Abstract
Cancer-germline genes (CGGs) code for immunogenic antigens that are present in various human tumors and can be targeted by immunotherapy. Their expression has been studied in a wide range of human tumors in adults. We measured the expression of 12 CGGs in pediatric brain tumors, to identify targets for therapeutic cancer vaccines. Real Time PCR was used to quantify the expression of genes MAGE-A1, MAGE-A2, MAGE-A3, MAGE-A4, MAGE-A6, MAGE-A10, MAGE-A12, MAGE-C2, NY-ESO-1 and GAGE-1,2,8 in 50 pediatric brain tumors of different histological subtypes. Protein expression was examined with immunohistochemistry. Fifty-five percent of the medulloblastomas (n = 11), 86% of the ependymomas (n = 7), 40% of the choroid plexus tumors (n = 5) and 67% of astrocytic tumors (n = 27) expressed one or more CGGs. Immunohistochemical analysis confirmed qPCR results. With exception of a minority of tumors, the overall level of CGG expression in pediatric brain tumors was low. We observed a high expression of at least one CGG in 32% of the samples. CGG-encoded antigens are therefore suitable targets in a very selected group of pediatric patients with a brain tumor. Interestingly, glioblastomas from adult patients expressed CGGs more often and at significantly higher levels compared to pediatric glioblastomas. This observation is in line with the notion that pediatric and adult glioblastomas develop along different genetic pathways.
Similar content being viewed by others
Avoid common mistakes on your manuscript.
Introduction
Despite major advances in the treatment of childhood cancer, cancer remains a common cause of death for children >1 year of age [1]. Twenty-two percent of all pediatric cancers are CNS tumors. Pediatric patients with relapsed cancers of the CNS have a poor prognosis, and therefore novel therapies for these patients are urgently needed. Immunotherapy against brain tumors presents unique challenges since the brain is considered an immune privileged site. However, recent studies demonstrated that the immune cells have access to the brain in spite of the blood-brain barrier [2, 3]. Within malignant brain tumors the blood-brain barrier is generally considered non-functional. Progress in our understanding of immune responses to CNS tumors have already led to novel clinical applications [4, 5]. Most experience has been obtained with immunotherapeutic trials with dendritic cell vaccinations, as reviewed by De Vleeschouwer et al. [6].
Immunotherapy is an attractive therapeutic option for pediatric cancer patients because of its mild toxicity, and because the child’s immune system is more potent and flexible compared to adults [7, 8]. However, implementation of immunotherapy in pediatric oncology has been hampered by the lack of known tumor-specific antigens on pediatric tumors.
Cancer-germline genes (CGGs) are expressed in a wide range of human tumors and have a highly restricted expression pattern in normal tissues [9, 10]. Antigens encoded by CGGs have been extensively studied because of their immunogenicity, tumor specificity, and their expression in a significant proportion of adult tumors of various histological types. Recently, we have shown that CGGs are expressed in a large percentage of pediatric extra-cranial solid tumors [11].
The aim of this study was to analyze CGG expression in pediatric brain tumors. We report the results of a quantitative real-time PCR analysis of the expression of 12 CGGs in a panel of medulloblastomas, ependymomas, tumors of the choroid plexus and astrocytic tumors.
Materials and methods
Tumor samples
Fresh-frozen tumor samples were available at the Department of Pathology at the Radboud University Nijmegen Medical Centre. All samples were from pediatric patients (0–19-years-old) with a brain tumor diagnosed at the Department of Pediatric Hemato-Oncology. Sections of the frozen samples were stained with hematoxylin-eosin and reviewed by the pathologist to verify tumor histology and to evaluate the percentage of tumor cells. Samples were only considered for study if the contents of tumor cells was ≥80%.
RNA isolation and cDNA synthesis
Total RNA was isolated with TriZol reagent (Invitrogen, Carlsbad, CA) and samples were treated with Deoxyribonuclease I (Invitrogen) according to the manufacturer’s protocol. To generate cDNA, 1 μg DNase-treated RNA was reverse-transcribed with the SuperScript First-Strand Synthesis System for RT-PCR (Invitrogen) using oligo(dT) primer and 50 units SuperScript II, according to the manufacturer’s protocol. After first-strand synthesis, samples were diluted to a final volume of 100 μl with water.
