BRAF cell line TZ07 showed minimal inhibition to vemurafenib, while TZ08 was inhibited 20% and TZ05 60% by day 2, responses that were sustained until day 4 (Figure 1D).

BRAF inhibitors and MEK inhibitors reduced melanoma cell survival more effectively than radiation. Based on the results of the BRAF inhibitor dose-response and time course experiments, melanoma cell lines were treated with a combination of drugs and varying doses of ionizing radiation (0, 2, 6, and 10 Gy). The MEK inhibitors trametinib and cobimetinib were also tested alone and in combination with BRAF inhibitors according to their use as a clinical treatment for melanoma patients, i.e. vemurafanib with cobimetinib, or dabrafenib with trametinib. Results from the representative cell lines TZ03 (for mutant V600E BRAF) and TZ07 (for WT BRAF) are illustrated in Figures 2, 3 and 4.

Figure 1.
Figure 1.

Primary human melanoma cell survival responses to BRAF inhibitors. WT and mutant V600E BRAF melanoma cell lines were exposed to increasing concentrations of (A) dabrafenib and (B) vemurafenib, and the WST-1 responses were measured following 2 days of drug treatment. Melanoma cell lines treated with (C) 1 μM dabrafenib and (D) 60 μM vemurafenib were also examined at the indicated time points. Data are presented as mean±SEM of 2 to 4 separate experiments performed in duplicate.

All mutant V600E BRAF melanoma lines tested were sensitive to BRAF inhibitors, MEK inhibitors, and the combination treatments in the WST-1 assay (Figures 1 and 2). WT BRAF cell lines were less sensitive to BRAF inhibitors than the mutant BRAF cell lines, with the exception of TZ05, which was inhibited by vemurafenib (Figure 1). MEK inhibitors and the combination BRAF inhibitor/MEK inhibitor treatments suppressed the WT BRAF cell lines in a manner similar to the mutant BRAF cell lines (Figure 2). In all cell lines tested, the responses to combination BRAF inhibitor/MEK inhibitor treatment were similar to the responses to MEK inhibitor alone (Figure 2).

Regardless of BRAF mutation status, all melanoma cell lines tested were radio-resistant (Figure 2). For cell lines that were sensitive to vemurafenib or dabrafenib, BRAF inhibitor treatment alone inhibited cell survival better than radiation alone (Figure 2). MEK inhibitor treatment suppressed cell survival more than radiation in all cell lines (Figure 2).

To test for a synergistic effect of BRAF inhibitors and ionizing radiation, the WST-1 response of cells to radiation was compared with the response to radiation following drug treatment. Although the mutant V600E BRAF cell lines had a reduced cell survival in the presence of BRAF inhibitor plus radiation compared with radiation alone (Figure 2 A), this effect was not synergistic because it was similar to the response to BRAF inhibitor treatment alone. All cell lines tested had reduced cell survival in the presence of radiation plus a MEK inhibitor (with or without a BRAF inhibitor) compared with radiation alone, but this effect was also not additive because it was similar to MEK inhibitor treatment alone (Figure 2).

Figure 2.
Figure 2.

WST-1 cell survival responses of melanoma cell lines to radiation, BRAF inhibitors, and MEK inhibitors. Mutant V600E BRAF (A) and WT BRAF (B) melanoma cell lines were treated with vemurafenib, dabrafenib, trametinib, cobimetinib, vemurafenib plus cobimetinib, or dabrafenib plus trametinib prior to radiation at 0, 2, 6, or 10 Gy. Data are presented as mean±SEM of 3 separate experiments performed in duplicate. A two-way ANOVA was conducted on the influence of drug and radiation on cell survival. The effect of drugs (p<0.05), but not radiation or the interaction effect, was statistically significant for all cell types.

Figure 3.
Figure 3.

Melanoma cell death responses to BRAF inhibitors and radiation. Mutant V600E BRAF (A) and WT BRAF (B) melanoma cell lines were treated with vemurafenib or dabrafenib followed by 0 or 6 Gy radiation, and early apoptosis and necrosis were measured by flow cytometry. Annexin+/propidium iodide singlet events (white) and propidium iodide+ singlet events (black) as a percent of the total cell population are shown as mean±SEM of 3 separate experiments. Asterisks indicate statistical significance compared with corresponding control (*p<0.05 in a one-way ANOVA followed by a Bonferroni post-hoc test).

Dabrafenib and vemurafenib did not alter the melanoma cell death response to radiation. The cell death profile was analyzed by annexin+/propidium iodide staining for early apoptosis and by propidium iodide+ staining for necrosis in the melanoma cell lines following treatment with the BRAF inhibitors vemurafenib or dabrafenib, 6 Gy radiation, or a combination of BRAF inhibitor plus radiation. Radiation alone did not increase apoptotic or necrotic cell death in all cell lines tested (Figure 3). Dabrafenib treatment significantly increased apoptotic, as well as necrotic cell death in the mutant V600E BRAF cell line TZ06, but not in the other cell lines (Figure 3 and data not shown). Vemurafenib significantly increased necrosis in all of the melanoma cell lines, except TZ04, regardless of BRAF status, but it did not alter apoptosis (Figure 3 and data not shown).

