Human retinoblastoma cell line RB-Y79 was purchased from American Type Culture Collection (ATCC, Rockville, MD, USA), human retinal pigment epithelium cell line hTERT-RPE1 was purchased from JENNIO Biological Co. (Guangzhou, China). All the cells were cultured at 37°C in a humidified incubator under 5% CO₂ in RPMI-1640 (Gibco, USA) with 10% fetal bovine serum (FBS) (Gibco, Australia) and 1% penicillin-streptomycin solution (Gibco, USA). All anti-human CD3-FITC, CD8-APC, CD56-PE, CD80-PE, CD83-APC, CD86-FITC antibodies were obtained from BD Co. (BD, USA). Cytokines recombinant mutant human tumor necrosis factor-α (TNF-α), recombinant human interferon-γ (IFN-γ), recombinant human interleukin-2 (IL-2), recombinant human granulocyte/macrophage colony-stimulating factor (GM-CSF), recombinant human interleukin-4 (IL-4) and CD3 monoclonal antibody were purchased from Peprotech (Rocky Hill, NJ, USA). Propidium iodide (PI) and 5-carboxy-fluorescein diacetate succinimidyl ester (CFSE) were purchased from Beyotime Institute of Biotechnology (Shanghai, China), Carboplatin was purchased from Qilu Pharmaceutical Co. (Ji’nan, Shandong, China).

Blood was freshly drawn from healthy volunteers according to our protocol accepted by the local ethics committee (LEC). PBMCs were isolated by Ficoll/Hypaque density gradient centrifugation, according to standard procedures (25). PBMCs at a density of 5×10⁶ cells/ml were allowed to adhere in Alys-505 complete culture medium (Alys-505 medium supplemented with 0.5% auto-plasma and 1% penicillin/streptomycin) for 3 h at 37°C in a humidified 5% CO₂ incubator. The adherent PBMCs were cultured in Alys-505 complete medium with 500 U/ml GM-CSF and 1000 U/ml IL-4 to generate DCs. The medium was changed every 3 days. In the experiment where TNF-α was tested, 1000 U/ml of TNF-α was added to the media on day 6. The non-adherent PBMCs were cultured in Alys-505 complete medium containing 1000 IU/ml IFN-γ, 200 ng/ml CD3 monoclonal antibody and 250 U/ml IL-2 for generating CIK cells. After day 7 in culture, CIK cells were sub-cultured in fresh Alys-505 complete culture medium with 200 U/ml IL-2 every 3 days.

RB-Y79 tumor lysates were generated by three rapid freeze-thaw cycles. Briefly, confluent cultures of RB-Y79 were detached by incubation with trypsin-EDTA 0.05% for 5 min, washed in PBS and resuspended in PBS at a density of 1.5×10⁷ cells/ml. The cells in suspension were frozen in liquid nitrogen and disrupted by three freeze-thaw cycles. The cell lysis was clarified by centrifugation for 10 min at 600 × g. The supernatant was then collected and stored at −80°C. DCs were incubated in the presence of the tumor lysates from the day 3 of DC maturation.

CIK cells were co-cultured on day 7 with autologous 7-day DC or DC-Ag in a 3:1 ratio. All the groups were cultured at 37°C in a humidified 5% CO₂ incubator and sub-cultured every 3 days in Alys-505 complete culture medium with 200 U/ml IL-2. Cell number was counted from day 7 to 15 in culture using Counter Star with the software Automated Cell Counter.

DCs were phenotyped with a panel of antibodies: CD80-PE, CD83-APC and CD86-FITC. CIK cells were phenotyped with antibodies against CD3-FITC, CD8-APC and CD56-PE. A mouse IgG (PE/FITC/APC) (BD) was used as a negative control in all the assays. Briefly, 1×10⁶ cells were incubated with the corresponding antibodies at 4°C for 15 min and then washed with PBS. A total of 10,000 cells were measured and analysed using CellQuest Pro software. Dual-color flow cytometric analysis was performed on a BD FACSCalibur.

On day 15, supernatants from all experimental groups were collected. IL-6 and IL-10 levels in the media culture were quantitatively measure by using a Cytometric Bead Array Human Th1/Th2 Cytokine kit II (BD) according to the manufacturer’s instructions.