Conventional PCR
Duplex PCR amplification of β-actin and GAPDH transcripts was carried out in a 25-μl reaction volume containing 2.5 μl of cDNA, 1× PCR Buffer (10 mM Tris–HCl pH 8.3, 50 mM KCl, 1.5 mM MgCl2), 100 μM each dNTP, 0.4 μM each primer, and 0.625 units Taq DNA polymerase (TaKaRa, Shiga, Japan). β-actin primers were as described [12]. GAPDH primers (originally available from Clontech, Palo Alto, CA; kindly provided by Dr. B. Lethé) were 5′-TgAAggTCggAgTCAACggATTTggT-3′ (sense) and 5′-CATgTgggCCATgAggTCCACCAC-3′ (antisense). Cycling was performed in a TRIO-Thermoblock thermocycler (Biometra, Göttingen, Germany) as follows: 94°C for 4 min, followed by 22 cycles of 1 min at 94°C, 1 min at 65°C, and 1 min at 72°C. Cycling was concluded with a final extension step at 72°C for 15 min. PCR products were fractionated in 1.3% agarose gel and visualized by ethidium bromide fluorescence (β-actin, 626 bp; GAPDH, 983 bp). PCR amplification of MAGE-A transcripts was carried out with the primer pair designed by Zammatteo et al. [13]. These primers derive from a consensus nucleotide sequence for the last exon of the 12 MAGE-A genes and give amplicons of ~539 bp. PCR conditions were as described above, except that PCR was performed for 30 cycles.
Quantitative real-time PCR
Expression of CGGs and of the reference gene β-actin, was measured by quantitative PCR, based on TaqMan methodology, using the ABI PRISM 7700 Sequence Detection System (Applied Biosystems, Warrington, UK). PCR reactions were prepared with the qPCR Core Kit w/o dUTP reagents (Eurogentec, Seraing, Belgium). Each reaction (25 μl) contained 2.5 μl of cDNA, 1× PCR buffer containing the passive reference dye ROX, 5 mM MgCl2, 200 μM each dNTP, 200 nM each primer, 100 nM probe, and 0.625 units DNA polymerase. Primers, probes and thermal cycling conditions are given in Table 1 [14, 15]. Probes with 6FAM and TAMRA labels were from Eurogentec. Probes with 6FAM and MGB-NFQ labels (for MAGE-A3, MAGE-A6 and MAGE-A12) were from Applied Biosystems. Quantification of the samples was achieved by extrapolation from a standard curve of serial dilution points of cDNA of the relevant gene (Supplementary Figure 1). Samples and standard dilution points were assayed in duplicate or triplicate. Standard calibration curves for β-actin and all CGGs were linear over 4 (CGGs) or 5 (ß-actin) orders of magnitude and had similar PCR efficiencies (slope from −3.45 to −3.77). Differences in sensitivity between the assays for the various genes (y-intercept from 38.7 to 41.6) were due in part to differences in the actual cDNA copy number in the standard dilutions. cDNA copy numbers in the standards were verified by testing minimally 12 replicates of the 1-copy dilution in each qPCR run. If needed, copy numbers of the test samples were corrected by a factor calculated on the basis of the results for the 1-copy dilution. Normalization of samples was achieved by dividing the copy number of CGG by that of the reference gene, β-actin.