The cell death responses to BRAF inhibitor treatment plus radiation were not significantly different from the responses to BRAF inhibitor alone (Figure 3). Taken together, these results suggest that BRAF inhibitors do not sensitize melanoma cells to radiation.

Radiation and BRAF inhibitors independently induced cell-cycle arrest in melanoma cells. To determine whether BRAF inhibitors and radiation induce changes in the primary melanoma cell cycle, WT and mutant V600E BRAF melanoma cell lines were treated with drugs or vehicle followed by 6 Gy radiation. The cell cycle was examined in fixed cells by propidium iodide labeling and analyzed by flow cytometry 24 hours post-irradiation. As shown in Figure 4, radiation increased G2 cell-cycle arrest in all melanoma cell lines.

Figure 4.
Figure 4.

Cell-cycle analyses of melanoma cell lines following treatment with BRAF inhibitors and radiation. Mutant V600E BRAF (A) and WT BRAF (B) melanoma cell lines were treated with vemurafenib or dabrafenib followed by 0 or 6 Gy radiation, and the cell cycle was assessed. Data are presented as mean±SEM of 3 separate experiments.

Dabrafenib increased G1 cell-cycle arrest in all the mutant V600E BRAF cell lines (Figure 4 A). Vemurafenib increased G1 arrest in TZ02, TZ03, TZ04, and TZ05 and G2 arrest in TZ06 and TZ07 (Figure 4 and data not shown).

BRAF inhibitor treatment prior to radiation led to a cell cycle profile similar to BRAF inhibitor alone in melanoma lines that were sensitive to BRAF inhibitors in this assay (Figure 4). For cell lines that were not sensitive to BRAF inhibitors, the combination treatment of BRAF inhibitor plus radiation yielded a cell cycle profile similar to radiation alone (Figure 4B).

Discussion

The results presented here show that dabrafenib rapidly and selectively inhibited cell survival of primary human mutant V600E BRAF melanoma cell lines, and that vemurafenib inhibited mutant BRAF as well as some WT BRAF melanoma lines. All cell lines tested were resistant to 10 Gy of ionizing radiation. BRAF inhibitor plus ionizing radiation did not inhibit cell survival better than either treatment alone in any of the cell lines tested. Although vemurafenib increased necrotic cell death in 6 of the 7 melanoma lines, it had no effect on apoptosis. Dabrafenib only increased necrotic and apoptotic cell death in the mutant V600E BRAF line TZ06. These discrepancies between dabrafenib and vemurafenib may be due to the higher specificity of dabrafenib to mutant BRAF compared to vemurafenib, which also binds WT BRAF and CRAF (15, 16). We found that radiation and BRAF inhibitors induced varying but independent effects on cell cycle arrest. No synergistic or additive effects of BRAF inhibitors and radiation were observed in any of the assays. Based on the results presented here, we would expect that the antitumor effects of BRAF inhibitors and radiotherapy are not enhanced by concomitant use.

A previous in vitro study has shown that vemurafenib can induce radiosensitization in mutant BRAF cancer cell lines. Radiosensitivity was observed in 4 melanoma cell lines harboring the V600E BRAF mutation, but not in WT lines, when treated with vemurafenib and ionizing radiation in a colony-forming assay (17). Differences in results may be due to the individual nature of human tumor cell lines, the passage number at which the cell lines were used, as well as the assays. A colony-forming assay will discriminate between cells that are senescent, which are generally detected as dying in shorter-term assays, versus cells that have been damaged and no longer have the ability to replicate (also detected as dying in shorter-term assays). Since we did not observe any short-term additive effects with BRAF inhibitors plus radiation on cell survival, cell death, or cell cycle, no longer-term additive effects are expected with these experimental conditions. An additive effect of the BRAF inhibitor PLX4720 and ionizing radiation was also observed in various mutant V600E BRAF cancer cell lines but not in WT lines (18, 19). However, these studies are difficult to compare with ours, as they did not use dabrafenib or vemurafenib, and they only included one melanoma cell line.

In summary, our data suggest that the BRAF inhibitors dabrafenib and vemurafenib do not synergize with ionizing radiation to inhibit the growth of primary human melanoma cells. Neither synergistic nor additive effects of BRAF inhibition and ionizing radiation were observed in assays of cell survival, cell death, and cell cycle. Although BRAF inhibitors may lead to radiosensitivity side-effects in patients, our study does not support the possibility that this may carry over into a potential treatment regimen in melanoma.

Acknowledgements

The Authors thank Waltraud Froehlich for excellent technical support, Regine Schneider-Stock for BRAF sequencing, Luitpold Distel for use of the radiation chamber, and Gerold Schuler for general support. This work was supported by Novartis Pharma GmbH (Nuremberg, Germany) and the German Federal Ministry of Education and Research (BMBF).

  • Received December 21, 2017.
  • Revision received January 31, 2018.
  • Accepted February 1, 2018.

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BRAF Inhibitors and Radiation Do Not Act Synergistically to Inhibit WT and V600E BRAF Human Melanoma
LISA WALTER, LUCIE HEINZERLING
Anticancer Research Mar 2018, 38 (3) 1335-1341;
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