All participants provided written informed consent, and this research protocol was approved by the Saga University Institutional Review Board (2018-01-R-04). All normal and cancerous colorectal tissue samples were obtained during surgery according to the guidelines of the Human Tissue Research Committee at our hospital.

Between January 2003 and December 2011, 102 pairs of cancerous and normal tissue samples were collected from consecutively recruited patients who underwent curative surgery for pathologically confirmed stage II or III primary CRC at Saga University Hospital in Japan. All patients (stage II, n=56; stage III, n=46) were registered in our prospectively maintained comprehensive database, which contained their medical records including surgical outcomes. Specimens from cancerous and normal regions in the resected tissues were immediately frozen using liquid nitrogen and stored at −80°C until use. Thirty-one patients with a good performance status received adjuvant chemotherapy following surgery due to the presence of lymph node metastasis or lymphatic invasion.

Before extracting DNA, we homogenised tissue specimens on ice. DNA was extracted from the homogenates using a DNA Extractor^® TIS Kit (Wako Pure Chemical Industries, Ltd., Osaka, Japan). Obtained DNA was digested into mononucleosides via treatment with nuclease P1 followed by alkaline phosphatase using an 8-OHdG Assay Preparation Reagent Set (Wako Pure Chemical Industries, Ltd.). 8-OHdG levels were assessed in tissues using a commercially available highly sensitive ELISA kit for 8-OHdG (cat. no. KOG-HS10/E; Japan Institute for the Control of Aging, Fukuroi, Shizuoka, Japan) according to the manufacturer's instructions. In brief, 96-well plates were pre-coated with the 8-OHdG antigen. Both a DNA solution and monoclonal antibody against 8-OHdG were added to 96-well plates, which were incubated at 4°C overnight. During this step, the monoclonal antibody reacted competitively with 8-OHdG in sample solutions and 8-OHdG bound to the plate. After washing the plate with PBS, an enzyme-labelled secondary antibody was added, followed by incubation at room temperature for 1 h. Next, unbound enzyme-labelled secondary antibody was removed by washing the plate. Finally, the plate was incubated with 100 µl of the reaction-terminating solution for 15 min in the dark, and colour development was measured on a plate reader at 450 nm.

For IHC, paraffin blocks (20 mm × 30 mm) were first sectioned on slides at a thickness of 4 µm. Sections were incubated at 37 and 54°C for 24 h and 30 min, respectively. Next, to remove the paraffin, slides were soaked in xylene and then rehydrated in a graded alcohol series. For antigen retrieval, the tissue sections were heated in EDTA (pH 9.0) using a microwave for 60 min. Then, IHC was performed automatically using an Autostainer Plus^® (Dako; Agilent Technologies, Inc., Santa Clara, CA, USA). Antibodies against 8-OHdG (dilution 1:200; cat. no. sc-66036; mouse monoclonal; Santa Cruz Biotechnology, Inc., Dallas, TX, USA) and the EnVision+^® System (ready-to-use; Code K5007; Dako; Agilent Technologies, Inc.) were used as the primary and secondary antibodies, respectively. The slides were visualised using 3,3′-diaminobenzidine tetrahydrochloride and nuclei were counterstained with hematoxylin.

Immunostained tissue slides were digitised using a NanoZoomer 2.0HT digital slide scanner (Hamamatsu Photonics, Hamamatsu, Japan), and resulting whole-slide digital images in NDPI files were visualised using NDP.view2 software (Hamamatsu Photonics). NDPI files were converted to JPEG files using NDP.view2 software for the imaging analysis.

The proportion of positive 8-OHdG staining was estimated in the whole field of the slide by the pathologist. Furthermore, the intensity of cytoplasmic 8-OHdG staining was assessed using the average marker intensity, which was automatically calculated by the imaging analysis software (Tissue Studio^®4.0; Definiens, München, Germany). Finally, the 8-OHdG value was calculated using the following calculation formula: Percentage of positive 8 - OHdG expression (%) × average marker intensity.

Categorical variables are presented as numbers. The biomarkers for each background categorical variable are expressed as the median [interquartile range (IQR)], and Wilcoxon's signed-rank tests were used to compare biomarkers and background categorical variables. A Cox proportional hazards model was used in the univariate and multivariate analyses of disease-free survival (DFS) and disease-specific survival (DSS). Time-dependent receiver-operating characteristic (ROC) curves with Youden indices were used to identify the optimal cut-off values of 8-OHdG ratios (for both ELISA and qIHC), distinguishing the high- and low-risk groups with respect to the recurrence event. Kaplan-Meier curves of patients with high or low 8-OHdG ratios were plotted, and log-rank tests were conducted. All tests were two-tailed, and P<0.05 was considered to indicate a statistically significant difference. All analyses were conducted using R Statistical Software (version 3.3.3; R Foundation for Statistical Computing, Vienna, Austria) and JMP Pro version 13 (SAS Institute, Inc., Cary, NC, USA).

The CONSORT flow diagram detailing the selection of patients is presented in Fig. 1. Five patients were deemed ineligible because adequate amounts of DNA for ELISA could not be extracted (n=3) or the 8-OHdG ratio for qIHC could not be calculated (n=2).