CIK cells, DC-CIK cells and DC-Ag-CIK cells were harvest on day 15 and the cytotoxic activity was measured on target cells, either RB-Y79 or hTERT-RPE1 cells. Briefly, RB-Y79 cells and hTERT-RPE1 cells were suspended in PBS at a density of 1×10⁵ cells/ml and stained with 2 μmol/l CFSE for 10 min at 37°C. After washing 3 times with RPMI-1640 medium containing 10% FBS, the CFSE-labeled RB-Y79 cells or hTERT-RPE1 cells were co-cultured with CIK cells, DC-CIK cells, DC-Ag-CIK cells, respectively. A 10:1, 20:1 and 40:1 effector:target cell ratio was used. RB-Y79 or hTERT-RPE1 cells were cultured with media from the respective effector cell group and they were used as control for the natural death percentage. After culturing for 24 h, the cells from all groups were collected and washed twice with PBS and then incubated with PI (1 μg/ml) at room temperature for 10 min. Life and dead cells were analysed using dual-color flow cytometric analysis performed on a BD FACSCalibur. Each group was tested in triplicate.

For testing the effect of the media on CIK cytotoxicity, 1×10⁵ RB-Y79 cells were co-cultured with 1×10⁶ CIK cells using conditioned media from CIK cells, DC medium and DC-Ag medium. The cytotoxicity was analysed in triplicate as desribed above. In all experiments the cytotoxic activity was defined as the percentage of dead cells after 24 h of treatment less the natural death percentage of the respective cell type.

RB-Y79 cells in logarithmic phase were incubated with 40 μg/ml at 37°C in a humidified 5% CO₂ incubator for 2 h. After centrifugation and washing, the medium containing the drug was discarded. Cells were cultured then in complete culture medium (RPMI + 10% FBS and 1% penicillin/streptomycin). Once the culture growth into the logarithmic phase again the Carboplatin treatment was repeated. The same procedure was repeated for several months until generating a stable resistant cell line at 40 μg/ml carboplatin.

For testing RB-R cell resistance to carboplatin, RB-Y79 and RB-R cells were cultured in the presence of 10, 20, 40, 50, 60, 70, 80, 90 or 100 μg/ml carboplatin respectively. After 24 h, cell numbers were counted in the culture using Counter Star with the Automated Cell Counter software. In addition, 1×10⁵ RB-Y79 and RB-R cells were cultured with carboplatin at 40 μg/ml, respectively. The cytotoxicity was analysed as described above.

For the cytotoxicity assay, CIK, DC-CIK cells and DC-Ag-CIK cells were harvest on day 15 and co-cultured with RB-Y79 and RB-R cells in a ratio 20:1 in the presence or absence of 40 μg/ml carboplatin. After culturing for 24 h, the cells from all groups were collected and washed twice with PBS and then stained with 2 μmol/l CFSE and PI 1 μg/ml. Viable and dead cells were analysed using dual-color flow cytometric analysis performed on a BD FACSCalibur. Each group was tested in triplicate.

For every experiment the cytotoxic activity was defined as the percentage of dead cells after 24 h of treatment less the percentage of natural death of the respective cell type.

In this study mature and active DCs were generated in vitro from peripheral blood mononuclear cells (PBMCs) taken from a healthy volunteer. Cell differentiation in culture was followed over time by checking cell morphology. The mature phenotype was recognized by analyzing the expression of the clusters of differentiation (CD80, CD83, CD86) in the cell membrane using flow cytometry (FCM) (Fig. 1).

Freshly isolated PBMCs were spherical and small, the cell surface was smooth and no protrusions were observed by light microscopy (Fig. 1A, left image). After culturing for 3 days in the presence of cytokine-enriched media, the adherent cells became larger and oval. On day 7, cells lost the ability to adhere to the plastic and started to grow in suspension. An additional morphological feature of these cells was the increment in size, irregular shaped nuclei and the formation of numerous dendritic-like actin processes emerging from the cell body (Fig. 1A, middle and right images) depicting the typical DC morphology corresponding to a mature phenotype. As expected, this change in morphology was accompanied by an increase in the cell surface expression of the CDs (Fig. 1B). After 7 days in culture, FCM assay detected values for the CDs significantly higher compared with the cells on day 3 (P<0.01) [compare CD80 (11.60±1.37)%, CD83 (12.11±0.94)% and CD86 (15.28±0.35)% on day 3 with CD80 (46.65±1.26)%, CD83 (26.14±1.16)% and CD86 (31.05±1.12)% on day 7]. The results showed that DCs developed into the mature phenotype after 7 days (Fig. 1C).

To test the effect of tumor antigen on DC differentiation and maturation in vitro, tumor lysed from RB-Y79 cells (Ag) was added to the DCs from day 3 in culture. On day 7, DC-Ag cells were harvested and the same CDs as above were analysed by FCM. As shown in Fig. 1B and D (top panels), the DC-Ag cells expressed higher levels of CD80 and CD86 compared with DC cultured in cytokine enriched media alone (without Ag) (P<0.01). However, no significant differences were found for CD83 levels.

