The proliferation marker Ki67, but not neuroendocrine expression, is an independent factor in the prediction of prognosis of primary prostate cancer patients

Detailed histopathological and clinical data were retrospectively collected for 166 patients, who were diagnosed with primary prostate cancer in a single institution of the North-eastern Italy from January 1992 to December 1994, therefore associated to a long follow-up period. Inclusion criteria for this study were: a) diagnosis of prostate cancer and b) availability of formalin-fixed and paraffin-embedded tissues for immunohistochemical staining and molecular analyses. Only TURP (N = 122, 73.9%) and prostatectomy (N = 43, 26.1%) specimens were used (missing information for one patient). Fine needle biopsies were excluded because of the low amount of tissue. Patients did not receive any treatment before diagnosis. The use of formalin-fixed and paraffin-embedded prostate cancer tissues and their related clinical information were approved by the Ethical Committee of the University of Trieste (Report 23; 5.10.2009) before the beginning of the study.

Representative multiple areas of the primary tumours were selected by two pathologists (G.S. and R.B.) for TMA construction. Tissue cores were chosen at the border of the primary tumour. Tissue cylinders of 1.0 mm in diameter were taken from the selected regions of the donor’s paraffin block and were placed into a recipient paraffin block using a tissue-arrayer (Galileo TMA CK3500; Integrated Systems Engineering, Milano, Italy), as previously described.²⁸ Multiple cores were taken for cases as representative of heterogeneous histological areas. Neuroendocrine differentiation (NED) was evaluated using NSE, ChrA, Syp as neuroendocrine markers.

Immunostainings for Ki67 (clone MIB-1; DakoDenmark A/S, Glostrup, Denmark), 1:200 dilution; NSE (clone E27; NeoMarker; ThermoScientific, Waltham, MA, USA) 1:2500; ChrA (clone LK2H10; NeoMarker; ThermoScientific, Waltham, MA, USA), 1:500; Syp (clone SY 38; Thermo-Fisher; ThermoScientific, Waltham, MA, USA) 1:75 were performed in a Lab Vision Autostainer 480S (Thermo Scientific, Waltham, MA, USA) with the UltraVision LP Large Volume Detection System HRP Polymer (Lab Vision Corporation, Thermo Scientific) according to manufacturer’s recommended protocol. For evaluation of the immunostaining, positively stained cells were counted across 3 high-power fields. Staining intensity was not taken into consideration. Due to technical issues related to the detachment of tissue cores it was not possible to analyze the four biomarkers in all samples (Figure 1). The percentage of the positively stained cells was reported for each specimen. Ki67 expression was dichotomized for assessing its prognostic value using a cut-off of 10%.⁷,²⁹

Figure 1

The Kaplan-Meier method was used to generate overall survival (OS) curves, which was defined as the time between the date of diagnosis and the date of death or the last follow-up (FU) observation. Patients were censored if they were still alive or they were lost to FU. The log-rank test was used to evaluate differences between groups. Association of OS with each prognostic factor was evaluate in univariate and multivariate analyses by using the Cox proportional hazards model. All variables associated with univariate value of p ≤ 0.05 were included in the multivariate model using a stepwise method. The proportional hazards assumptions were checked before applying the Cox regression model. The goodness of fit was assessed using a likelihood-ratio test. The discrimination ability was quantified by calculating the concordance index that ranges from 0.5 (no discrimination) to 1 (perfect discrimination). Possible correlations of the expression of Ki67 and neuroendocrine markers with the other prognostic variables were assessed by χ² test or Wilcoxon rank sum. All statistical tests were performed using STATA software (StataCorp. 2011. Stata Statistical Software: Release 12. College Station, TX: StataCorp LP) and p values ≤; 0.05 were considered as statistically significant.

NSE expression was assessable in 89 prostate cancer cases. Of those, 28 cases (31.5%) were completely negative, whereas 61 (68.5%) revealed a cytoplasmic positivity, referring to diffuse, focal and spotty staining (Table 1). Detachment of tissue cores did not allow analyzing NSE in some cases. ChrA was negative in 49 out of 121 cores (40.5%) and it was positive on the cytoplasmic level in 72 cores (59.5%). Positive cases had weakly to highly diffused, or focal or spotty reactivity (Table 1). Syp was analyzed in 127 cases of which 44 (34.6%) were negative and 83 (65.4%) showed a cytoplasmic positivity, from spotty to focal to diffused (Table 1). Only diffused expression was considered as positive for each marker. Focal or spotty stainings were evaluated as negative.

