This Article Abstract Full Text (PDF) Supplementary Data Alert me when this article is cited Alert me if a correction is posted Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Das, T. Articles by Tannenbaum, C. Search for Related Content PubMed PubMed Citation Articles by Das, T. Articles by Tannenbaum, C.

GM1 and Tumor Necrosis Factor-, Overexpressed in Renal Cell Carcinoma, Synergize to Induce T-Cell Apoptosis

¹ Molecular Medicine Division, Bose Institute, Kolkata, India; ² Department of Immunology, Lerner Research Institute and ³ Experimental Therapeutics, Taussig Cancer Center, Cleveland Clinic, Cleveland, Ohio

Requests for reprints: Charles Tannenbaum, Department of Immunology/NE4-308, Lerner Research Institute, Cleveland Clinic Foundation, Cleveland, OH 44195. Phone: 216-445-0575; Fax: 216-444-9329; E-mail: tannenc{at}ccf.org.

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

 
The ability to induce T-cell apoptosis is one mechanism by which tumors evade the immune system, although the molecules involved remain controversial. We found that renal cell carcinoma (RCC)–induced T-cell apoptosis was inhibited by >50% when cocultures were performed with ganglioside-depleted tumor cells, caspase-8–negative lymphocytes, or anti–tumor necrosis factor- (TNF) antibodies, suggesting that tumor gangliosides synergize with signals delivered through TNF death receptors to mediate T-cell killing. The synergy between tumor-derived TNF and the RCC-overexpressed ganglioside GM1 for killing resting T cells is corroborated by studies using purified GM1 and rTNF, which indicate that a 48-hour pretreatment with the ganglioside optimally sensitizes the lymphocytes to a TNF-induced apoptotic death. However, activated T cells, which synthesize TNF themselves, can be killed by exogenous GM1 alone. RelA-overexpressing lymphocytes are protected from GM1 plus TNF-mediated apoptosis, a finding consistent with our previous studies indicating that gangliosides inhibit nuclear factor-B activation. These results are clinically relevant because, similar to T-cells cocultured with GM1-overexpressing RCC lines, T cells isolated from the peripheral blood of patients with metastatic RCC are also heavily coated with that tumor-shed ganglioside. This population of patient cells, unlike T cells isolated from normal donors, is highly susceptible to apoptosis induced by rTNF or by metastatic patient sera, which contain elevated levels of the cytokine. This report thus extends our previous studies by demonstrating that tumor-derived TNF enhances RCC apoptogenicity not only by inducing ganglioside synthesis but also by initiating receptor-dependent apoptosis in T cells in which the nuclear factor-B activation pathway has been inhibited by GM1. [Cancer Res 2008;68(6):2014–23]

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

 
Numerous studies indicate that tumors do elicit immune responses, with tumor-specific T-lymphocytes clonally expanding in many individuals harboring malignancies (1, 2). These initial responses seem to be either short lived or ineffective, however, because the majority of tumors progress and metastasize, and most patients eventually die of their disease (3). Our laboratory studies tumor-induced T-cell apoptosis as a mechanism by which renal cell carcinoma eludes immune destruction: when examined by in situ terminal nucleotidyl transferase (TdT)–mediated nick end labeling (TUNEL) analysis, 30% to 100% of renal cell carcinoma (RCC) tumor-infiltrating lymphocytes (TIL) are Annexin V/amino actinomycin D–positive (4). The systemic reach of tumor-mediated immunosuppression is suggested by the fact that even patient peripheral blood T cells are susceptible to activation-induced cell death upon explantation (4). It is the tumors themselves that mediate these effects because T lymphocytes undergo the same physiologic changes associated with apoptosis following in vitro culture with cancer cell lines (5–7).

A variety of tumors have been reported to express aberrantly elevated levels of FasL, TNF-related apoptosis-inducing ligand, or CD70, ligands that can mediate proapoptotic effects upon binding their specific cognate receptors (8–10). Our laboratory has also recently elucidated a role for soluble, tumor-associated products in mediating T-cell apoptosis (11, 12). Further studies have shown that shed, overexpressed tumor-associated gangliosides play a significant part in these events (13–16). Renal cell carcinomas, for example, display increased levels of GM1, GM2, and GD1a (17). Although there is precedence for gangliosides suppressing antitumor immunity (18, 19), the mechanism by which they act is unclear.

Our previous studies indicated that gangliosides purified from RCC supernatants depressed nuclear factor-B (NFB) activation in lymphocytes, and also triggered cytochrome c release and induced apoptosis if coincubated with T cells for extended periods (7, 11, 12, 20). All of these effects were also mediated by the tumor cells themselves, but were abrogated when tumor ganglioside synthesis was inhibited prior to coculture by pretreatment with the glycosylceramide synthase inhibitor 1-phenyl-2-hexadecanoylamino-3-pyrrolidino-1-propanol. Our finding that caspase-8–negative Jurkat cells were also largely resistant to a ganglioside-overproducing RCC line suggested that another tumor-derived product, likely acting through a death receptor, might also synergize with glycosphingolipids to mediate T-cell death. Interestingly, loss of function mutations in the von Hippel-Lindau (VHL) tumor suppressor protein are common in clear cell RCC (21, 22). Because tumor necrosis factor- (TNF) is up-regulated in tumors harboring the mutation (23), most RCCs synthesize TNF constitutively. Reports demonstrating that TNF stimulates ganglioside expression in several normal cell types (24) led to our experiments revealing that TNF could augment tumor killing of cocultured T-lymphocytes via a mechanism involving increased tumor ganglioside synthesis (13). Left unresolved, however, was the molecular pathway(s) by which these TNF- and ganglioside-producing tumor cells mediated their toxic effects. Here, we report that RCC-derived products GM1 and TNF, in both their tumor-associated and purified forms, could induce T-cell dysfunction by synergistically activating the receptor-dependent apoptotic pathway in lymphocytes. The physiologic relevance of these studies stems from our findings that, unlike lymphocytes from healthy donors, peripheral blood T cells isolated from patients with RCC stain strongly for GM1, and are induced to apoptosis when treated in vitro with either TNF or with RCC patient serum, which we find contains elevated levels of TNF.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