First, we quantitatively assessed 8-OHdG in CRC tissue DNA using ELISA and examined 8-OHdG expression in CRC tissues via qIHC. According to ELISA, the median 8-OHdG level in normal tissue DNA was 1.176 (IQR=0.864–1.527) ng/ml, compared with 1.124 (IQR=0.792–1.577) ng/ml in cancer tissue, with no significant difference identified (Fig. 2A). In IHC analysis, positive 8-OHdG staining was observed in the cytoplasm, but not in the nucleus. Fig. 2B shows examples of normal (Fig. 2B-a) and cancer tissue specimens (Fig. 2B-b, and -c) assessed via qIHC. The 8-OHdG value in normal samples was estimated at 0.398 (Fig. 2B-a). The value in one CRC sample with strongly positive 8-OHdG staining was estimated at 0.873 (Fig. 2B-b), whereas another CRC sample with weakly positive expression had a value of 0.131 (Fig. 2B-c). Fig. 2C shows that the median 8-OHdG values in normal and CRC tissues were 0.280 (IQR=0.156–0.351) and 0.263 (IQR=0.116–0.412), respectively, with no significant difference observed.

To eliminate the individual backgrounds of the 97 patients, we next determined 8-OHdG ratios (8-OHdG level in cancerous tissue/8-OHdG level in normal tissue) using both ELISA and qIHC. Table I reveals the relationship between the clinicopathological characteristics and the 8-OHdG ratios in DNA. No significant differences in the 8-OHdG ratio in DNA were noted in terms of age (<75 years vs. ≥75 years), sex (male vs. female), tumor depth (T4 vs. ≤T3) or venous invasion. However, significant differences in the ratio were observed according to lymph node metastasis, lymphatic invasion and the use of postoperative adjuvant chemotherapy. Conversely, no clinicopathological factor was associated with a difference in the 8-OHdG ratio in the cytoplasm (Table I). In addition, we performed correlation analysis between the 8-OHdG ratio in DNA and the 8-OHdG ratio in the cytoplasm. The results revealed a negative linear correlation between the two 8-OHdG ratios; however, the coefficient was small (r=−0.229, P=0.024) (data not shown).

During the observation period, 22 patients experienced CRC recurrence, which was fatal in 11 patients. We conducted analyses of DFS and DSS in the 97 enrolled patients using a Cox proportional hazard model (Tables II and III). Univariate analysis demonstrated that DFS was significantly correlated with the 8-OHdG ratio in DNA [hazard ratio (HR)=5.15; 95% confidence interval (CI)=2.59–10.23; P=0.0001], the 8-OHdG ratio in the cytoplasm (HR=0.34; 95% CI=0.15–0.77; P=0.0094), lymph node metastasis (HR=2.42; 95% CI=1.02–5.77; P=0.0461), lymphatic invasion (HR=3.28; 95% CI, 1.21–8.89; P=0.0197) and the receipt of postoperative adjuvant chemotherapy (HR=2.32; 95% CI, 1.01–5.36; P=0.0484) (Table II). Additionally, the 8-OHdG ratio in DNA was significantly correlated with DSS (HR=8.14; 95% CI, 3.51–18.90; P<0.0001) (Table III). According to multivariate analyses, the 8-OHdG ratio in DNA (HR=6.48; 95% CI, 2.61–16.09; P=0.0001), the 8-OHdG ratio in the cytoplasm (HR=0.14; 95% CI, 0.04–0.51; P=0.0031) and sex (HR=0.30; 95% CI, 0.09–0.96; P=0.0425) were independently correlated with DFS (Table II). Furthermore, the 8-OHdG ratio in both DNA (HR=10.74; 95% CI, 3.54–32.6; P<0.0001) and the cytoplasm (HR=0.17; 95% CI, 0.04–0.83; P=0.0285) were independently correlated with DSS (Table III).

Time-dependent ROC curve analysis was conducted to determine the most informative cut-off point of the 8-OHdG ratio in both DNA and the cytoplasm for predicting CRC recurrence. Fig. 3 reveals the estimated ROC curve with respect to the 5-year DFS. The ROC curve analysis indicated that the optimal cut-off 8-OHdG ratio in DNA, as determined using the Youden index, was 1.087 (sensitivity=58.8%; specificity=76.2%). The optimal cut-off value for the 8-OHdG ratio in the cytoplasm was 0.999 (sensitivity=85.3%; specificity=58.7%) (Fig. 3).

Based on ROC analyses, the impact of the 8-OHdG ratio in DNA or the cytoplasm on DFS and DSS was further analysed using Kaplan-Meier curves (Fig. 4). DFS and DSS were significantly poorer in the high 8-OHdG ratio in DNA group than in the low ratio group (Fig. 4A; P=0.0043 for DFS, P=0.0044 for DSS). By contrast, DFS was significantly poorer in the low 8-OHdG ratio in the cytoplasm group than in the high ratio group, whereas DSS was not significantly different between these groups (Fig. 4B; P=0.0006 for DFS, P=0.0520 for DSS). Furthermore, we divided the patients into three groups as follows. Group I included patients with an 8-OHdG ratio in DNA ≥1.087 and an 8-OHdG ratio in the cytoplasm <0.999 [n=33 (34.0%)]. Group II included patients with an 8-OHdG ratio in DNA <1.087 and an 8-OHdG ratio in the cytoplasm ≥0.999 [n=19 (19.6%)]. Group III included patients with an 8-OHdG ratio in DNA ≥1.087 and an 8-OHdG ratio in the cytoplasm ≥0.999, or an 8-OHdG ratio in DNA <1.087 and an 8-OHdG ratio in the cytoplasm <0.999 [n=45 (46.4%)]. Fig. 5 demonstrated that the DFS and DSS were markedly lower in group I than in the other groups (P<0.0001 for DFS, P=0.0007 for DSS). Finally, Table IV presents the comparative analysis of the hazard ratios for recurrence or death among groups I–III. Group I had an increased risk of recurrence or death compared with the findings in the other groups (Table IV).