Immunohistochemistry
Immunochemistry was performed on 4 μm tissue sections of formalin-fixed paraffin-embedded tissue blocks. Sections were heated for 20 min in citrate buffer (10 mM, pH 6.0) for antigen retrieval. The following mouse IgG1 monoclonal antibodies (mAb) were used: E978 (anti-NY-ESO-1) [16] (Zymed, San Francisco, CA), MA454 (anti-MAGE-A1) [17] (Zymed, San Francisco, CA), and 57B (anti-MAGE-A4) [18, 19] (kindly provided by Dr. G.C. Spagnoli, University Hospital Basel, Switzerland). Testis tissue with intact spermatogenesis was used as positive control. Tissue sections were incubated with mAb diluted in PBA: E978 (2.5 μg/ml), MA454 (1 μg/ml), or 57B (5 μg/ml), or with IgG1 negative control antibody, at room temperature for 1 h. Binding sites of primary antibodies were then detected by a biotinylated horse-antimouse secondary reagent (Vector Laboratories, Burlingame, CA) followed by an avidin–biotin complex system (ABC Elite, Vector Laboratories). Diaminobenzidine tetrachloride served as a chromogen. Immunoreactivity was assessed blindly with respect to the mAb used.
Statistical analysis
Normalized CGG values are presented as means ± standard deviation (SD). The SD of the normalized CGG values was calculated from the SD of the CGG and the β-actin values using the following formula: CV = SQRT [CV2 β-actin + CV 2CGG ], where CV = SD/mean value (as described in the Sequence Detection System User Bulletin 2, 1997, Applied Biosystems). Differences in mRNA expression levels between pediatric and adult glioblastomas are calculated with the Spearman rank correlation. All statistical tests were two-sided, significance was determined as P < 0.05.
Results
Study population
We analyzed cancer-germline gene (CGG) expression in 50 fresh-frozen tumors by reverse transcription and polymerase chain reaction (PCR) amplification. All samples were histologically proven brain tumors from pediatric patients, ≤19-years old at the time of tumor resection and classified according to the WHO 2007 classification [20] (Table 2). An extra-cohort of nine glioblastoma samples from adult patients was also analyzed, for comparison to pediatric glioblastoma. Integrity of cDNA samples was verified by conventional, 22-cycle PCR amplification of a 626 bp β-actin and a 983 bp GAPDH product (data not shown). Samples were subjected to conventional PCR amplification with consensus primers for the 12 genes of the MAGE-A family. Twenty-seven samples were positive, indicating that, depending on the tumor type, 33–64% of the investigated pediatric tumors expressed at least one MAGE-A gene (Table 2).
CGG expression in pediatric brain tumors
The 27 MAGE-A-positive samples were subsequently analyzed by quantitative real-time PCR (qPCR), using the TaqMan methodology, to measure the expression of the individual MAGE genes, MAGE-A1, A2, A3, A4, A6, A10, and A12. In addition, all 50 samples were tested by qPCR for expression of genes MAGE-C2, NY-ESO-1 and GAGE-1,2,8 (Table 2). CGG expression levels were normalized to those of the β-actin gene (Fig. 1).
Medulloblastoma. Six of the 11 medulloblastoma tumors expressed at least 1 of the 10 CGGs that were analyzed. The expression of CGGs in medulloblastomas was highly clustered (Table 3). One sample expressed high levels (CGG/ß-actin ratios > 10−2) of 6 CGG genes. The other medulloblastoma samples only sporadically expressed CGGs, with CGG/ß-actin ratios above 10−4.
Ependymoma. Six out of seven ependymoma samples expressed at least 1 CGG. None expressed more than 3. Here the expression was therefore not clustered. Most positive samples expressed NY-ESO-1 and/or GAGE-1,2,8. The overall levels of CGG expression in ependymoma samples were low, with CGG/β-actin ratios below 1 × 10−3.
Choroid plexus tumor. Of the five choroid plexus tumors analyzed, three showed no detectable CGG expression. Samples #1 and #2 expressed at least three CGGs. Only in one sample the CGG/β-actin ratio exceeded 1 × 10−3.
Pilocytic astrocytoma. Nine out of 14 pilocytic astrocytomas expressed at least one CGG. The overall expression was low, one low pilocytic astrocytoma had a CGG/β-actin ratio >1 × 10−4.
Diffuse astrocytoma. Two out of three diffuse astrocytomas expressed at least one CGG. The overall expression level of CGGs on diffuse astrocytomas was low.