 
Reagents. Anti-TNF, anti-TNFR1, anti–caspase-8, anti–caspase-9, and anti-FADD antibodies were rabbit polyclonal antibodies from Santa Cruz Biotechnology, and murine monoclonal antiactin was purchased from Abcam. Horseradish peroxidase–conjugated sheep anti-mouse and donkey anti-rabbit immunoglobulin antibodies were from Amersham. FITC-labeled cholera toxin was from List Biologicals, and anticholera toxin antibody was from Calbiochem. Protein Sepharose beads were from Pierce. Phorbol 12-myristate 13-acetate (PMA) and ionomycin were from Sigma-Aldrich. Monoclonal anti-CD3 (OKT3) and monoclonal anti-CD28 (BD Immunocytometry Systems) were from Ortho Biotech. Caspase-8 inhibitor I (IETD-CHO), used at 50 µmol/L, was from Calbiochem. GM1 was from Matreya. Gangliosides were isolated from RCC tissues, purified and subjected to high-performance liquid chromatography (HPLC) as previously described (25). Human recombinant interleukin-2 [Aldesleukin (Proleukin), CHIRON Corporation] was used at 20 units/mL to maintain the viability of activated T cells.

Plasmids and transfection. TNF was cloned from activated T cells, and the cDNA was inserted into the HindIII and Xba sites of PcDNA3. Jurkat cells were transfected and selected with G418 as described previously (20) and clones generated by limiting dilution were characterized for cytokine production using a TNF ELISA kit (R&D Systems). The RelA cDNA and RelA-transfected Jurkat cells were prepared as described previously (20).

Cell culture. Peripheral blood was obtained and T cells purified and activated as described previously (13). The Jurkat leukemic T-cell line was purchased from American Type Culture Collection. Caspase-8–negative Jurkat cells were a gift from John Blenis (Department of Cell Biology, Harvard Medical School, Boston, MA; ref. 26). The long-term renal cell carcinoma line (SK-RC-45; ref. 27) was obtained, grown, and used experimentally in cocultures as described previously (13). A variant clone of SK-RC-45 with enhanced apoptogenicity for resting T cells was isolated from the parental stock, expressed elevated levels of TNF, and hence, was designated SK-RC-45_hi. SK-RCC-45 clone 24 was derived by transfecting the parental SK-RC-45_low cells with a TNF-encoding plasmid. A normal kidney epithelial (NKE) cell line was used as a negative control in coculture experiments.

Immunofluorescence. Tumor lines were immunostained to assess GM1- and TNF expression levels. Cells were fixed in paraformaldehyde and permeabilized with Triton X-100 (Sigma). Cells were blocked with 2% fetal bovine serum/1% bovine serum albumin, and incubated overnight at 4°C with either FITC-labeled cholera toxin or anti–TNF antibodies. Cells were subsequently incubated with the appropriate, labeled secondary antibodies (Molecular Probes), washed, and counterstained with 4',6-diamidino-2-phenylindole (DAPI) to visualize the nuclei.

Analysis of DNA fragmentation by TUNEL analysis. Cells were fixed in 1% paraformaldehyde, and were stained and analyzed for apoptosis using the APO-BRDU system (Invitrogen), as described previously (20).

Cell lysates and analysis of protein by Western blotting. Cell pellets were resuspended in lysis buffer and subjected to Western analysis as described (7).

Analysis of TNF expression using reverse transcription-PCR and chemiluminescent ELISAs. Total cellular RNA was extracted and subjected to semiquantitative reverse transcription-PCR (RT-PCR) analysis according to previously described methods and cycling conditions (28). The primer and probe sequences for TNF and glyceraldehyde-3-phosphate dehydrogenase were as described (28, 29). Sera isolated from 19 patients with RCC and 6 normal controls were assessed for their TNF concentrations using the QuantiGlo Human TNF chemiluminescent ELISA kit (R&D Systems) according to the manufacturer's instructions.

HPLC analysis of tumor gangliosides. Tumor gangliosides isolated from SK-RC-45_low and SK-RC-45_hi were subjected to HPLC analysis as previously described (13).

Statistical analysis. Student's t test (two paired samples for mean or two samples using equal variances) was used to determine P using Microsoft Excel Software (version 2003). SE was calculated from SD using Microsoft Excel software.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
RCC tumor cells kill resting T-lymphocytes by a mechanism dependent on gangliosides and the TNF receptor/ligand pair. Gangliosides are overexpressed by a variety of tumor types (19), and have been reported to mediate cytotoxic effects by disrupting the mitochondrial function of target cells (7, 30). The data presented in Fig. 1 support the notion that tumor gangliosides also contribute to T-cell apoptosis by a mechanism exhibiting death receptor dependency. When NKE cells and two RCC cell lines differing vastly in their TNF expression levels (SK-RC-45_low and SK-RC-45_hi; Fig. 1A and B) were compared for their relative abilities to kill cocultured resting T cells in vitro, the NKE cells were found to have a negligible effect whereas the tumor lines mediated apoptosis in proportion to their levels of TNF expression (Fig. 1C). Unlike the NKE cells, which even if pretreated with TNF did not overexpress gangliosides and could not induce T-cell apoptosis, SK-RC-45_hi (13) and the TNF-transfected SK-RC-45 clone 24 stimulated an average of 55% to 60% of the lymphocytes to TUNEL positivity (Fig. 1C and D). This was more than twice the level of T-cell apoptosis induced by the parental SK-RC-45_low line, which also became more apoptogenic if pretreated with TNF prior to a coculture experiment (Fig. 1C).

