Sixty-two HCCs and corresponding non-cancer liver tissues were obtained from patients of the Department of Hepatobiliary Surgery, Xijing Hospital of the Fourth Military Medical University (Xi’an, China), between March 2004 and September 2006. Informed consent for research use of the specimens was obtained for all cases and all study protocols were approved by the Ethics Committee for Clinical Research of the Fourth Military Medical University. None of the patients received radiotherapy or chemotherapy before routine surgery. All of the specimens were fixed in 10% buffered formalin solution and embedded in paraffin and consecutive 4-μm-thick sections were cut.

Paraffin-embedded sections were deparaffinised with xylene, rehydrated and then immersed in 3% hydrogen peroxide solution for 10 min to inhibit endogenous peroxidase activity. For antigen retrieval, slides were boiled in 0.01 mol/l sodium citrate buffer (pH 7.0) for 10 min in a microwave oven. After being blocked with 1% bovine serum albumin (BSA), the sections were incubated with mouse monoclonal anti-Bmi-1 antibody (1:50, Abcam, Hong Kong, China) at 4°C overnight. Following incubation with biotinylated secondary antibody, a streptavidin-biotin complex/horseradish-peroxidase was applied. Finally, antibody binding was visualised with 3, 3′-diaminobenzidine (DAB) and counterstained with hematoxylin. The primary antibody was replaced by PBS in negative controls. Two pathologists who were blinded to the clinical and histopathologic outcomes evaluated the results of the staining independently. The Bmi-1 expression was scored for staining intensity and extent of involved tissue. The staining intensity was scored as 0 (no staining), 1 (weakly stained), 2 (moderately stained), or 3 (strongly stained). The extent of staining was scored as 0 (<5%), 1 (5–25%), 2 (26–50%), or 3 (>50%), according to the percentage of positively stained cells. The sum of the intensity and extent scores was used as the final staining score ranging from 0 to 9. We defined Bmi-1 expression according to the final scores as follows: 0–1, negative; 2–9, positive.

Three human hepatocellular carcinoma cell lines, HepG2, SMMC-7721 and MHCC97-H and a normal hepatocyte cell line, HL-7702, were obtained from American Type Culture Collection (Manassas, VA, USA) and were maintained in DMEM medium (Gibco, Gaithersburg, MD, USA) supplemented with 10% fetal bovine serum (Invitrogen, Carlsbad, CA, USA) at 37°C in a humidified chamber with 95% air and 5% CO₂.

Lentivirus vectors for human Bmi-1 small hairpin RNA (shRNA) encoding a green fluorescent protein (GFP) and a puromycin resistance gene were constructed, packed and purified by GeneChem Corp. (Shanghai, China). Bmi-1 shRNA was designed according to the human Bmi-1 mRNA sequence (GenBank accession no. NM_005180). The shRNA target sequence was 5′-CGGAAAGTAAACAAAGACAAA-3′ and a negative control shRNA was provided by GeneChem. Cells were seeded in 24-well plates overnight before transfection for a target confluence of 30–50%. For transfection, according to the MOI value (number of lentiviruses:number of cells), the appropriate amounts of lentiviruses mixed with medium containing polybrene were added to the cells. After 24 h of transfection at 37°C, the medium was replaced by fresh DMEM medium containing 10% FBS. Three days after transfection, cells were selected with 2 μg/ml puromycin for 3 days and harvested for subsequent studies.

Total RNA was extracted with TRIzol reagent (Invitrogen) according to the manufacturer’s instructions. Total RNA (1 μg) was reverse-transcribed into cDNA using the Primescript RT reagent kit (Takara, Japan) in accordance with the manufacturer’s instructions. Bmi-1 expression levels were quantified by real-time quantitative polymerase chain reaction (PCR). Bmi-1 mRNA levels were standardised to glyceraldehyde 3-phosphate dehydrogenase (GAPDH) as a reference housekeeping gene. The forward primer for Bmi-1 was 5′-GCTTCAAGATGGCCGC TTG-3′; the reverse primer was 5′-TTCTCGTTGTTCGATGC ATTTC-3′. The forward primer for GAPDH was 5′-GCACCGT CAAGGCTGAGAAC-3′; the reverse primer was 5′-TGGTGA AGACGCCAGTGGA-3′. Quantitative real-time PCR was performed in a Bio-Rad iCycler IQ™ 5 (Bio-Rad, Hercules, CA, USA) with SYBR Master Mix (Takara) according to the manufacturer′s instructions. Each reaction was performed in a final volume of 20 μl containing 2.0 μl of appropriately diluted cDNA, 1.0 μl (10 μM) of forward and reverse primers specific for human Bmi-1 or GAPDH, 10 μl of SYBR Premix Ex Taq and 6.0 μl of water. The cycling conditions were as follows: a denaturation step at 95°C for 3 min; 40 cycles of denaturation at 95°C for 10 sec, specific annealing at 59°C for 30 sec and elongation at 72°C for 30 sec. At the end of the cycles, the temperature was raised to 95°C for 1 min. The melting curve was achieved by first cooling samples to 55°C for 1 min, followed by 81 cycles (30 sec/cycle) in which the temperature was raised by 0.5°C per cycle to a maximum temperature of 95°C.

