An evaluation in vitro of PARP-1 inhibitors, rucaparib and olaparib, as radiosensitisers for the treatment of neuroblastoma

Rucaparib and olaparib were purchased from Selleckchem (Suffolk, UK) and were reconstituted using phosphate buffered saline (PBS) and dimethyl sulfoxide (DMSO), respectively. Drugs were then diluted in culture medium, maximum DMSO concentration was 0.2 % (v/v). Unless otherwise stated, all other cell culture reagents were purchased from Life Technologies (Paisley, UK) and all chemicals were purchased from Sigma-Aldrich (Poole, UK).

Human neuroblastoma SK-N-BE(2c) cells were purchased from the American Type Culture Collection. SK-N-BE(2c) cells were maintained in high glucose Dulbecco’s Modified Eagle Medium (DMEM) containing 15 % (v/v) foetal calf serum, 2 mM L-glutamine and 1 % (v/v) non-essential amino acids. Human glioblastoma UVW cells [38] were transfected with a plasmid containing the bovine noradrenaline transporter (NAT) gene [39]. UVW/NAT cells were maintained in Minimum Essential Medium (MEM) containing 10 % (v/v) foetal calf serum, 2 mM L-glutamine, 1 % (v/v) non-essential amino acids and 1 mg/ml geneticin. Cells were incubated at 37 °C, 5 % CO₂ in a humidified incubator, and were passaged every 3-4 days. Cell lines were cultured in this study for less than 6 months after resuscitation.

Monolayers were cultured at a density of 10⁵ cells in 25 cm² flasks. Cells in the exponential growth phase were treated with fresh culture medium containing rucaparib or olaparib and were simultaneously irradiated using an Xstrahl RS225 X-Ray irradiator (Xstrahl Limited, Surrey, UK) at a dose rate of 0.93 Gy/min. After 24 h incubation at 37 °C, cells were seeded in 21.5 cm² petri dishes at a density of 500 (SK-N-BE(2c)) or 250 (UVW/NAT) cells per dish in triplicate. After 8 days (UVW/NAT) or 14 days (SK-N-BE(2c)), colonies containing ≥50 cells were fixed with 50 % (v/v) methanol in PBS and stained with crystal violet. Stained colonies were counted and expressed as a fraction of the untreated, unirradiated control. Radiation survival curves were fitted assuming a linear-quadratic relationship between survival and radiation dose using GraphPad Prism 5.01 (GraphPad Software, San Diego, USA). The data were used to calculate the dose required to sterilise 50 % of clonogens (IC₅₀), as well as the dose-enhancement factor at IC₅₀ (DEF₅₀).

Cells were seeded at a density of 1x10⁵ (SK-N-BE(2c)) or 0.5x10⁵ (UVW/NAT) cells on to glass coverslips in 6-well plates. After 48 h, fresh medium was added containing rucaparib or olaparib, before incubating for 1.5 h at 37 °C. PARP-1 activity was stimulated by treatment with 20 mM hydrogen peroxide for 20 min at room temperature in the dark. PBS or DMSO treatment of 0.09 % (v/v) in medium constituted negative controls. Cells were fixed with ice cold methanol/acetone (1:1) on ice for 15 min, before blocking with 2 % (w/v) bovine serum albumin (BSA) in PBS for 30 min at room temperature. Fixed cells were incubated for 1 h at room temperature with a 1:200 dilution of mouse anti-PADPR monoclonal antibody (Abcam, Cambridge, UK; Cat# ab14459) in antibody buffer (10 mM Tris–HCl pH 7.5, 150 mM NaCl, 0.1 % (w/v) BSA in distilled water). Bound anti-PADPR primary antibody was visualised after 1 h incubation at room temperature using goat anti-mouse Alexa Fluor 488-conjugated secondary antibody (Life Technologies, Paisley, UK; Cat# A11029), at a dilution of 1:500 in antibody buffer. Cells were fixed by treatment with 4 % (w/v) paraformaldehyde for 30 min at room temperature in the dark, before mounting on to microscope slides using Vectashield mounting medium containing DAPI nuclear stain (Vector Laboratories, Peterborough, UK). Fluorescence was visualised by means of a Zeiss Axio Observer LSM 780 confocal microscope, using identical laser power and gain settings for all images.