View larger version (34K): [in this window] [in a new window] [Download PPT slide]   Figure 1. RCC tumor cells expressing elevated levels of TNF exhibit enhanced apoptogenicity for T cells. A, RNA preparations from NKE cells and two RCC clones were subjected to RT-PCR using 5' and 3' primers for TNF, demonstrating the isolation of an SK-RC-45 variant clone (SK-RC-45hi) expressing 7-fold higher levels of the cytokine than SK-RC-45low. Primers for glyceraldehyde-3-phosphate dehydrogenase (GAPDH) served as a control for RNA levels in each sample. B, NKE, SK-RC-45low, and SK-RC-45hi cells were subjected to immunostaining with 2 µg/mL of anti-TNF, followed by Alexa 488–labeled secondary antibody. Nuclei were revealed by DAPI staining. C, resting T cells were cocultured for 72 h with NKE cells, SK-RC-45hi, SK-RC-45low, TNF-transfected SK-RC-45low (clone 24), or SK-RC-45hi in the continuous presence of anti-TNF antibodies (10 µg/mL), at which time, lymphocytes were evaluated by TUNEL for apoptosis. Columns, mean of three experiments; bars, SE (*, P < 0.001; **, P < 0.01 versus medium alone). D, resting T cells incubated in medium or cocultured with SK-RC-45hi for 72 h were analyzed for tumor-induced apoptosis by TUNEL analysis. Typical data obtained by flow cytometry which was used to generate the results in C, and all subsequent experiments assessing T cell apoptosis under various experimental conditions.

Caspase-8–deficient Jurkat cells are resistant to the apoptogenic SK-RC-45_hi line. Because caspase-8 is a requisite for death receptor–dependent activation of the caspase cascade (31), the use of caspase-8–negative Jurkat cells provided an opportunity to assess the role of TNFR1 in SK-RC-45_hi–mediated killing (Fig. 2A and B ). Wild-type and caspase-8–negative Jurkat cells were thus analyzed for DNA breaks by TUNEL following a 72-hour coincubation with adherent SK-RC-45_hi monolayers. Wild-type Jurkat cells were highly sensitive to SK-RC-45_hi, with an average of 55% of the cocultured lymphocytes testing positive for apoptosis (Fig. 2C), although only minimal TUNEL positivity was evident when, as controls, the lymphocytes were exposed to NKE cells (7.0% apoptosis) or fresh medium alone (3%; data not shown). The defect in T-cell death receptor signaling conferred by the caspase-8 mutation, however, dramatically decreased the susceptibility of that Jurkat cell clone to SK-RC-45_hi by 55%, suggesting that the tumor-derived TNF, beyond inducing ganglioside synthesis, is additionally acting in a death receptor and caspase-8–dependent manner (Fig. 2C). Supporting this conclusion was the even greater inhibition of tumor-induced apoptosis observed (65% inhibition) when SK-RC-45_hi cells were coincubated with wild-type Jurkat cells in the presence of caspase-8 inhibitor I (IETD-CHO; Fig. 2C). The fact that SK-RC-45_hi–induced Jurkat cell apoptosis can be reduced by >50% either by abrogating tumor cell ganglioside synthesis or by inhibiting death receptor–mediated activation of the caspase cascade, indicates that the RCC tumor line synthesizes multiple proapoptotic products (i.e., TNF and gangliosides) that synergize to induce the apoptosis of Jurkat cells and normal T cells.

View larger version (31K): [in this window] [in a new window] [Download PPT slide]   Figure 2. Caspase-8 negativity protects T cells from apoptosis induced by SK-RC-45hi. A, wild-type and caspase-8–negative Jurkat cells were stained with anti-TNFR1 to assess TNFR1 receptor expression by flow cytometric analysis, as described in Materials and Methods. B, cytoplasmic lysates made from wild-type and caspase-8–negative Jurkat cells were subjected to Western blot analysis using 10 µg protein/lane and antibodies to FADD, caspase-8, caspase-9, caspase-3, and actin. C, wild-type Jurkat cells, caspase-8–negative Jurkat cells or wild-type Jurkat cells, pretreated for 90 min with 50 µmol/L of caspase-8 inhibitor I were incubated with SK-RC-45hi for 72 h prior to analyzing the lymphocytes by TUNEL for tumor-induced apoptosis, as described in Materials and Methods. Columns, mean of three experiments; bars, SE (*, P < 0.001).

RCC tumor cells overexpress GM1 and induce apoptosis of resting T-lymphocytes in proportion to their level of TNF synthesis.