High grade astrocytoma. Eight out of 10 anaplastic astrocytomas and glioblastomas expressed at least one CGG. CGG/β-actin ratio in high grade astrocytomas did not exceed 1 × 10−3.
CGG expression in pediatric versus adult glioblastomas
The relatively low expression of MAGE genes in high grade astrocytomas was unexpected since MAGE expression has been reported in almost all adult glioblastomas [21]. In these studies different methods were used, immunohistochemistry [21–24] and conventional, non-quantitative PCR [22–24]. Therefore we decided to select nine new adult glioblastoma samples for MAGE qPCR analysis. All samples expressed at least five MAGE-A genes at high levels. The difference between the levels of MAGE-A genes expression in pediatric versus adult glioblastomas is shown in Fig. 2 (P = 6.1 × 10−6).
Cancer-germline protein distribution
Immunohistochemistry with monoclonal antibodies (mAbs) E978 (anti-NY-ESO–1), MA454 (anti-MAGE-A1) and 57B (anti-MAGE-A4) was performed on available paraffin-embedded tissues. Sections from normal testis tissue were used as positive controls. The intensity of the stainings correlated well with the level of CGG expression, as shown in Fig. 3a, b. The MAGE-A1, MAGE-A4 and NY-ESO-1 proteins were distributed homogenously throughout the tissues. However, a minority of the tissues had a heterogeneous staining pattern such as the MAGE-A4 expression in medulloblastoma sample #1 (Fig. 3c). No staining could be observed for samples that scored either negative or with CGG/β-actin ratios below 10−4.
CGG expression and tumor stage
The number of patients in each specific group of tumors was too small to try to establish a correlation between CGG expression and clinicopathological parameters. Stratification of the pediatric astrocytic tumors in pilocytic astrocytoma (grade I), diffuse astrocytoma (grade II) and high grade anaplastic astrocytomas and glioblastomas (grade III and IV, respectively), revealed that the level of CGG expression was not significantly different between groups. These data suggest that CGG expression in astrocytic tumors is not correlated with the grade of the astrocytic tumor in pediatric patients.
Discussion
Antibodies and T cells can be identified that recognize antigenic fragments derived from gene products expressed by tumors [10, 25, 26]. A critical role for these anti-tumor immune mechanisms in the eradication of cancer has been demonstrated in numerous animal models and some clinical trials [27, 28]. In the last decennia promising new strategies for the development of antibodies and activated T cells against tumor associated antigens have been developed [29, 30]. In spite of the blood brain barrier, there is accumulating evidence that even brain tumors can cause immune activation and are amenable for immunotherapy [2, 4, 31].
The identification of immunogenic tumor associated antigens is an essential step in the development of rational cancer vaccines. The potential of CGGs as vaccine targets has led to detailed studies of their expression in various malignancies in adult patients [10, 32]. Previously, we reported on the expression of CGGs in pediatric extra-cranial tumors [11]. Here we report that, in our cohort of 50 pediatric brain tumors, 68% expressed one or more CGGs. Immunohistochemical data correlated well with the qPCR results. Apart from a few exceptions, the overall level of CGG expression on pediatric brain tumors is low. Preliminary data from cytotoxicity assays indicated that glioblastoma cell lines that express low levels of CGGs (CGG/β-actin ratio < 1 × 10−4) are not specifically lysed by HLA-matched anti-MAGE A3 CTL cell lines (data not shown).
In contrast to the limited CGG expression found in pediatric brain tumors, glioblastomas from adult patients express significantly higher levels of CGGs (P < 0,001). This finding is in line with reported differences between adult and pediatric glioblastomas in p53 and EGFR expression [33, 34]. The differences in protein expression may be explained by chromosomal aberrations and differences in microsatellite stability between adult glioblastomas and pediatric glioblastomas [35, 36]. The significant difference in MAGE-A expression between adult and pediatric glioblastomas supports the view that these tumors develop along distinct genetic pathways.
In conclusion, we report limited CGG expression in pediatric brain tumors. Only a small percentage of brain tumors express high levels of CGGs. These data indicate that CGGs can only be used as immune target in a selected group of pediatric brain tumors.
