Abstracts

INTRODUCTION

Little is known about the etiology of gliomas, although they are the most common histological type of tumor in the central nervous system (CNS). Recently, it was suggested that some virus families could be important contributors towards glioma development. Viruses may contribute towards human tumor development by inducing immunosuppression, modifying host cells through inducing oncoproteins, or altering the expression of host cell proteins at viral integration sites.

Herpes viruses can infect humans easily. Te timing of infection is related to living conditions, and several members of the herpes family possess known transformational properties, notably the Epstein-Barr virus (EBV). About 90% of the world's population is estimated to be infected by EBV. Primary EBV infection is spread mainly through saliva transfer between individuals. Following primary infection, which may be either symptomatic or silent, this virus has two distinct life cycles in the human host: a lytic cycle, during which the production of new virions occurs; and a latent form, which remains in the host.¹1. Pattle SB, Farrell PJ. The role of Epstein-Barr virus in cancer. Expert Opin Biol Ther. 2006;6(11):1193-205.

EBV is associated with several human malignancies including Burkitt's lymphoma, Hodgkin's disease, nasopharyngeal carcinoma (NPC), peripheral T-cell lymphoma, thymoma and gastric cancer.²2. Weiss LM, Strickler JG, Warnke RA, Purtilo DT, Sklar J. Epstein-Barr viral DNA in tissues of Hodgkin's disease. Am J Pathol. 1987;129(1):86-91.–⁵5. de Aquino PF, Carvalho PC, da Gama Fischer JS, et al. Epstein-Barr virus DNA associated with gastric adenocarcinoma and adjacent non-cancerous mucosa in patients from Manaus, Brazil. Genet Mol Res. 2012;11(4):4442-6.

EBV has been intensely studied, not only because of its ability to cause lifelong persistent infection but also because it is causally associated with a number of diseases in the CNS (infectious mono-nucleosis, demyelinating disease, acute encephalitis, acute cerebellar ataxia, myelitis or meningitis).⁶6. Fujimoto H, Asaoka K, Imaizumi T, et al. Epstein-Barr virus infections of the central nervous system. Intern Med. 2003;42(1):33-40. EBV is thought to be responsible for a number of neurological syndromes, such as diffuse or focal encephalitis, aseptic meningitis, Guillain-Barré syndrome and peripheral neuropathy, among others.⁷7. Cleary TG, Henle W, Pickering LK. Acute cerebellar ataxia associated with Epstein-Barr virus infection. JAMA. 1980;243(2):148-9.,⁸8. Gilbert JW, Culebras A. Cerebellitis in infectious mononucleosis. JAMA. 1992;220(5):727. It has been demonstrated that astrocyte cell lines and human fetal astrocytes are the only brain cells that express complement receptor type 2 (CR2), the major cellular receptor for EBV.⁹9. Gasque P, Chan P, Mauger C, et al. Identification and characterization of complement C3 receptors on human astrocytes. J Immunol. 1996;156(6):2247-55. EBV has been found to be able to infect astrocyte cell lines.¹⁰10. Menet A, Speth C, Larcher C, et al. Epstein-Barr virus infection of human astrocyte cell lines. J Virol. 1999;73(9):7722-33. These findings together support the idea that EBV could act as an etiological agent in brain diseases.

OBJECTIVE

The aim of this study was to screen 75 primary astrocytomas for the presence of specific EBV DNA sequences, by means of the polymerase chain reaction (PCR), with confirmation using direct sequencing.

METHODS

Patients and tumor samples

Between 1997 and 2001, a total of 75 primary glioma biopsies and six others from other tumors from the CNS were obtained during surgery performed by the neurosurgery service at a cancer treatment institution in the city of Rio de Janeiro, Brazil. This work was approved by the institution's ethics board, under registration number 35/02. Te patients' participation was voluntary and their data was confidential. To confirm the participation, the volunteer signed a clear statement of informed consent, after having been informed of all aspects of the study. When the patient was underage, his/her parents were asked to sign the informed consent. Te number of patients recruited was based on the number of new registrations in the Neurosurgery Service between the years 1997 and 2001.

The tissues were immediately snap-frozen in liquid nitrogen, and subsequently stored at − 70 °C until deoxyribonucleic acid (DNA) extraction. Histological diagnoses were first made on the specimens during surgery and were later on confirmed by the pathology service of the same institution. These patients had no clinical evidence demonstrating that the tumors generated metastasis. We followed the World Health Organization (WHO) brain tumor classification.