View larger version (31K): [in this window] [in a new window] [Download PPT slide]   Figure 3. TNF-producing RCC cells overexpress the ganglioside GM1, which adheres to T-cell membranes and participates in lymphocyte killing. A, NKE cells, SK-RC-45low, SK-RC-45hi, and primary RCC tumor cells were stained with 2 µg/mL of FITC-labeled cholera toxin and examined by fluorescent microscopy for GM1 expression, as described in Materials and Methods. B, HPLC profiles of gangliosides isolated from SK-RC-45low and SK-RC-45hi cell lines were obtained as described in Materials and Methods, demonstrating the elevated levels of GM1 in SK-RC-45hi. C, normal, peripheral blood resting T-cells were either cocultured with SK-RC-45hi, or incubated in the presence or absence of 25 µg/mL of GM1 for 2 h, prior to staining the lymphocytes with FITC-labeled cholera toxin to assess levels of T-cell membrane–associated GM1. D, conditioned medium from confluent cultures of NKE cells, SK-RC-45low, or SK-RC-45hi were immunodepleted or not of GM1 with cholera toxin/anti–cholera toxin/protein A-Sepharose beads. Resting T cells from normal donors were then cultured for 72 h in each (diluted 50% with fresh medium), and then subjected to TUNEL analysis to assess the involvement of GM1 in apoptosis induced by tumor supernatants. Supernatants treated with control IgG and protein A-Sepharose beads served as negative controls. Columns, mean of three experiments; bars, SE (*, P < 0.005 vs. GM1-depleted NKE supernatants; **, P < 0.05 vs. NKE-depleted supernatants).

Both purified GM1 and purified RCC gangliosides synergize with recombinant TNF to induce apoptosis of resting T cells.

View larger version (23K): [in this window] [in a new window] [Download PPT slide]   Figure 4. Gangliosides and TNF synergistically induce T-cell apoptosis. A, resting peripheral blood T-cells were treated with escalating doses of GM1 for 48 h prior to stimulating them or not for 24 h with 100 ng/mL of TNF. Cells were subsequently analyzed for apoptosis by TUNEL. Columns, mean of three experiments; bars, SE (*, P < 0.001; **, P < 0.01 vs. 0 µg/mL GM1). B, resting peripheral blood T-cells were treated with 25 µg/mL of GM1 for 24, 48, 72, and 96 h, the last 24 h in the presence or absence of 100 ng/mL of TNF. Cells were subsequently analyzed for apoptosis by TUNEL. Columns, mean of three experiments; bars, SE (*, P < 0.001; **, P < 0.01; ***, P < 0.05 vs. 0 h GM1 pretreatment). C, resting peripheral blood T-cells were treated or not with 25 µg/mL of GM1 with or without TNF as described in A, prior to being stained with DAPI to quantify apoptotic nuclei by fluorescent microscopy. D, RCC gangliosides were isolated from SK-RC-45hi as described in Materials and Methods, and were used at different concentrations to treat resting T cells prior to a subsequent stimulation with 100 ng/mL of TNF. After 72 h, cells were subjected to TUNEL analysis to quantify apoptosis induced by the different treatments (*, P < 0.001; **, P < 0.01 vs. 0 µg/mL RCC gangliosides).

GM1 can synergize with T cell–derived TNF to kill activated T lymphocytes directly. Although 25 µg/mL of GM1 alone was not significantly apoptogenic for resting T cells (Fig. 4A), it could induce the apoptotic death of TNF-expressing activated T-cells (Fig. 5A ). Although both resting and activated T cells express TNFR1 (Fig. 5B), only the activated cells express detectable TNF (Fig. 5B). Thus, it may be that because activated T cells can provide their own source of synergizing TNF, they can be killed by GM1 alone (Fig. 5A). This contrasts with TNF-deficient, resting T-cells, which can only be killed by GM1 plus TNF (Fig. 4A–C) or by an RCC tumor line that expresses both gangliosides and TNF (Figs. 1C, D, and 3D). Indeed, incubation of activated T cells with GM1 in the presence of antibodies to TNF significantly abrogated the ganglioside-mediated killing (Fig. 5A), whereas control IgG had essentially no effect. This line of reasoning was further supported by experiments showing that Jurkat cells treated with GM1 or TNF did not undergo apoptosis unless the two reagents were used in synergy, in which case, >55% of the cells succumbed (Fig. 5C). Jurkat cells engineered to secrete their own source of TNF, on the other hand, remained viable when cultured in medium or if treated with additional TNF, but could be induced to apoptosis if treated with 25 µg/mL of purified GM1 alone, the latter likely synergizing with cellular sources of TNF to mediate the effect (Fig. 5C).

View larger version (25K): [in this window] [in a new window] [Download PPT slide]   Figure 5. GM1 alone can induce the apoptosis of activated T-cells and TNF-transfected Jurkat cells. A, peripheral blood T-cells preactivated with anti-CD3/anti-CD28 were treated with increasing doses of GM1 (10, 25, 50 µg/mL), in the continuous presence or absence of control IgG or anti-TNF antibodies for 72 h, prior to being assessed for apoptosis by TUNEL. Columns, mean of three experiments; bars, SE (**, P < 0.01; ***, P < 0.05 vs. No IgG). B, resting peripheral blood T-cells were stimulated or not with either PMA/ionomycin or anti-CD3/anti-CD28 prior to subjecting whole cell lysates to Western blot analysis using antibodies to TNF and TNFR1. Actin served as a loading control. C, wild-type Jurkat cells and a Jurkat cell line permanently transfected with TNF-encoding cDNA were treated for 48 h with 100 ng/mL of TNF alone, 25 µg of GM1 alone, or GM1 for 24 h followed by TNF for 24 h, at which point, cells were analyzed by TUNEL for apoptosis. Columns, mean of three experiments; bars, SE (*, P < 0.001 vs. medium alone).

Jurkat cells genetically defective for NFB activation are susceptible to TNF alone, with GM1 providing no additional effect; conversely, Jurkat cells engineered to overexpress RelA are resistant to the synergistic, apoptotic effects of GM1 and TNF.