Because TNF-α have a positive effect on DC differentiation and maturation (26), we tested whether the antigen had a co-stimulatory effect after 1 day of treatment with TNF-α on DC maturation. To examine this hypothesis we analysed CD expression levels on cell surface by FCM (Fig. 1D, bottom panels). The results showed that the addition of TNF-α to the culture medium on day 6 increased significantly CD80, CD83 and CD86 expressions compared to DC without TNF-α (P<0.01), with more obvious differences in the expression level of CD83. TNF-α had a similar effect on DC-Ag cells (Fig. 1E) (P<0.05).

Overall, our findings showed that the antigen could upregulate the expression of the CDs that act as co-stimulatory molecules promoting DC differentiation. In addition, TNF-α had a strong effect on the overall maturation of DCs.

Because TNF-α favored DC differentiation in vitro, the following experiments were performed in the presence of TNF-α. Thus, we can discriminate the effects on DC function attributable to Ag that are independent of maturation.

CIK cells are a sub-population of cytotoxic T-lymphocytes with the characteristic CD3⁺CD56⁺ phenotype. In order to generate CIK cells in vitro, the non-adherent PBMCs were separated and cultured in the presence of interferon-γ (IFN-γ), CD3 monoclonal antibody and IL-2 among other cytokines. After the 7th day in culture, cell morphology indicated that CIK cells had acquired the mature phenotype (Fig. 2A). At day 7, the cell area was on average five times bigger than at day 1 in culture (data no shown) depicting irregular shape. Multiple cells formed clusters and gathered into cell aggregates (arrows in Fig. 2A, left panel). Interestingly, we noted that the actin cytoskeleton of these mature CIK cells attained a polarized distribution (Fig. 2A, middle and right panels).

Next, we analysed the proportion of cells expressing CD3⁺CD56⁺, CD3⁺CD8⁺, CD3⁺ and CD8⁺ in the cell population that had grown in the cytokine-enriched media. As shown in Fig. 2B and C, the proportion of CD3⁺CD56⁺ and CD3⁺CD8⁺ cells increased on day 15 compared with day 7 (P<0.01).

It has been reported that the CIK cells could interact with DCs resulting in an increment of CIK cytotoxic and cytolytic activities against tumor cells. To examine if this applies to our CIK in the presence of DC-Ag, we further examined whether these DC-Ag cells could expand the proportion of mature CD3⁺CD56⁺ CIK cells in culture. CIK and DC-CIK or DC-Ag-CIK phenotypes were assayed with fluorescence-activated cell sorting analyses. On day 15, the proportion of CD3⁺CD56⁺ and CD3⁺CD8⁺ cells were higher when the CIK cells were co-cultured with DC-Ag cells (P<0.01). No obvious differences were found when DC-CIK cells were compared with CIK cells (P>0.05). There were no significant differences for the population of CD3⁺ and CD8⁺ cells compared between the other groups (P>0.05) (Fig. 2D and E).

The results stated above showed the CD3⁺CD56⁺ CIK cell proportion increases in the T-lymphocyte population when they are co-cultured with DC-Ag cells.

We found that CIK cells in culture proliferated in a non-exponential manner, especially from day 9 onwards (Fig. 3A). To examine whether DCs or DC-Ag affected CIK proliferation, CIK cells were co-cultured with DCs or DC-Ag from day 7 to 15 and the cell number per ml of medium was quantified everyday in the different groups (Fig. 3A). After 15 days in culture the absolute cell number had significantly (P<0.01) increased 5.36±1.58, 8.37±2.19 and 9.38±1.97-fold in CIK, DC-CIK and DC-Ag-CIK, respectively (Fig. 3A).

To investigate a possible cause for the differences observed on CIK cell proliferation, we determined the level of two cytokines that have been shown to play a role in the proliferation of these cells (IL-6 and IL-10). IL-6 was selected because it was shown to have stimulatory effect on CIK proliferation and IL-10 because it has inhibitory effect on primary alloreactive T-cell responses (27,28). The supernatants from CIK and DC-CIK or DC-Ag-CIK cultures were collected on day 15 and the specific cytokines were quantified by using a Cytometric Bead Array Human Th1/Th2 cytokine kit. As shown in Fig. 3B and C, IL-6 levels increased 3-fold when CIK cells were grown in the presence of DC cells or DC-Ag (1.65±0.13 pg/ml) and (1.78±0.28 pg/ml), respectively, compared with levels of secreted IL-6 in CIK culture alone (0.57±0.16 pg/ml) (P<0.01). In contrast, secreted IL-10 level was two-fold lower in DC-Ag-CIK cell co-culture (Fig. 3C) compared with CIK or CIK co-cultured with DC cells (Fig. 3B and D). These results indicate that CIK cells increased proliferation in the presence of DCs and DC-Ag might be a consequence of the combination of a low level of the inhibitory IL-10 and elevation of the stimulatory IL-6 levels in these co-culture conditions.