DNA extraction

The samples were subjected to proteinase K digestion (100 mg/ml) in the presence of 0.5% SDS at 37 °C overnight. This was followed by phenol-chloroform-isoamyl alcohol (25:24:1) extraction and ethanol precipitation. Te DNA was resuspended in buffer and stored at −20 °C until molecular analysis was performed.¹¹11. Martins GA, Gattas CR, da Costa Carvalho MG. Free DNA induces modification on the protein synthesis profile of human peripheral blood mononuclear cells of healthy donors. Int J Mol Med. 2000;5(5):511-3.

Polymerase chain reaction

The PCRs were carried out in a final volume of 25 ml containing 100 ng of DNA, 1 mM of each primer, 10 mM of Tris-HCl (pH 8.3), 50 mM of KCl, 1.5 mM of MgCl₂, 200 μM of each nucleotide and 0.125 U of Taq polymerase. Te primers were selected so as to amplify a 288 bp DNA product from the EBV BamM region: CAGGCTTCCCTGCAATTTTACAAGCGG and CCCAGAAGTATACGTGGTGACGTAGA.¹²12. Saito I, Servenius B, Compton T, Fox RI. Detection of Epstein-Barr virus DNA by polymerase chain reaction in blood and tissue biopsies from patients with Sjogren's syndrome. J Exp Med. 1989;169(6):2191-8. A negative DNA– free control and a positive control from the EBV-positive Raji cell lineage were included in each assay.

Thermal cycling was performed using the following conditions: initial denaturation at 95 °C for five minutes; 40 cycles of ramping to 94 °C for one minute; cooling to 55 °C for two minutes; heating to 72 °C for one minute; and a final extension step at 72 °C for seven minutes. PCR fragments were separated by means of electrophoresis on 8% PAGE gel in 1X TBE buffer, co-migrating with a 100 bp ladder marker, and this was followed by silver staining as previously described.¹³13. Rosenbaum V, Riesner D. Temperature-gradient gel electrophoresis. Thermodynamic analysis of nucleic acids and proteins in purified form and in cellular extracts. Biophys Chem. 1987;26(2-3):235-46. As an internal control for DNA quality, we used primers to amplify exon 5 of the tumor suppressor gene TP53: GCAACCAGCCCTGTCGTGTCTCCA and GAATTCTGTTCACTTGTGCCCTGACTTTCAAC.¹⁴14. Pestaner JP, Bibbo M, Bobroski L, Seshamma T, Bagasra O. Potential of the in situ polymerase chain reaction in diagnostic cytology. Acta Cytol. 1994;38(5):676-80. All the samples analyzed for the presence of EBV amplified the suppressor gene TP53.

Sequencing reaction

The PCR product was purified using the GFX PCR DNA gel band purification kit (GE Healthcare Biosciences, Buckinghamshire, UK), in accordance with the manufacturer's instructions, and this was used for direct sequencing in an ABI 3130 device (Life Technologies, CA, USA). Te alignments were obtained through the GenBank online Blast-N sofware, which is available from the National Center for Biotechnology Information (http://www.ncbi.nlm.nih.gov).

RESULTS

The glioma specimens were classified as astrocytoma grade I (7/75), astrocytoma grade II (25/75), astrocytoma grade III (16/75), glioblastoma multiforme (18/75), ependymoma (5/75), oligodendroglioma (2/75) and oligoastrocytoma (2/75). These tumors were from 40 males and 35 females; 25 patients were children (under 21 years of age) and 50 were adults. Te location of the tumors in the brain was variable: temporal lobe, fourth ventricle, thalamus, cerebellar vermis, brain stem, cerebral ventricle, supra tentorial, occipital lobe and parietal lobe.

The DNA extracted from the gliomas was screened for the presence of EBV DNA. Te result was positive in 11/75 (14.7%) of the tumor specimens. Te tumors positive for EBV DNA were: astrocytoma grade II (6/11); astrocytoma grade III (2/11); oli-goastrocytoma (1/11); ependymoma (1/11); and glioblastoma multiforme (1/11) (Table 1).

Figure 1 shows a gel containing positive PCR reactions. Additionally, the presence of EBV DNA was also screened for in other CNS tumors (one neurilemma, two non-Hodgkin lymphomas, two pituitary adenomas and one cortical dysplasia) and they were all negative for EBV DNA.