To further assess the notion that GM1 might act by inhibiting NFB, we tested the possibility that NFB-overexpressing cells might be resistant to GM1 plus TNF–mediated apoptosis. RelA-transfected and wild-type Jurkat cells were treated or not with GM1, TNF, or both in synergistic combination. As compared with GM1 or TNF, which independently exerted minimal apoptogenicity for either cell line, in synergy, those reagents stimulated 50% of the wild-type Jurkat cells to undergo apoptosis (Supplementary Fig. S1B). RelA overexpression bestowed significant protection against GM1 plus TNF, however, as only 20% of the transfectants were killed by the treatment.

Circulating RCC patient T-cells are coated with tumor-derived GM1, and can be induced to apoptosis in vitro with patient sera but not with normal sera. Unlike normal T cells which stain only weakly for GM1, but strongly after coincubation with the SK-RC-45_hi tumor line (Fig. 3C), TILs and peripheral blood T cells from RCC patients are already coated with the ganglioside upon isolation (Fig. 6A ). These results suggest that elevated levels of circulating GM1 exist in these patients, consistent with our finding that explanted, primary RCC tumors stain brightly for GM1 with FITC-labeled cholera toxin (Fig. 3A). Our results, demonstrating the close positive correlation between TNF and ganglioside production by RCC lines (Fig. 1A and B), suggested the notion that patients bearing intensely GM1-positive RCC tumors would also have elevated serum TNF. To assess this possibility, serum samples from 11 RCC patients with metastatic disease, 8 RCC patients with localized disease, and 6 healthy controls were measured for TNF content by ELISA. The results of this analysis, presented in Fig. 6B, indicated that the molecule was essentially undetectable in the normal serum (0.2 pg/mL), varied in concentration from 1 to 10 pg/mL in the sera of patients with localized disease, and ranged between 4 and 34 pg/mL in the sera of patients with metastatic disease.

View larger version (23K): [in this window] [in a new window] [Download PPT slide]   Figure 6. TILs and peripheral blood T-cells isolated from RCC patients were coated with GM1, and could be induced to apoptosis in vitro with either TNF or RCC patient serum. A, peripheral blood T-cells isolated from healthy donors and patients with RCC, as well as TILs, were stained with FITC-labeled cholera toxin to assess GM1 levels. B, a TNF chemiluminescent ELISA kit was used to measure the TNF levels present in the sera obtained from 6 healthy donors, 8 RCC patients with localized disease, and 11 RCC patients with metastatic disease. Columns, mean of 6 to 11 samples; bars, SE; dots, TNF levels present in the serum of a single individual (*, P < 0.001; ***, P < 0.05 vs. normal serum). C, an RCC patient serum sample (1:1 dilution in complete medium) previously determined by ELISA to contain elevated levels of TNF was incubated for 72 h with T cells from either the corresponding RCC patient or from a healthy donor, at which time, the cells were assessed for apoptosis by TUNEL. One aliquot of patient serum was first treated with anti-TNF antibodies to neutralize the cytokine present in the sample. Cells treated with TNF alone or with GM1 plus TNF served as controls. Columns, mean of three experiments; bars, SE (*, P < 0.001; **, P < 0.01 vs. media alone; ***, P < 0.05 vs. normal serum). D, resting peripheral blood T-cells isolated from three patients with RCC were incubated in vitro with their own respective sera (1:1 dilution in complete medium) for 72 h prior to being assessed for apoptosis by trypan blue exclusion. T cells from three healthy donors treated with autologous sera served as negative controls. Columns, mean of patient sera from three experiments done in triplicate; bars, SE (*, P < 0.001 vs. normal serum).

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

 
Here, we show that multiple RCC-derived molecules can act in synergy to mediate the apoptotic death of T lymphocytes: RCC-induced T-cell apoptosis can be substantially inhibited if the tumor cell/T-cell coincubations are performed with either ganglioside-depleted tumor cells, or in the presence of neutralizing anti-TNF antibodies. The notion that there is a synergistic interaction between tumor-derived gangliosides and TNF for inducing T-cell apoptosis is further corroborated by studies with recombinant TNF and a purified form of the overexpressed RCC ganglioside GM1 (17), which shows similar cooperativity for killing T cells when used together in vitro.

Previous studies from our laboratory indicated that RCC cell lines stimulate the apoptosis of Jurkat cells and T lymphocytes by a mechanism that could be largely inhibited by the glucosylceramide synthesis inhibitor 1-phenyl-2-hexadecanoylamino-3-pyrrolidino-1-propanol (7), an indication that tumor gangliosides were involved. This inhibition was maximal when the tumor cells were pretreated with the ganglioside synthesis inhibitor for 5 days prior to initiating the coculture experiment, a time frame consistent with that required for maximal reduction of tumor ganglioside synthesis, as assessed by HPTLC (33). In this study, the substantial resistance of caspase-8–negative Jurkat cells to a ganglioside-shedding RCC tumor line provided the first suggestion that multiple tumor products might be synergizing to induce T-cell death. The fact that the expression of caspase-8, the apical molecule in the receptor-dependent apoptotic pathway (32), is requisite for maximum lymphocyte susceptibility to RCC-mediated apoptosis, indicates that the renal tumor cells mediate at least some components of their apoptogenicity through a death ligand. In this regard, TNF was hypothesized to be an RCC-associated death ligand potentially involved in tumor-induced T-cell apoptosis. This is because mutations in the VHL tumor suppressor protein are common in clear cell RCC (21), and lead to dysregulated synthesis of a number of proteins, including TNF (23). Indeed, reporter gene assays confirm that TNF mRNA is repressed by the wild-type VHL gene but is actively translated in the VHL mutants (23). These findings are consistent with Northern blot analyses, RT-PCR, and immunohistochemical studies, which all indicate that, unlike normal kidney, human kidney cancer cells themselves constitutively synthesize TNF (34). Because in addition to the TNF generated by VHL-mutated tumor cells, a significant bolus of RCC-associated TNF also likely derives from macrophages that so commonly infiltrate those tumors in vivo (35), it is probable that the renal tumor environment typically contains high levels of TNF. Supporting this notion is the fact that sera obtained from RCC patients assessed in our study had highly elevated levels of TNF as compared with undetectable levels present in the sera from healthy volunteers.

