HT29 and HCT116 cells were obtained from the laboratory of the General Surgical Department, Union Hospital, Tongji Medical College, Huazhong University of Science and Technology (Hubei, China) and maintained in RPMI-1640 medium supplemented with 10% foetal bovine serum. The cells were cultured in a humidified incubator with 5% CO₂ at 37°C. IH was provided by Zhejiang Beta Pharma Ltd. (Hangzhou, China), and dissolved in 100% dimethyl sulfoxide (DMSO) (Sigma, St. Louis, MO, USA) to a final concentration of 30 mg/ml and stored at −20°C.

A total of 0.5-1×10⁵ exponentially growing cells were seeded in 96-well micro-titre plates (Corning Inc., New York, NY, USA) and were treated with different concentrations of IH (0.01, 0.03, 0.1, 0.3 and 0.9 mg/ml) following incubation in growth medium overnight at 37°C. After 24 h of IH addition, a microculture tetrazolium (MTT) assay was performed by adding 20 μl of 3-(4,5-diethyl-2-thiazolyl)-2,5-diphenyltetrazolium bromide (5 mg/ml) (Sigma) to each well for 4 h at 37°C to allow metabolically active cells to generate formazan crystals from MTT. The medium was aspirated and 150 μl of DMSO (Sigma) was added to dissolve the formazan. After 10 min, the above mixture was measured in a microplate reader (Bio-Tek, Winooski, VT, USA) at a wavelength of 490 nm. The percentage inhibition rate was calculated as: (1 - OD value of experimental group/control group OD) ×100%. The IC₂₀ was selected as the subsequent experiment concentration.

HCT116 and HT29 cells were collected from exponential phase cultures by trypsinisation, counted, and then seeded in 6-well plates (Corning Inc.) with densities varying from 1×10² to 5×10³ cells/well depending on the intended radiation dose. According to the MTT assay, the IC₂₀ was selected for subsequent experiments. IH (0.03 and 0.06 mg/ml for HCT116 and HT29 cells, respectively) was added 24 h prior to radiation exposure with single doses ranging from 0 to 10 Gy. Irradiation treatments in this study were performed on a clinically calibrated Siemens Oncor accelerator using 6 MV photons at a nominal dose rate of 3 Gy/min (Siemens Medical Solutions, Concord, CA, USA). After 24 h, the medium containing IH or DMSO was substituted with medium that only contained 10% foetal bovine serum. After 10–14 days, the cells were fixed with methanol (Guge, Wuhan, China) and stained with 10% crystal violet (Guge). The colonies were counted, and a grouping of >50 cells was considered a colony. The plating efficiency (PE) was the percentage of cells seeded that grew into colonies under special culture conditions. The survival fraction, expressed as a function of the radiation dose, was calculated as: Survival fraction = colonies counted/(cells seeded × PE/100). Experiments were repeated three times.

After 24 h of seeding, the cells were exposed to IH (0.06 and 0.03 mg/ml for HT29 and HCT116 cells) for 24 h, radiotherapy (10 Gy) for 24 h, or the combination treatment. The trypsinised cells were re-suspended in 1X binding buffer at a concentration of 2×10⁵ cells/ml, and Annexin V-FITC and propidium iodide (PI) (Sigma) were added. The cells were incubated for an additional 15 min at room temperature in the dark and then subjected to analysis with flow cytometry (BD Biosciences, San Jose, CA, USA). A minimum of 10,000 cells in each sample were analysed, and the data were analysed using the Cell Quest software (BD Biosciences).

Cells were collected after 24 h of exposure to IH, 10 Gy radiation, or the combination treatment. The cells were washed with PBS (Boster, Wuhan, China) and harvested by trypsinisation. After centrifugation at ? for ?, the cell pellets were fixed in 70% cold ethanol. Following removal of the ethanol by centrifugation, the cells were stained with a DNA staining solution (20 μg/ml of propidium iodide and 10 μg/ml of RNase A) for 30 min. The stained cells were then suspended and immediately subjected to analysis using a flow cytometer (BD Biosciences). The resulting DNA distribution was analysed by ModFit for the proportion of cells in the sub-G0, G1, S, and G2-M phases of the cell cycle. A minimum of 10,000 cells was counted in each sample, and the cell cycle distribution was calculated using the Cell Quest software (BD Biosciences).