No-carrier-added (n.c.a.) ¹³¹I-MIBG was prepared using a solid phase system wherein the precursor of ¹³¹I-MIBG was attached to an insoluble polymer via the tin-aryl bond [40, 41]. The reaction conditions, HPLC purification procedure, and radiochemical yield were as described previously [42]. Cells were treated with ¹³¹I-MIBG for 2 h, by which time ¹³¹I-MIBG uptake was maximal [43].

Cells were seeded at a density of 7x10⁵ (SK-N-BE(2c)) or 4x10⁵ (UVW/NAT) cells into 75 cm² flasks. After 48 h, fresh medium was added containing rucaparib or olaparib and cells were simultaneously irradiated before incubating for 1.5 h at 37 °C. Cells were trypsinised and washed with PBS, before fixing with 70 % (v/v) ethanol in water at -20 °C. Ethanol was removed by washing with PBS. Cells were permeabilised by treatment with 0.05 % (v/v) Triton X-100 in PBS containing a 1:50 dilution of rabbit anti-phospho-Histone H2AX(Ser139)-Alexa Fluor 647-conjugated monoclonal antibody. After 40 min incubation at room temperature, excess antibody was removed by washing with PBST buffer (0.1 % (v/v) Tween 20 in PBS). Finally, cell pellets were resuspended in PBS containing propidium iodide (10 μg/ml) and RNase A (200 μg/ml), before analysis using a BD FACSVerse flow cytometer (BD BioSciences, Oxford, UK). FACS data were quantified using FlowJo 7.6.5 software. For cell cycle analysis, cells were treated separately, and were incubated with propidium iodide and RNase A only as detailed above.

Cells were seeded as for PARP-1 activity assay. Fresh medium was added containing rucaparib or olaparib, and cells were simultaneously irradiated, before incubating for 1.5 h at 37 °C. After treatment, cells were fixed with 4 % (w/v) paraformaldehyde for 30 min at room temperature before blocking with 2 % (w/v) BSA (in PBS) for 30 min at room temperature. Fixed cells were then incubated overnight at 4 °C with a 1:50 dilution of rabbit anti-phospho-Histone H2AX(Ser139)-Alexa Fluor 647-conjugated monoclonal antibody (Cell Signalling Technology, supplied by New England Biolabs, Hitchin, UK, Cat# 9720), followed by overnight incubation with a 1:250 dilution of mouse anti-β-tubulin (Life Technologies, Paisley, UK) in antibody buffer (10 mM Tris–HCl pH 7.5, 150 mM NaCl, 0.1 % (w/v) BSA in distilled water). Bound anti-β-tubulin primary antibody was visualised after 1 h incubation at room temperature using goat anti-mouse Alexa Fluor 488-conjugated secondary antibody (Life Technologies, Paisley, UK; Cat# A11029), at a dilution of 1:500 in antibody buffer. Cells were mounted and fluorescence visualised as for PARP-1 activity assay.

All statistical analyses were performed using GraphPad Prism version 5.01 (GraphPad Software, California, USA). The number of experimental repeats is provided in figure legends. Data are presented as means ± standard error of the mean (SEM). Statistical significance was determined by either the unpaired Student’s two-tailed t test, or the one-way ANOVA followed by post-hoc testing using Bonferroni correction for multiple comparisons. A probability (p) value < 0.05 was considered statistically significant and < 0.01 highly significant.

Neither rucaparib nor olaparib was cytotoxic at 1 μM. Minor yet significant clonogenic cell kill was induced by both drugs at 10 μM. Rucaparib at 30 μM was significantly toxic to SK-N-BE(2c) and UVW/NAT cells (Fig. 1a; p < 0.01). Neither cell line survived 24 h treatment with 50 μM rucaparib. In contrast, 30 μM olaparib, though highly toxic to UVW/NAT cells (p < 0.01), induced modest kill of SK-N-BE(2c) clonogens (Fig. 1b; p < 0.5).