It is interesting to note that whereas RCC lines elaborating both gangliosides and high levels of TNF could efficiently mediate the apoptosis of resting T cells, activated T cells can readily be killed by an RCC line synthesizing gangliosides alone. This likely relates to the fact that whereas both resting and stimulated T cells express TNFR1, only the activated lymphocytes express TNF. We would thus postulate that SK-RC-45_hi–derived TNF efficiently kills resting T cells in conjunction with tumor-derived gangliosides, although SK-RC-45_low (the RCC line synthesizing GM1 but only low levels of TNF) kills activated T cells by virtue of a synergistic interaction between tumor-derived gangliosides and T cell–derived TNF. Similar findings hold true for the purified reagents: efficient apoptosis of resting T cells requires treatment with both GM1 and TNF, whereas activated T cells can be killed by a low dose of GM1 alone.

NFB is a transcription factor whose activity is a requisite for the de novo synthesis of numerous antiapoptotic proteins (36). Because previous studies indicated that RCC gangliosides inhibit PMA/ionomycin–induced NFB activation (11, 12, 20), we hypothesized that ganglioside-mediated sensitization of T cells to TNF-induced activation of the caspase cascade (37) might be a mechanism for the observed synergy. Consistent with this thought are the results presented here indicating that RelA overexpression protects T-cell targets from ganglioside/TNF-induced apoptosis, and that the ability of TNF to kill Jurkat cells that are already NFB-inhibited (by a transgene encoding the IB super repressor) cannot be further enhanced by pretreatment with GM1.

The importance and in vivo relevance of these studies is amplified by our finding that peripheral blood T-cells isolated from patients with RCC stain much more strongly for GM1 than do the T cells isolated from healthy controls. That this enhanced GM1 staining on T cells derives from tumor-shed gangliosides is suggested by two additional observations: (a) when stained with FITC-labeled cholera toxin, tumor cells from eight of eight resected RCC expressed highly elevated GM1 levels as compared with the negligible levels characterizing NKE cells; and (b) when cultured in vitro with either GM1-overexpressing RCC tumor cells or their cell-free, spent culture supernatants, T cells from healthy donors became coated with the ganglioside. Other experiments reported here showed that, functionally, the strong GM1 positivity of patient T cells correlated with their susceptibility to apoptotic death if treated in vitro with either TNF or with patient serum, the latter's toxicity is based on its elevated TNF concentration, as indicated both by ELISA and the ability of anti-TNF antibodies to inhibit the effect.

These studies thus elucidate a novel mechanism by which RCC may be enhancing its own growth and metastatic expansion while combining previous, seemingly unrelated, anecdotal observations into a unified hypothesis defining the means by which renal tumors may be killing T cells. Earlier reports from a variety of laboratories described a role for death receptor–based apoptotic schemes in mediating T-cell death, but definitive tumor-associated ligands have remained elusive and uncertain (38). Other laboratories characterized gangliosides as overexpressed, tumor-associated immunosuppressive molecules (39–41), somehow involved in tumor progression and metastasis (42, 43), yet the mechanism by which these glycosphingolipids produced their deleterious effects on the immune system were obscure. Our laboratory did show that RCC gangliosides could suppress NFB activation in T cells as well as their downstream synthesis of NFB-dependent antiapoptotic proteins (6, 7, 11, 12, 20), but the subsequent events or "second signal" that could render lymphocytes apoptotic was undetermined. In the series of experiments described here, we now show that tumor-derived gangliosides can sensitize T cells to TNFR1-mediated apoptosis, induced by TNF present in the RCC tumor microenvironment. The fact that numerous histologically distinct tumors both overexpress gangliosides and are infiltrated by macrophages, suggests the possibility that this synergistic mechanism of tumor-induced T-cell apoptosis may extend to many forms of cancer. Interestingly, a role for RCC-associated TNF in tumor-induced T-cell apoptosis is consistent with the reported efficacy of infliximab in a phase II clinical trial, in which the anti-TNF antibodies slowed or stabilized disease in 32% of RCC patients with advanced disease (44). In a second, more recent phase II, trial, 46% of RCC patients entering the study with progressive disease obtained a clinical benefit from infliximab therapy, and at higher doses of the anti-TNF antibody, the clinical benefit increased to 61% of patients (45). These results collectively imply that agents which neutralize tumor-associated TNF or block ganglioside synthesis might enhance both spontaneous antitumor immune responses and the efficacy of immunotherapeutic interventions. Current studies are directed at defining the mechanism by which gangliosides inhibit NFB activation, and determining whether TNF and gangliosides synergize through additional pathways to mediate T-cell killing.

	Acknowledgments

 
Grant support: NIH grants RO1-CA111917, CA056937, and CA116255.

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

We gratefully acknowledge the Department of Science and Technology and Indian Council of Medical Research, Government of India.

	Footnotes

 
Note: Supplementary data for this article are available at Cancer Research Online (http://cancerres.aacrjournals.org/).