Having shown that the DC-Ag cell enhanced CIK proliferation and differentiation in vitro (Figs. 1 and 2) we next tested whether these processes translated to an increment in CIK cytotoxic activity on RB-Y79 cells (Fig. 4).

CIK cells were co-cultured either with autologous non-pulsed DCs or tumor lysate-pulsed DCs (DC-Ag) for 7 days starting on culture day 7 and tested for cytotoxicity against RB-Y79 cell line at day 14. The cytotoxicity was assayed by FCM using specific dyes for labeling viable and dead cells. The results, shown in Fig. 4, are expressed as the proportion of cells that are dead relative to the total number of cancer cells in the culture, minus the natural cell death observed in each condition.

As shown in Fig. 4A, CIK cells generated by the cytokine-enriched media killed ~6% of the RB-Y79 cells after co-culturing for 24 h at a ratio of 10:1 [effector cells:target cells (E:T)]. The cytotoxicity doubled when the CIK had been co-cultured with the DCs for 7 days. Moreover, the CIK cytotoxicity was significantly higher when they were in the presence of DC-Ag (P<0.001). Higher E:T ratios resulted in significantly higher cytotoxicity (P<0.01) throughout the experimental conditions. This observation suggests that the effects are unlikely to result from unspecific influences, other than the killer cells.

To rule out the possibility that the cytotoxicity was the result of some unidentified agent present in the cell media rather than by the CIK cell activity, the cytotoxic of the assay was performed on RB-Y79 cells incubating the CIK with conditioned media taken from DC or DC-Ag cultures instead of with the DCs or DC-Ag. No significant difference was found on the CIK cytotoxic activity on RB-Y79 cells between the 3 treatments (Fig. 4B) (P>0.05). These observations suggested that the enhancement of cytotoxic activity on tumor cells could be at least in part explained by the direct interaction of CIK cells with mature DC rather than by activity of the components we added to the culture media.

CIK cells have been described as a highly efficient cytotoxic effector capable of lysing tumor cell targets by a mechanism that is non-MHC restricted. Because of this, we explored whether CIK cells (mature and activated with DC and DC-Ag) have specific cytotoxic activity on RB cell lines or if they also targeted normal retinal cells. We set up the cytotoxic assay as described above and we determined the CIK cytotoxic activity on hTERT-RPE1 cells. Surprisingly, no significant cytotoxicity was detected on hTERT-RPE1 cells in any of the assayed groups. The CIK cytotoxic activity on these cells was 1.13% at an E:T ratio of 10:1 (Fig. 4C).

After establishing the RB-Y79 carboplatin-resistant cell line, cells were tested for their ability to survive and proliferate in a media containing carboplatin. Resistant and sensitive RB cells were cultured with increasing dosis of carboplatin and the cell survival was analysed after 24 h. The result showed that the number of live RB-sensitive cells decreased significantly as the carboplatin concentration increased. In contrast, the number of RB-resistant living cells was not significantly affected until a dose of 50 μg/ml of carboplatin. However, RB-resistant survival cells gradually decreased with 50 μg/ml or higher drug concentration (Fig. 5A and B). Given this ability of the RB-resistant cells to survive at 40 μg/ml carboplatin, we named it RB-R cells.

In order to prove that RB-R cells are resistant to carboplatin, 40 μg/ml of carboplatin was used on RB-sensitive cells and RB-R cells. The result showed that the ability to survive carboplatin was more than two-fold increased in RB-R cells compared to the sensitive RB cells (Fig. 5C).

We have shown that CIK, DC-CIK and DC-Ag-CIK cells had a strong cytotoxic activity on normal RB cells, we wanted to test whether the effector cells could kill RB-R cells efficiently. CIK, DC-CIK and DC-Ag-CIK cells were used after 7 days co-culture on day 14 and tested for cytotoxicity against RB-R cell line at 40 μg/ml. The cytotoxicity was assayed by FCM using specific dyes for labeling viable and dead cells. DC-Ag-CIK cells generated by the cytokine-enriched media killed ~20% of the RB-R cells after co-culturing for 24 h at an E:T ratio of 20:1 (Fig. 5D). The cytotoxicity of DC-Ag-CIK cells against RB-R cells were higher than DC-CIK and CIK cells (P<0.01), but there was no significant difference between DC-CIK and CIK cells (P>0.05). To test the combined effect of carboplatin, RB-R cells co-cultured with effector cells were incubated with 40 μg/ml carboplatin for 24 h. The cytotoxicity of DC-Ag-CIK in combination with carboplatin showed the best antitumor activity compared with DC-CIK and CIK cells, and DC-CIK were higher than CIK cells (P<0.01). In all groups, the effector cells that were combined with carboplatin showed higher cytotoxicity than effector cells alone (P<0.01).