Incubation with 10 μM rucaparib or olaparib (termed drug alone in Fig. 2) induced a 50 % reduction in endogenous PARP-1 activity compared with cells which were treated only with the drug vehicle. In contrast, PARP-1 activity was significantly enhanced by treatment with the DNA damaging agent hydrogen peroxide (H₂O₂) at 20 mM – labelled no drug on Fig. 2. This was demonstrated by a 3.5-fold (p < 0.01) and 9.4-fold (p < 0.01) increase in PARP-1 activity compared to untreated SK-N-BE(2c) (Fig. 2b) and UVW/NAT cells (Fig. 2c), respectively. However, the H₂O₂-induced increase in PARP-1 activity was reduced to levels comparable with untreated cells after treatment with 1 μM or 10 μM rucaparib or olaparib in both cell lines (p < 0.01).

To investigate the radiosensitising potential of rucaparib and olaparib in SK-N-BE(2c) and UVW/NAT cells, clonogenic survival was assessed following drug treatment in simultaneous combination with external beam X-irradiation or treatment with the NAT-targeting radiopharmaceutical ¹³¹I-MIBG. In combination treatments, PARP-1 inhibitors were administered at non-cytotoxic (1 μM) or cytotoxic (10 μM and 30 μM) concentrations, all of which inhibited PARP-1 activity in both cell lines.

Rucaparib and olaparib sensitised SK-N-BE(2c) cells (Fig. 3a and b) and UVW/NAT cells (Fig. 3d and Fig. 3e) to X-irradiation. This was indicated by the reduced X-radiation dose required to achieve 50 % cell kill (IC₅₀). In the absence of PARP-1 inhibition, the IC₅₀ value corresponding to X-radiation treatment alone of SK-N-BE(2c) cells was 3.57 ± 0.15 Gy (Fig. 3c). This value was decreased to 3.18 ± 0.18, 1.76 ± 0.41 (p < 0.01) or 2.52 ± 0.22 Gy by treatment with 1, 10 or 30 μM rucaparib, respectively. Exposure to 1, 10 or 30 μM olaparib reduced IC₅₀ values to 3.42 ± 0.60, 3.22 ± 0.24 and 2.21 ± 0.18 Gy (p < 0.001) respectively, in SK-N-BE(2c) cells. Likewise in UVW/NAT cells, IC₅₀ values observed after exposure to X-radiation alone, or in the presence of 1, 10 or 30 μM rucaparib were 4.44 ± 0.21, 3.50 ± 0.53, 2.42 ± 0.17 (p < 0.01) and 3.44 ± 0.28 Gy, respectively (Fig. 3f). Similarly, treatment with 1, 10 or 30 μM olaparib reduced IC₅₀ values to 3.54 ± 0.14, 1.89 ± 0.09 (p < 0.001) and 2.09 ± 0.47 Gy (p < 0.01), respectively. These results suggest a plateau at 10 μM rucaparib or olaparib, with respect to clonogenic kill.

The dose enhancement factor (DEF₅₀) was calculated as the radiation dose required to achieve 50 % kill in the absence of drug divided by the radiation dose required to kill cells in the presence of drug. Therefore, a DEF₅₀ greater than 1 is indicative of radiosensitisation. Both PARP-1 inhibitors radiosensitised SK-N-BE(2c) and UVW/NAT cells. In the case of SK-N-BE(2c) cells, the DEF₅₀ values were 2.01 and 1.22 following 10 μM rucaparib and olaparib treatment, respectively (Fig. 3c). In UVW/NAT cells, the corresponding values were 1.76 and 2.27 for 10 μM rucaparib and olaparib treatment, respectively (Fig. 3f). Dose enhancement was not further increased by treatment of cells with rucaparib or olaparib at concentrations greater than 10 μM.