Cells (2×10⁵) were plated in chamber slides. IH was added following cell adhesion, resulting in a final concentration of 0.06 and 0.03 mg/ml for HT29 and HCT116 cells, respectively. After 24 h, the cells were treated with radiation. After another 24 h, the medium was aspirated and the cells were fixed with 4% paraformaldehyde. The cells were rinsed with PBS three times and permeabilised with 0.2% Triton-X-100 (Boster) for 20 min at 4°C. The cells were rinsed with PBS three times again and blocked with 5% BSA for 1 h at room temperature. The cells were again washed with PBS three times and anti-γ-H2AX antibody (1:200, Abcam, Cambridge, MA, USA) and anti-53BP1 antibody (1:200, Bethyl, Inc., Montgomery, TX, USA) were added at a dilution of 1:800 and 1:200 in 1% BSA, respectively. Subsequently, the slides were incubated overnight at 4°C. The cells were rinsed with PBS prior to incubation with cyanine 3 (CY3)-labelled secondary antibody (Protientech Group, Chicago, IL, USA) at a dilution of 1:200 in 1% BSA for 1 h in the dark. The secondary antibody was aspirated, and the cells were rinsed with PBS three times and incubated with 4′,6-diamidino-2-phenylindole dihydrochloride (DAPI) (Vector Laboratories Inc., Burlingame, CA, USA) in the dark for 10 min. The slides were examined using a fluorescent microscope. The images were captured with a confocal laser scanning microscope (CLSM) (Olympus, Tokyo, Japan) equipped with a camera. For each sample, the γ-H2AX and 53BP1 foci were determined in ≥100 cells.

The cells were seeded and allowed to adhere in complete medium overnight. They were then treated with or without IH (0.06 and 0.03 mg/ml for HT29 and HCT116 cells) 24 h prior to irradiation with a 10 Gy dose, and the cells were lysed with a lysis buffer (Beyotime, Wuhan, China). The protein lysates were harvested and centrifuged, and the supernatants were collected. The proteins were separated via 10 or 12% sodium dodecyl sulphate (SDS)/polyacrylamide gel electrophoresis and then transferred to polyvinyl difluoride membranes (Millipore, Billerica, MA, USA). The membranes were then blocked with 5% bovine serum albumin or milk and finally incubated with γ-H2AX (Abcam), 53BP1 antibody (Bethyl, Inc.) or β-actin antibody (Santa Cruz Biotechnology, Inc., Santa Cruz, CA, USA). The membranes were incubated with the primary antibodies overnight at 4°C and rinsed with TBST three times, followed by incubation with secondary antibodies labelled with horseradish peroxidase (HRP) (Protientech Group). The bands were then visualised using enhanced chemiluminescence (ECL) (Pierce, Rockford, IL, USA).

Exponential phase HT29 and HCT116 cells were prepared at a concentration of 2×10⁷ cells/ml in serum-free RPMI medium. Female athymic nude mice (nu/nu, body weight, 20–25 g, 8–12 weeks of age) were obtained from Beijing HFK Bioscience Co., Ltd. The mice were provided with sterilised food and water and housed in a barrier facility with 12-h light/dark cycles in laminar flow hoods at a constant temperature and humidity for the entire course of the experiments and supplied with a standard laboratory diet and water. The tumour xenografts were established via the subcutaneous injection of a 0.2 ml volume of the prepared cell stock into the right hind leg. After 7 days, when the diameter of each tumour increased to 10 mm, the mice were pooled and randomly assigned to 4 groups (control, IH alone, radiation alone, and radiation in combination with IH) of 6 animals each. IH (35 mg/kg) was administered via oral gavage once a day for 5 days, and locoregional irradiation was administered in a single 2 Gy fraction once a day (6-MV linear accelerator, MDX, Siemens) for 5 days. The tumour size was measured using callipers every two days. Animal protocols and studies were conducted in accordance with the guidelines of the Institutional Animal Care and Use Committee of the Korea Institute of Radiological and Medical Sciences, Korea.

The tumour volumes (V) were determined according to the two axes of the tumour (L, longest axis; W, shortest axis). The volume was calculated according to the formula: Tumour volume (mm³) = (L × W²)/2 mm³, where L and W are the shortest and the longest diameter.

SPSS 13.0 software was used for the data analysis. The data are reported as the mean ± SEM and analysed using one-way ANOVA to compare means in multiple groups. A q-test was used for the pairwise comparison among groups. A difference was regarded as significant if P<0.05.

The effect of icotinib on cell viability was measured with the MTT assay. The inhibitory effect of icotinib positively correlates with the drug concentration (Fig. 1). The IC₅₀ (median inhibition concentration) and IC₂₀ (inhibiting concentration 20) values were obtained. The IC₂₀ value was selected as the drug concentration for subsequent experiments, with values of 0.06 and 0.03 mg/ml for HT29 and HCT116.