References
Linet MS, Ries LA, Smith MA et al (1999) Cancer surveillance series: recent trends in childhood cancer incidence and mortality in the United States. J Natl Cancer Inst 91:1051–1058
Ransohoff RM, Kivisakk P, Kidd G (2003) Three or more routes for leukocyte migration into the central nervous system. Nat Rev Immunol 3:569–581
Galea I, Bernardes-Silva M, Forse PA et al (2007) An antigen-specific pathway for CD8 T cells across the blood-brain barrier. J Exp Med 204:2023–2030
Lampson LA (2003) Brain tumor immunotherapy: an immunologist’s perspective. J Neurooncol 64:3–11
Khan-Farooqi HR, Prins RM, Liau LM (2005) Tumor immunology, immunomics and targeted immunotherapy for central nervous system malignancies. Neurol Res 27:692–702
de Vleeschouwer S, Rapp M, Sorg RV et al (2006) Dendritic cell vaccination in patients with malignant gliomas: current status and future directions. Neurosurgery 59:988–999 discussion 99–1000
Mackall CL, Fleisher TA, Brown MR et al (1995) Age, thymopoiesis, and CD4 + T-lymphocyte regeneration after intensive chemotherapy. N Engl J Med 332:143–149
Heitger A, Greinix H, Mannhalter C et al (2000) Requirement of residual thymus to restore normal T-cell subsets after human allogeneic bone marrow transplantation. Transplantation 69:2366–2373
van der Bruggen P, Traversari C, Chomez P et al (1991) A gene encoding an antigen recognized by cytolytic T lymphocytes on a human melanoma. Science 254:1643–1647
Van Der Bruggen P, Zhang Y, Chaux P et al (2002) Tumor-specific shared antigenic peptides recognized by human T cells. Immunol Rev 188:51–64
Jacobs JF, Brasseur F, Hulsbergen-van de Kaa CA et al (2007) Cancer-germline gene expression in pediatric solid tumors using quantitative real-time PCR. Int J Cancer 120:67–74
Raff T, van der Giet M, Endemann D et al (1997) Design and testing of beta-actin primers for RT-PCR that do not co-amplify processed pseudogenes. Biotechniques 23:456–460
Zammatteo N, Lockman L, Brasseur F et al (2002) DNA microarray to monitor the expression of MAGE-A genes. Clin Chem 48:25–34
So T, Hanagiri T, Chapiro J et al (2007) Lack of tumor recognition by cytolytic T lymphocyte clones recognizing peptide 195–203 encoded by gene MAGE-A3 and presented by HLA-A24 molecules. Cancer Immunol Immunother 56:259–269
Kholmanskikh O, Loriot A, Brasseur F et al (2008) Expression of BORIS in melanoma: lack of association with MAGE-A1 activation. Int J Cancer 122:777–784
Jungbluth AA, Chen YT, Stockert E et al (2001) Immunohistochemical analysis of NY-ESO-1 antigen in normal and malignant human tissues. Int J Cancer 92:856–860
Chen YT, Stockert E, Chen Y et al (1994) Identification of the MAGE-1 gene product by monoclonal and polyclonal antibodies. Proc Natl Acad Sci USA 91:1004–1008
Kocher T, Schultz-Thater E, Gudat F et al (1995) Identification and intracellular location of MAGE-3 gene product. Cancer Res 55:2236–2239
Landry C, Brasseur F, Spagnoli GC et al (2000) Monoclonal antibody 57B stains tumor tissues that express gene MAGE-A4. Int J Cancer 86:835–841
Louis DN, Ohgaki H, Wiestler OD et al (2007) The 2007 WHO classification of tumours of the central nervous system. Acta Neuropathol (Berl) 114:97–109
Bodey B, Siegel SE, Kaiser HE (2002) MAGE–1, a cancer/testis-antigen, expression in childhood astrocytomas as an indicator of tumor progression. In Vivo 16:583–588
Rimoldi D, Romero P, Carrel S (1993) The human melanoma antigen-encoding gene, MAGE-1, is expressed by other tumour cells of neuroectodermal origin such as glioblastomas and neuroblastomas. Int J Cancer 54:527–528