Cells were lysed in ice-cold RIPA lysis buffer containing 50 mM Tris-HCl (pH 7.4), 1% Triton X-100, 5 mM EDTA, 1 mM leupeptin, 1 mM phenylmethylsulfonyl fluoride, 10 mM NaF and 1 mM Na₃VO₄ and then centrifuged at 20,000 g for 30 min at 4°C to remove debris. Protein concentrations were determined by a BCA assay (Pierce, Rockford, IL, USA). Equal amounts of cell lysate protein were subjected to SDS-polyacrylamide gel electrophoresis (PAGE) and transferred to polyvinyl difluoride (PVDF) membranes. Membranes were blocked with 5% non-fat dry milk in Tris-buffered saline with Tween-20 for 1 h, then incubated overnight at 4°C with specific primary antibodies. Primary antibodies against Bmi-1 were purchased from Abcam and primary antibodies against MMP-2, MMP-9, VEGF, PTEN, Akt, p-Akt and GAPDH were purchased from Santa Cruz Biotechnology (Santa Cruz, CA, USA). The membranes were next incubated with horseradish peroxidase-conjugated secondary antibodies and then developed with an enhanced chemiluminescence detection system (Amersham Life Science, Piscataway, NJ, USA) according to the manufacturer’s instructions.

Transwell cell culture chambers (8-μm pore size; Millipore, Billerica, MA, USA) were used for in vitro invasion assays. The upper side of the filter was covered with Matrigel (Collaborative Research Inc., Boston, BD, USA) (1:3 dilution with DMEM free of serum) before the assays. Cells (5×10⁵) were serum-starved for 24 h and then transferred in 350 μl serum-free DMEM to the upper chamber and DMEM with 15% fetal bovine serum was added to the lower chamber as a chemoattractant. The cells were incubated under normoxic conditions for 24 h. Cells on the upper side of the filter were removed and cells that remained adherent to the underside of the membrane were fixed in 4% formaldehyde and stained with 0.5% crystal violet for 10 min. For pharmacological inhibition assays with LY294002, cells were pre-treated for 2–4 h and the treatment continued during the invasion experiment. Finally, the number of invasive cells was counted in ten contiguous fields of each sample and the average was determined.

An enzyme-linked immunosorbent assay (ELISA) (Amersham, Buckinghamshire, UK) was used to quantify the individual activities of MMP-2, MMP-9 and VEGF. The samples were thawed on ice and all reagents were equilibrated to room temperature; assays were carried out according to the manufacturer’s instructions.

The data are expressed as the means ± SD. Correlations between clinicopathological variables and Bmi-1 expression were analysed with Pearson’s χ² tests. Survival curves were calculated using the Kaplan-Meier method and compared using the log-rank test. The Cox proportional hazard model was carried out to explore the value of clinicopathological factors and Bmi-1 expression on survival. Variance analysis between groups was performed by one-way ANOVA and the significance of differences between control and treatment groups was tested using Dunnett’s multiple comparisons test. All statistical analyses were performed using the SPSS software package (SPSS, Chicago, IL, USA). P<0.05 was considered statistically significant.

We evaluated 62 tissue specimens from HCC patients by immunohistochemistry for Bmi-1 expression. Consistent with previous reports (14), Bmi-1 protein was mainly observed in neoplastic epithelial cell nuclei. Positive staining for Bmi-1 protein was observed in 46.8% (29/62) of HCC tissues. By contrast, no staining or only weak staining was observed in normal liver tissues. Staining of representative samples is presented in Fig. 1.

We compared Bmi-1 expression with the clinicopathological parameters of 62 patients to investigate the clinical significance of Bmi-1 expression during hepatocyte carcinogenesis. As shown in Table I, there was no correlation between the expression of Bmi-1 and certain clinical features, such as age, gender, tumour location, histological grade, satellite lesions, tumour number and AFP level. However, Bmi-1 expression was strongly associated with tumour size, metastasis, venous invasion and AJCC TNM stage. This result indicated a correlation between Bmi-1 expression and HCC invasion and metastasis.

To evaluate the overall survival rate of HCC patients in relation to Bmi-1 expression, we carried out Kaplan-Meier survival analysis and log-rank test. The result demonstrated that patients with positive Bmi-1 expression had a significantly shorter 5-year survival rate than patients with negative levels of Bmi-1 expression (P<0.001, log-rank test; Fig. 2).

A univariate Cox regression analysis showed that the overall survival was directly influenced by metastasis, venous invasion, satellite lesions, AJCC TNM stage and Bmi-1 protein expression (Table II). To determine the relative importance of each variable, multivariate Cox regression analyses were performed. Multivariate analysis revealed that expression of Bmi-1 (P<0.001, HR = 5.095; 95% CI, 2.169–11.969), metastasis (P<0.001, HR = 18.163; 95% CI, 4.854–67.968) and venous invasion (P=0.034, HR = 3.083; 95% CI, 1.091–8.711) were independent prognostic factors for overall survival in patients who have undergone curative resection for HCC (Table II).