Rucaparib and olaparib also sensitised SK-N-BE(2c) and UVW/NAT cells to treatment with ¹³¹I-MIBG (Fig. 4). In SK-N-BE(2c) cells, the ¹³¹I-MIBG activity concentration corresponding to the IC₅₀ was reduced from 0.78 ± 0.06 MBq/ml to 0.35 ± 0.02 (p < 0.05) or 0.63 ± 0.17 MBq/ml after treatment with 10 μM rucaparib or olaparib, respectively (Fig. 4c). Similarly, in UVW/NAT cells, the corresponding IC₅₀ values were 1.58 ± 0.14 MBq/ml for ¹³¹I-MIBG treatment alone and 1.20 ± 0.22 and 0.71 ± 0.24 MBq (p < 0.05) in the presence of rucaparib or olaparib, respectively. DEF₅₀ values were calculated as 2.36 and 1.17 in SK-N-BE(2c) cells treated with 10 μM rucaparib or olaparib respectively (Fig. 4c). In UVW/NAT cells, DEF₅₀ values obtained were 1.39 and 1.91 following treatment with 10 μM rucaparib or olaparib, respectively.

The interaction between radiation treatment and PARP-1 inhibitors was further determined using X-irradiation doses (3 Gy) and activity concentrations (1 MBq/ml) that were responsible for 50 % kill of SK-N-BE(2c) clonogens. Combination treatment included rucaparib or olaparib at 10 μM. The expected clonogenic cell surviving fraction, if the two treatments had an additive effect, was calculated as the product of the surviving fractions resulting from single agent treatments. This is designated as “combination expected” in Fig. 5. The “combination observed” was the experimental surviving fraction following combination treatment.

Combined treatments produced significantly greater cell kill than single modality treatments. This was indicated by combination expected surviving fractions of 0.36 ± 0.05 or 0.38 ± 0.05 following an additive interaction between rucaparib or olaparib with X-irradiation, respectively, in SK-N-BE(2c) cells (Fig. 5a). The surviving fraction of the observed combination of rucaparib (0.17 ± 0.04; p < 0.05) or olaparib (0.20 ± 0.02; p < 0.01) with X-irradiation in SK-N-BE(2c) cells was less than that of the expected combination, indicating supra-additivity. Similarly, in UVW/NAT cells, the surviving fraction of the observed combination of rucaparib (0.25 ± 0.02) or olaparib (0.14 ± 0.02) with X-radiation was less than that of the expected combination (rucaparib: 0.45 ± 0.02; olaparib: 0.35 ± 0.05) (Fig. 5b).

Supra-additive clonogenic cell kill also resulted from combination treatments comprising PARP-1 inhibition and ¹³¹I-MIBG (Fig. 5c and d). The surviving fraction resulting from combination treatments of UVW/NAT cells (rucaparib: 0.44 ± 0.03; olaparib: 0.32 ± 0.08) was less than of the expected combination (rucaparib: 0.61 ± 0.03; olaparib: 0.50 ± 0.04) (Fig. 5d). These results indicate that combination therapy produced greater cell kill than the administration of either treatment modality alone. Moreover, the observed surviving fraction following combination therapy was less than that expected from an additive interaction. No significant difference was observed in surviving fraction between the two PARP-1 inhibitors following single agent or combination therapy.

Irradiation administered as a single agent promoted a significant increase in the G₂/M cell population 12 h after irradiation, from 19 ± 1 % in SK-N-BE(2c) cells at 0 h, to 35 ± 1 % following 3 Gy irradiation (p < 0.01; Fig. 6a). However, 24 h after irradiation, the proportion of SK-N-BE(2c) cells in G₂/M phase had decreased and was no longer significantly elevated relative to 0 h. Similarly, in UVW/NAT cells, the proportion of G₂/M cells significantly increased from 22 ± 1 % at 0 h to 40 ± 5 % (p < 0.05) and 32 ± 3 % (p < 0.05), 12 h and 24 h after 3 Gy irradiation, respectively (Fig. 6b). In contrast, exposure to a radiation dose of 10 Gy caused a significant increase in the proportion of cells in G₂/M phase at 12 h, which persisted at 24 h in both cell lines (Fig. 6a and b).