Chi DD, Merchant RE, Rand R et al (1997) Molecular detection of tumor-associated antigens shared by human cutaneous melanomas and gliomas. Am J Pathol 150:2143–2152
Sahin U, Koslowski M, Tureci O et al (2000) Expression of cancer testis genes in human brain tumors. Clin Cancer Res 6:3916–3922
Velders MP, Markiewicz MA, Eiben GL et al (2003) CD4+ T cell matters in tumor immunity. Int Rev Immunol 22:113–140
Kershaw MH, Trapani JA, Smyth MJ (1995) Cytotoxic lymphocytes: redirecting the cell-mediated immune response for the therapy of cancer. Ther Immunol 2:173–181
Boon T, Cerottini JC, Van den Eynde B et al (1994) Tumor antigens recognized by T lymphocytes. Annu Rev Immunol 12:337–365
Rosenberg SA (2001) Progress in human tumour immunology and immunotherapy. Nature 411:380–384
Kalos M (2003) Tumor antigen-specific T cells and cancer immunotherapy: current issues and future prospects. Vaccine 21:781–786
Sinkovics JG, Horvath JC (2000) Vaccination against human cancers (review). Int J Oncol 16:81–96
Bodey B, Bodey B Jr, Siegel SE (1995) Immunophenotypic characterization of infiltrating polynuclear and mononuclear cells in childhood brain tumors. Mod Pathol 8:333–338
Simpson AJ, Caballero OL, Jungbluth A et al (2005) Cancer/testis antigens, gametogenesis and cancer. Nat Rev Cancer 5:615–625
Litofsky NS, Hinton D, Raffel C (1994) The lack of a role for p53 in astrocytomas in pediatric patients. Neurosurgery 34:967–972 discussion 72–73
Sure U, Ruedi D, Tachibana O et al (1997) Determination of p53 mutations, EGFR overexpression, and loss of p16 expression in pediatric glioblastomas. J Neuropathol Exp Neurol 56:782–789
Rickert CH, Strater R, Kaatsch P et al (2001) Pediatric high-grade astrocytomas show chromosomal imbalances distinct from adult cases. Am J Pathol 158:1525–1532
Szybka M, Bartkowiak J, Zakrzewski K et al (2003) Microsatellite instability and expression of DNA mismatch repair genes in malignant astrocytic tumors from adult and pediatric patients. Clin Neuropathol 22:180–186
Acknowledgements
The authors wish to thank Dr. B. Lethé for providing the reagents for LAGE-2/NY-ESO, GAGE-1,2,8 and ACTB quantitative PCR. Dr. E. De Plaen for the reagents for MAGEA2 and MAGEA12 quantitative PCR. Riki Willems for assistance with the pathology database. Thérèse Aerts and Madeleine Swinarska for technical assistance. This work was supported by grants from “The Quality of Life Gala” and “Stichting Vrienden van het Kinderoncologisch Centrum Zuid-Oost Nederland”.
Open Access
This article is distributed under the terms of the Creative Commons Attribution Noncommercial License which permits any noncommercial use, distribution, and reproduction in any medium, provided the original author(s) and source are credited.
Author information
Authors and Affiliations
Corresponding author
Electronic Supplementary Material
Rights and permissions
Open Access This is an open access article distributed under the terms of the Creative Commons Attribution Noncommercial License (https://creativecommons.org/licenses/by-nc/2.0), which permits any noncommercial use, distribution, and reproduction in any medium, provided the original author(s) and source are credited.
About this article
Cite this article
Jacobs, J.F.M., Grauer, O.M., Brasseur, F. et al. Selective cancer-germline gene expression in pediatric brain tumors. J Neurooncol 88, 273–280 (2008). https://doi.org/10.1007/s11060-008-9577-6
Received:
Accepted:
Published:
Issue Date:
DOI: https://doi.org/10.1007/s11060-008-9577-6