No significant associations were found between neuroendocrine markers and clinicopathological variables. A slight association was revealed between NSE expression and Gleason score (p = 0.04). Moreover, a positive relationship was found between CgA and SYP expression (p = 0.01). The type of intervention was significantly associated with CgA (p = 0.009) and NSE (p = 0.001) expression.

Ki67 staining analysis was measured in 146 out of 166 prostatic cases. The median Ki67 staining score was 5% with an IQR of 9 whereas the mean value was 10.3% with a standard deviation of 14.2% (range of 0 – 90%). The percentage of the positively stained cells was recorded for each sample (Table 2, Figures 2,3).

Figure 2

Figure 3

Ki67 was scored and stratified into two groups (low ≤ 10%; high > 10%) as already reported.²³,²⁴ No statistically significant difference was observed for Ki67 staining between TURP and prostatectomy specimens (p = 0.08). Ki67 expression was significantly associated with Gleason score and nuclear grading, but not with age at diagnosis or with neuroendocrine markers (Table 3).

In univariate analysis, diffuse expression of NSE, Ki67 expression > 10%, Gleason score ≥ 7 and nuclear grading ≥ 2 predicted for shorter OS (Table 4).

Considering neuroendocrine markers, only NSE staining was significantly associated with OS. Patients with diffuse NSE expression had a reduced survival time (median OS 2 years; 95% CI, 2–4) compared to patients with negative expression (median OS 7; 95% CI, 5–10; p = 0.004), showing nearly double-fold increased risk of death (Table 4, Figure 4). Additionally, NED measured as positive at least at one of the three markers did not result significant.

Figure 4

Kaplan-Meier survival curves showed a significant difference (p < 0.001) between low and high levels of Ki67 staining with median survival time of 6 years (95% CI, 5–9) and 2 years (95% CI, 1–2) for patients with ≤; 10% and > 10% of positive cells, respectively (Figure 5A). Moreover, splitting group four categories according to Ki67 staining were obtained: negative, 1–10%, 11–20%, > 20%. Negative patients showed a median overall survival (10 years, 95% CI: 4–9) which was four years longer than in patients with Ki67 staining of 1–10% (6 years, 95% CI: 5–8; p < 0.001) (Figure 5B). An improved discrimination was also reached in the category > 10%. Patients with Ki67 staining > 20% were associated with a 2.5-fold increased risk of death, compared with patients showing Ki67 expression of 10–20% (the overall 2-year survival rate of 50%–95% CI: 25–70 vs 20%, 95% CI: 6–39, p < 0.001). These data further support the potential role of Ki67 immunostaining in selecting patients according to proliferation rate, and thus to tumor aggressiveness. However, we decided to assess the prognostic value of Ki67 for overall survival of prostate cancer patients by using the previous binary variable because of harmonization with already published studies.⁷,²⁹

Figure 5

Age at diagnosis and type of intervention significantly impacted on OS (p < 0.001). Thus, considering the relationship existing with other variables, they were included in multivariate analysis to take into account their possible confounding effect.

Multivariate analysis was done by stratifying according to type of intervention, because of no proportional risks between TURP and prostatectomy groups (Test of proportional-hazards assumption, χ² = 8.86, df = 1, p = 0.003). Ki67 expression, but not NSE, resulted as an independent prognostic factor for OS. In the final multivariable model the risk of death was higher for older patients (p = 0.001) with a nuclear grading of 3 (p = 0.04), a Gleason score ≥ 7 (p < 0.001) and Ki67 expression > 10% (p < 0.001) (Table 5). Unfortunately, our dataset did not include information on PSA before surgical intervention for all patients, because they were diagnosed many years ago before the routinely application of PSA screening.

Comparison of the multivariate model incorporating Ki67 expression with a base model including conventional variables only (nuclear grading, Gleason score, age at diagnosis stratified by type of intervention) showed an improved fit which suggested an enhanced prognostic ability over the models containing clinicopathological variables only (χ² = 11.33, df = 1, p = 0.0006). These data indicated that in a multivariate analysis Ki67 is a relevant and independent prognostic factor for OS of primary prostate cancer patients undergoing TURP or radical prostatectomy. The concordance index (0.72) revealed a good accuracy of the model in predicting OS.