To determine the radiosensitising effect of icotinib on the HT29 and HCT116 colorectal cell lines, a clonogenic formation assay was performed. The result was compared to gefitinib combined with radiation, similar to icotinib. IC₂₀ values of gefitinib on HT29 and HCT116 cells were explored and applied for further study of radiosensitisation. The L-Q model was used to investigate the difference in radiosensitivity from gefitinib or IH combined with irradiation or irradiation alone. The results showed that the Dq, Do and N values were reduced in response to treatment with gefitinib or icotinib combined with irradiation when compared with irradiaton alone for HT29 and HCT116. Furthermore, icotinib exhibited a stronger ability to reduce the Dq, Do and N values compared to gefitinib. Radiotherapy alone decreased the SF2 values of HT29 and HCT116 to 76 and 66%, whereas when gefitinib was added, the SF2 values decreased to 64 and 51%, respectively. Addition of icotinib resulted in the reduction of SF2 values to 44 and 39%, respectively, suggesting that icotinib more effectively sensitises colorectal cancer cells to radiation as compared to gefitinib (Table I, Fig. 2).

To determine whether icotinib combined with radiotherapy increased apoptosis, HT29 or HCT116 cells were treated with vehicle or IH with or without radiotherapy [control; IH alone; radiotherapy (RT) alone; IH+RT], and the cell apoptotic rate was then detected via flow cytometry 24 h after the treatment (Fig. 3). In HT29 cells, the apoptotic rate of the combined group was 26.97±7.15%, while it was 14.17±5.44% in the monotherapy group, 15.81±3.31% in the RT group and 12.5±2.93% in the control group. Significant differences were observed between the combined group and the remaining three groups (P<0.01). For HCT116 cells in the control group, the apoptotic rate was 10.08±0.62%, while it was 12.21±2.71% in the IH alone group, 18.45±3.45% in the RT group and 28.72±4.73% in the combined group. Compared with the remaining three groups, the apoptotic rate of the combined group was significantly increased (P<0.05).

The influence of icotinib in combination with or without radiotherapy on the HT29 and HCT116 cell cycle was detected via flow cytometry (Fig. 4). In HT29 cells, the G2/M phase of the single drug group was 10.45±0.89%, while it was 21.50±1.99% in the RT alone group and 35.79±1.10% in the combined group. The percentage of cells in the G2/M phase in the combined group was higher than that of the single drug or RT alone group (P<0.05). For HCT116 cells, the G2/M phase of the single drug group was 12.77±2.03%, while that of the RT alone group was 68.53±2.49% and that of the combined group was 74.00±1.33%. The combined group showed significantly longer arrest in the G2/M phase compared with the single drug group and a tendency to stagnate in the G2/M phase compared with the RT group, although without significant differences (P>0.05). Icotinib combined with RT treatment re-adjusted the cell cycle distribution, significantly increased sensitive cells and improved the effect of radiotherapy.

The present results showed that, H2AX was rapidly phosphorylated in the presence of DSB and aggregated at the DSB, making it an important symbol of DNA DSB, as well as an important method to detect DNA DSB repairability. Twenty-four hours after the various treatments, the γ-H2AX foci per cell were detected (Fig. 5). The results showed that the combination groups showed a significantly higher number of unrepaired double-stranded DNA in the HT29 and HCT116 cell lines, while the RT alone or combined treatment with icotinib group showed significant differences as compared to the combined group (P<0.01). In the drug-RT combination group, the number of γ-H2AX foci was significantly higher than that in the RT alone group.

53BP1 has been proven to participate in double-stranded DNA repair, and is an important early regulator of DNA damage. To further determine whether 53BP1 is involved in double-stranded DNA repair during tumour suppression, the present study detected 53BP1 expression in HCT116 and HT29 cells treated in different groups (Fig. 6). Similar to γ-H2AX expression in different treatment groups, 53BP1 exhibited the same trends in the two differently treated cell lines. Tumour cells in the icotinib-RT combined group showed high levels of 53BP1 foci/cell that significantly differed from the RT, single drug and control groups. 53BP1 expression was significantly increased in the icotinib-RT combined group compared to the RT alone group and drug treatment group (P<0.01). The results are in concordance with the γ-H2AX data presented for each group, suggesting that 53BP1 and γ-H2AX are involved in DNA double-strand repair and are involved in the tumour response to treatment and radiosensitisation.

To determine the factors that contribute to impaired DSB repair, the responses of the 53BP1 and γ-H2AX proteins, which play key roles in DSB repair, were determined. Western blots were used to detect the expression of γ-H2AX and 53BP1 protein in human colorectal cancer cells following interference in the different groups. As shown in Fig. 7, icotinib-RT combined treatment significantly increased the expression levels of γ-H2AX and 53BP1 proteins, suggesting that the combined treatment increased the DNA double-strand breaks, attenuated DNA repair and improved the effect of radiotherapy.

IH was shown to significantly inhibit HT29 and HCT116 cell xenograft growth (Fig. 8). The final tumour volume of the combination group was statistically significantly smaller than that of the other groups (P<0.05) in both the HCT116 and HT29 models. This finding indicates that icotinib in combination with radiotherapy significantly inhibited the growth of colorectal cancer tumours.