T. Das and G. Sa contributed equally to this work.

Received 10/29/07. Revised 12/20/07. Accepted 1/11/08.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

 

1. Tatsumi T, Herrem CJ, Olson WC, et al. Disease stage variation in CD4+ and CD8+ T-cell reactivity to the receptor tyrosine kinase EphA2 in patients with renal cell carcinoma. Cancer Res 2003;63:4481–9.[Abstract/Free Full Text]
2. Tatsumi T, Kierstead LS, Ranieri E, et al. MAGE-6 encodes HLA-DRβ1*0401-presented epitopes recognized by CD4+ T cells from patients with melanoma or renal cell carcinoma. Clin Cancer Res 2003;9:947–54.[Abstract/Free Full Text]
3. Finke J, Ferrone S, Frey A, Mufson A, Ochoa A. Where have all the T cells gone? Mechanisms of immune evasion by tumors. Immunol Today 1999;20:158–60.[CrossRef][Medline]
4. Uzzo RG, Rayman P, Kolenko V, et al. Mechanisms of apoptosis in T cells from patients with renal cell carcinoma. Clin Cancer Res 1999;5:1219–29.[Abstract/Free Full Text]
5. Gastman BR, Yin XM, Johnson DE, et al. Tumor-induced apoptosis of T cells: amplification by a mitochondrial cascade. Cancer Res 2001;60:6811–7.
6. Molto L, Rayman P, Paszkiewicz-Kozik E, et al. The Bcl-2 transgene protects T cells from renal cell carcinoma-mediated apoptosis. Clin Cancer Res 2003;9:4060–8.[Abstract/Free Full Text]
7. Kudo D, Rayman P, Horton C, et al. Gangliosides expressed by the renal cell carcinoma cell line SK-RC-45 are involved in tumor-induced apoptosis of T cells. Cancer Res 2003;63:1676–83.[Abstract/Free Full Text]
8. Whiteside TL, Rabinowich H. The role of Fas/FasL in immunosuppression induced by human tumors. Cancer Immunol Immunother 1998;46:175–84.[CrossRef][Medline]
9. Koyama S, Koike N, Adachi S. Expression of TNF-related apoptosis-inducing ligand (TRAIL) and its receptors in gastric carcinoma and tumor-infiltrating lymphocytes: a possible mechanism of immune evasion of the tumor. J Cancer Res Clin Oncol 2002;128:73–9.[CrossRef][Medline]
10. Wischhusen J, Jung G, Radovanovic I, et al. Identification of CD70-mediated apoptosis of immune effector cells as a novel immune escape pathway of human glioblastoma. Cancer Res 2002;62:2592–9.[Abstract/Free Full Text]
11. Uzzo RG, Rayman P, Kolenko V, et al. Renal cell carcinoma-derived gangliosides suppress nuclear factor-B activation in T cells. J Clin Invest 1999;104:769–76.[Medline]
12. Finke JH, Rayman P, George R, et al. Tumor-induced sensitivity to apoptosis in T cells from patients with renal cell carcinoma: role of nuclear factor-B suppression. Clin Cancer Res 2001;7:940–6s.
13. Raval G, Biswas S, Rayman P, et al. TNF- induction of GM2 expression on renal cell carcinomas promotes T cell dysfunction. J Immunol 2007;178:6642–52.[Abstract/Free Full Text]
14. Dall'Olio F, Chiricolo M. Sialyltransferases in cancer. Glycoconj J 2001;18:841–50.[CrossRef][Medline]
15. Black PH. Shedding from the cell surface of normal and cancer cells. Adv Cancer Res 1980;32:75–199.[Medline]
16. Ladisch S, Gillard B, Wong C, Ulsh L. Shedding and immunoregulatory activity of YAC-1 lymphoma cell gangliosides. Cancer Res 1983;43:3808–13.[Abstract/Free Full Text]
17. Ritter G, Livingston PO. Ganglioside antigens expressed by human cancer cells. Semin Cancer Biol 1991;2:401–9.[Medline]
18. Ladisch S, Kitada S, Hays EF. Gangliosides shed by tumor cells enhance tumor formation in mice. J Clin Invest 1987;79:1879–82.[Medline]
19. Birkle S, Zeng G, Gao L, Yu RK, Aubry J. Role of tumor-associated gangliosides in cancer progression. Biochimie 2003;85:455–63.[Medline]
20. Thornton MV, Kudo D, Rayman P, et al. Degradation of NF-B in T cells by gangliosides expressed on renal cell carcinomas. J Immunol 2004;172:3480–90.[Abstract/Free Full Text]
21. Schraml P, Struckmann K, Hatz F, et al. VHL mutations and their correlation with tumour cell proliferation, microvessel density, and patient prognosis in clear cell renal cell carcinoma. J Pathol 2002;196:186–93.[CrossRef][Medline]
22. Igarashi H, Esumi M, Ishida H, Okada K. Vascular endothelial growth factor overexpression is correlated with von Hippel-Lindau tumor suppressor gene inactivation in patients with sporadic renal cell carcinoma. Cancer 2002;95:47–53.[CrossRef][Medline]
23. Galban S, Fan J, Martindale JL, et al. von Hippel-Lindau protein-mediated repression of tumor necrosis factor translation revealed through use of cDNA arrays. Mol Cell Biol 2003;23:2316–28.[Abstract/Free Full Text]
24. Markotic A, Lumen R, Marusic A, Jonjic S, Muthing J. Ganglioside expression in tissues of mice lacking the tumor necrosis factor receptor. Carbohydr Res 1999;321:75–87.[CrossRef][Medline]