To further describe the role of Bmi-1 in the progression of HCC, Bmi-1 expression was first compared among three HCC cell lines (HepG2, SMMC-7721 and MHCC97-H) and an immortal hepatocyte cell line (HL-7702) that was used as a reference for Bmi-1 expression by real-time PCR and western blotting. The levels of Bmi-1 expression were significantly higher in all three HCC cell lines compared with that of the HL-7702 cells (Fig. 3).

Among these 3 HCC cell lines, HepG2 cells are the least invasive, SMCC-7721 is moderately invasive and MHCC97H cells are the most invasive (22). Our results showed that the invasive abilities of these cells were consistent with their Bmi-1 expression (Fig. 3). This finding indicated that the upregulated levels of Bmi-1 may play a role in invasive behaviour.

A shRNA vector that co-expresses GFP was generated for stable and efficient Bmi-1 reduction in HCC cells and the transfection efficiency was assessed by fluorescence microscopy. Almost all HepG2 and MHCC97-H cells were successfully transduced with lentivirus shRNA vector (Fig. 4A and B). These results confirmed that Bmi-1 shRNA was successfully introduced into the HepG2 and MHCC97-H cells.

As shown in Fig. 4C–F, endogenous Bmi-1 mRNA and protein levels were significantly reduced in HepG2 and MHCC97-H cells transfected with Bmi-1 shRNA vectors compared with the negative control shRNA vector transfected cells and untransfected cells examined by real-time PCR and western blotting, respectively. Thus, Bmi-1 expression was effectively downregulated by Bmi-1 shRNA vectors in two HCC cell lines in vitro.

Because high Bmi-1 expression was positively associated with venous invasion (P=0.009) and metastasis (P=0.025), we further determined whether Bmi-1 was involved in the invasion and metastasis of HCC. To examine whether suppression of Bmi-1 in HCC cell lines affected their invasive properties, we conducted transwell invasion assays in vitro. The numbers of HepG2 and MHCC97-H cells transfected with Bmi-1 shRNA vectors invading through the filter were markedly lower than the number of the negative control groups and mock groups (Fig. 4G and H). Bmi-1 knockdown dramatically inhibited the invasiveness of HepG2 and MHCC97-H cells.

Because Bmi-1 knockdown inhibited HCC cell invasion, we also investigated its effect on metastasis-related genes. MMP-2, MMP-9 and VEGF play important roles in cancer invasion and metastasis (23), including HCC (22). We determined the protein levels of these three genes by western blotting after transfection. As shown in Fig. 5A, transfection of HepG2 and MHCC97-H cells with Bmi-1-shRNA vectors reduced MMP-2, MMP-9 and VEGF protein levels. We confirmed the effect of Bmi-1-shRNA on MMP-2, MMP-9 and VEGF levels by ELISA. As shown in Fig. 5B–G, Bmi-1 knockdown in HCC cells significantly decreased MMP-2, MMP-9 and VEGF levels. These data indicate that the effects of Bmi-1 on invasion may be mediated by MMP-2, MMP-9 and VEGF.

One previous report indicated that Bmi-1 can downregulate the transcription of PTEN (24). Therefore, we investigated whether PTEN was upregulated in HCC cells with Bmi-1 knocked down. As shown in Fig. 5H, PTEN levels were increased in HCC cells with Bmi-1 knockdown compared to the mock groups and the control groups. These results demonstrated that PTEN was upregulated by Bmi-1 silencing.

PTEN is a tumour suppressor with phosphatase activity that can inhibit tumour metastasis via negative regulation of the PI3K/Akt pathway (25). Moreover, the PI3K/Akt signalling pathway is known to play a major role in signalling pathways responsible for the invasion and migration of various cancers (26). Furthermore, PTEN regulates the expression of MMPs and VEGF in HCC (27). Upregulation of Bmi-1 can activate the PI3K/Akt pathway (24). Therefore, we considered that Bmi-1 participates in the invasion and metastasis of HCC by activation of the PI3K/Akt pathway. To test this hypothesis, we examined the levels of phosphorylated Akt and total Akt. Western blot analyses showed less phosphorylated Akt in HCC cells with Bmi-1 knockdown compared to the negative control groups and mock groups but no change in the total amount of Akt. This experiment demonstrated that knockdown of Bmi-1 inhibited the Akt pathway (Fig. 5H).

To further study whether Bmi-1 participates in the invasion and metastasis of HCC cells via PI3k/Akt pathway, HepG2 and MHCC97-H cells were treated with the highly specific PI3K/Akt pathway inhibitor LY294002. LY294002 (10 μM) alone reduced HCC cell invasion. However, treatment with LY294002 in HCC cells with Bmi-1 knockdown did not further reduce the invasion ability compared to HCC cells treated with LY294002 alone or HCC cells with Bmi-1 knockdown alone (Fig. 5I and J). These results suggested that Bmi-1 may promote HCC cell invasion through the activation of the PI3K/Akt pathway with subsequent regulation of MMP-2, MMP-9 and VEGF expression.