The homology between the EBV sequences found in the astrocytoma patients was compared with the published EBV sequence, by examining their similarity. The identicalness rate observed (95.5%) confirmed that the virus found was EBV.

DISCUSSION

Over the past decade, several groups have examined the evidence for the presence and expression of viruses in CNS tumors and have analyzed the quantity of viral material. Reports on SV40 (simian virus 40), JCV (John Cunningham virus) and HCMV (human cytomegalovirus) have been made, with diverse findings.¹⁵15. Kouhata T, Fukuyama K, Hagihara N, Tabushi K. Detection of simian virus 40 DNA sequence in human primary glioblastomas multiforme. J Neurosurg. 2001;95(1):96-101.–²⁴24. Fonseca RF, Kawamura MT, Oliveira JA, et al. The prevalence of human cytomegalovirus DNA in gliomas of Brazilian patients. Mem Inst Oswaldo Cruz. 2012;107(7):953-4. More recently, JCV and HCMV have been accepted as being associated with CNS tumors.²⁵25. Alibek K, Kakpenova A, Baiken Y. Role of infectious agents in the carcinogenesis of brain and head and neck cancers. Infect Agent Cancer. 2013;8(1):7. Discordant findings may occur because of the sensitivity of the PCR/in situ techniques used, difficulty in working with paraffin-embedded tissues and also small numbers of samples. In the present study, it is important to note that we used 75 fresh frozen tissue samples and conventional PCR, which has the advantage of amplifying small target sequences. In this study, in order to search for EBV DNA in different histological types/grades (Table 1), we used the simple method of conventional PCR, which had been used in previous work.¹²12. Saito I, Servenius B, Compton T, Fox RI. Detection of Epstein-Barr virus DNA by polymerase chain reaction in blood and tissue biopsies from patients with Sjogren's syndrome. J Exp Med. 1989;169(6):2191-8. Te prevalence of EBV DNA found was 11/75 (14.7%).

Figure 1
Silver-stained 8% PAGE gel showing examples of polymerase chain reaction (PCR) products from the Epstein-Barr virus (EBV), from glioma biopsies.

There is evidence showing that EBV emerges from latency in immunosuppressed individuals. Many cancer patients present immunosuppression, which may be caused by aging, by the disease itself or even by medications, and EBV and other silent viruses may be activated in this manner.²⁶26. Martelius T, Lappalainen M, Palomäki M, Anttila VJ. Clinical characteristics of patients with Epstein Barr virus in cerebrospinal fluid. BMC Infect Dis. 2011;11:281.,²⁷27. Kleinschmidt-DeMasters BK, Damek DM, Lillehei KO, Dogan A, Giannini C. Epstein Barr virus-associated primary CNS lymphomas in elderly patients on immunosuppressive medications. J Neuropathol Exp Neurol. 2008;67(11):1103-11. Te EBV genome is complex and comprises at least 12 known genes; however, the most famous EBV transforming protein is LMP1 (latent-infection membrane protein 1).²⁸28. Kaye KM, Izumi KM, Kief E. Epstein-Barr virus latent membrane protein 1 is essential for B-lymphocyte growth transformation. Proc Natl Acad Sci U S A. 1993;90(19):9150-4 In spite of all of this knowledge, the role of EBV in glioma tumorigenesis is still not understood.

An EBV vaccine has been tested (in a phase I clinical trial) on Chinese nasopharyngeal carcinoma patients to determine the safe and immunogenic dose.²⁹29. Hui EP, Taylor GS, Jia H, et al. Phase I trial of recombinant modified vaccinia ankara encoding Epstein-Barr viral tumor antigens in nasopharyngeal carcinoma patients. Cancer Res. 2013;73(6):1676-88. In that study, it was concluded that the vaccine is both safe and immunogenic, thus allowing the highest dose to be moved forward to phase II studies. From our data, it is possible that in the future, in the same way as seen among those nasopharyngeal carcinoma patients, tests using an EBV vaccine may be found to benefit glioma patients.

CONCLUSION

The prevalence of EBV DNA was 11/75 (14.7%) in our glioma samples. Further molecular and epidemiological studies are needed in order to establish the possible role played by EBV in the tumorigenesis of gliomas.

Acknowledgements

We thank Marcelo Soares Mota for technical assistance and all members of the Neurosurgery Service (INCA)

REFERENCES

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