25. Biswas K, Richmond A, Rayman P, et al. GM2 expression in renal cell carcinoma: potential role in tumor-induced T-cell dysfunction. Cancer Res 2006;66:6816–25.[Abstract/Free Full Text]
26. Juo P, Kuo CJ, Yuan J, Blenis J. Essential requirement for caspase-8/FLICE in the initiation of the Fas-induced apoptotic cascade. Curr Biol 1998;8:1001–8.[CrossRef][Medline]
27. Ebert T, Bander NH, Finstad CL, Ramsawak RD, Old LJ. Establishment and characterization of human renal cancer and normal kidney cell lines. Cancer Res 1990;50:5531–56.[Abstract/Free Full Text]
28. Alatrash G, Hutson TE, Molto L, et al. Clinical and immunologic effects of subcutaneously administered interleukin-12 and interferon alfa-2b: phase I trial of patients with metastatic renal cell carcinoma or malignant melanoma. J Clin Oncol 2004;22:2891–900.[Abstract/Free Full Text]
29. Boucher D, Gogusev J, Droz D. [Expression of IL6 and TNF- in normal and pathological kidney. C R Seances Soc Biol Fil 1993;187:425–33.[Medline]
30. Garcia-Ruiz C, Colell A, Paris R, Fernandez-Checa JC. Direct interaction of GD3 ganglioside with mitochondria generates reactive oxygen species followed by mitochondrial permeability transition, cytochrome c release, and caspase activation. FASEB J 2000;14:847–58.[Abstract/Free Full Text]
31. Kiechle FL, Zhang X. Apoptosis: biochemical aspects and clinical implications. Clin Chim Acta 2002;326:27–45.[CrossRef][Medline]
32. Hengartner MO. The biochemistry of apoptosis. Nature 2001;407:770–6.[CrossRef]
33. Deng W, Li R, Ladisch S. Influence of cellular ganglioside depletion on tumor formation. J Natl Cancer Inst 2000;92:912–7.[Abstract/Free Full Text]
34. Gogusev J, Augusti M, Chretien Y, Droz D. Interleukin-6 and TNF production in human renal cell carcinoma. Kidney Int 1993;44:585–92.[Medline]
35. Waase I, Bergholz M, Iglauer A, et al. Heterogeneity of tumour necrosis factor production in renal cell carcinoma. Eur J Cancer 1992;28A:1660–4.[CrossRef]
36. Sonenshein GE. Rel/NF-B transcription factors and the control of apoptosis. Semin Cancer Biol 1997;8:113–9.[CrossRef][Medline]
37. Van Antwerp DJ, Martin SJ, Kafri T, Green DR, Verma IM. Suppression of TNF--induced apoptosis by NF-B. Science 1996;274:787–9.[Abstract/Free Full Text]
38. Restifo NP. Not so Fas: Re-evaluating the mechanisms of immune privilege and tumor escape. Nat Med 2000;6:493–5.[CrossRef][Medline]
39. Heitger A, Ladisch S. Gangliosides block antigen presentation by human monocytes. Biochim Biophys Acta 1996;1303:161–8.[Medline]
40. Ladisch S, Becker H, Ulsh L. Immunosuppression by human gangliosides: I. Relationship of carbohydrate structure to the inhibition of T cell responses. Biochim Biophys Acta 1992;1125:180–8.[Medline]
41. Ladisch S, Ulsh L, Gillard B, Wong C. Modulation of the immune response by gangliosides. Inhibition of adherent monocyte accessory function in vitro. J Clin Invest 1984;74:2074–81.[Medline]
42. McKallip R, Li R, Ladisch S. Tumor gangliosides inhibit the tumor-specific immune response. J Immunol 1999;163:3718–26.[Abstract/Free Full Text]
43. Valentino L, Moss T, Olson E, et al. Shed tumor gangliosides and progression of human neuroblastoma. Blood 1990;75:1564–7.[Abstract/Free Full Text]
44. Maisey NR, Hall K, Lee C, et al. Infliximab: a phase II trial of the tumor necrosis factor monoclonal antibody in patients with advanced renal cell cancer. 2004 ASCO Annual Meeting Proceedings. J Clin Oncol 2004;22:4514.
45. Harrison ML, Obermueller E, Maisey NR, et al. Tumor necrosis factor as a new target for renal cell carcinoma: two sequential phase II trials of infliximab at standard and high dose. J Clin Oncol 2007;25:4542–9.[Abstract/Free Full Text]

This article has been cited by other articles:

				S. Biswas, K. Biswas, A. Richmond, J. Ko, S. Ghosh, M. Simmons, P. Rayman, B. Rini, I. Gill, C. S. Tannenbaum, et al. Elevated Levels of Select Gangliosides in T Cells from Renal Cell Carcinoma Patients Is Associated with T Cell Dysfunction J. Immunol., October 15, 2009; 183(8): 5050 - 5058. [Abstract] [Full Text] [PDF]

				G. Sa, T. Das, C. Moon, C. M. Hilston, P. A. Rayman, B. I. Rini, C. S. Tannenbaum, and J. H. Finke GD3, an Overexpressed Tumor-Derived Ganglioside, Mediates the Apoptosis of Activated but not Resting T Cells Cancer Res., April 1, 2009; 69(7): 3095 - 3104. [Abstract] [Full Text] [PDF]

This Article Abstract Full Text (PDF) Supplementary Data Alert me when this article is cited Alert me if a correction is posted Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Das, T. Articles by Tannenbaum, C. Search for Related Content PubMed PubMed Citation Articles by Das, T. Articles by Tannenbaum, C.