Rucaparib and olaparib single agent treatments significantly increased the G₂/M population of SK-N-BE(2c) cells, from 24 ± 3 % in unirradiated controls, to 34 ± 3 % or 33 ± 3 % after administration of 10 μM rucaparib or olaparib, respectively (p < 0.05; Fig. 6c). Although radiation alone had no significant effect on cell cycle distribution 24 h after exposure, the effect of combination treatment was assessed at this time point to reflect the time at which combination treatments were assayed for clonogenic capacity. Combination treatment significantly increased the G₂/M arrest observed with drug alone. This was indicated by an increase in the G₂/M population to 49 ± 5 % (p < 0.001) and 51 ± 5 % (p < 0.001) following rucaparib or olaparib combination treatment, respectively, in SK-N-BE(2c) cells. Rucaparib and olaparib, both as single agents and as components of combination therapy, produced a similar level of G₂/M arrest.

Similar treatment-induced, cell cycle redistribution was observed in UVW/NAT cells (Fig. 6d). Single agent rucaparib or olaparib treatment increased the G₂/M population of UVW/NAT cells from 22 ± 1 % in unirradiated controls, to 32 ± 2 % (p < 0.01) or 30 ± 3 % (p < 0.05), respectively. Combination treatment significantly increased the G₂/M population from 22 ± 1 % in unirradiated controls, to 55 ± 1 % (p < 0.001) and 61 ± 2 % (p < 0.001) following rucaparib or olaparib combination treatment, respectively. Representative histograms obtained using SK-N-BE(2c) cells are shown in Fig. 6e.

The generation of γH2AX foci at the site of DNA double strand breaks follows phosphorylation of the H2AX histone variant protein at serine residue 139 [44]. γH2AX fluorescence intensity was proportional to the magnitude of DNA damage [45], and was detected with an anti-γH2AX Alexa Fluor 647-conjugated antibody. γH2AX foci co-localised with the DNA intercalating fluorescent stain DAPI, thereby confirming the nuclear location of γH2AX (Fig. 7a).

X-radiation treatment significantly increased DNA damage 2 h after irradiation (Fig. 7b, c and d). This was indicated by an increase from 6 to 27 % (p < 0.01) and from 2 to 21 % (p < 0.01) γH2AX positivity relative to total cellular DNA for SK-N-BE(2c) and UVW/NAT cells, respectively. Twenty four hours after irradiation, these values decreased to 14 % (SK-N-BE(2c)) and 6 % (UVW/NAT), indicating DNA repair. Combination treatment, consisting of rucaparib or olaparib with X-irradiation, resulted in greater DNA damage compared with irradiation alone. Combined X-irradiation with rucaparib caused an increase in γH2AX positivity to 45 % (p < 0.001) in SK-N-BE(2c) cells 2 h after treatment and, compared with irradiation alone, the damage was more sustained as indicated by 23 % γH2AX positivity (p < 0.05) 24 h after treatment. Similarly, combination treatment of cells with X-irradiation and olaparib caused 37 % DNA damage (p < 0.01) in SK-N-BE(2c) cells 2 h after treatment, which remained unrepaired (27 % DNA damage; p < 0.001) 24 h after treatment. Therefore, combining rucaparib or olaparib with X-irradiation produced a significantly greater amount of DNA damage, compared with X-irradiation alone (p < 0.05).

Similar inhibition of DNA damage repair was observed in UVW/NAT cells (Fig. 7c). Combining X-irradiation with rucaparib produced the greatest increase in γH2AX positivity compared with either single agent modality alone, exemplified by an increase in γH2AX from 2 and 3 % in untreated cells, to 37 % (p < 0.001) and 12 % (p < 0.01) 2 h and 24 h after treatment, respectively. Likewise, olaparib in combination with X-irradiation resulted in the greatest DNA damage 2 h after treatment (36 % γH2AX positivity; p < 0.01) compared with single agent treatments, which remained unrepaired 24 h after treatment (14 % γH2AX positivity; p < 0.001). Furthermore, combination treatment produced significantly greater initial DNA damage compared with X-irradiation alone (p < 0.05). These results indicate that PARP-1 inhibition prevented the restitution of radiation-induced DNA damage.