1. MGMT methylation in diffuse large B-cell lymphoma: validation of quantitative methylation-specific PCR and comparison with MGMT protein expression
- Author
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Silvia Uccella, Claudia Placidi, Carlo Capella, Roberta Cerutti, Barbara Bernasconi, Ileana Carnevali, Graziella Pinotti, Maria Grazia Tibiletti, Daniela Furlan, Ilaria Proserpio, and Silvia Marchet
- Subjects
Adult ,Male ,Methyltransferase ,Bisulfite sequencing ,Biology ,Polymerase Chain Reaction ,Pathology and Forensic Medicine ,hemic and lymphatic diseases ,Biomarkers, Tumor ,medicine ,Humans ,Progression-free survival ,DNA Modification Methylases ,neoplasms ,In Situ Hybridization, Fluorescence ,Aged ,Neoplasm Staging ,Aged, 80 and over ,Chromosomes, Human, Pair 10 ,Tumor Suppressor Proteins ,DNA, Neoplasm ,General Medicine ,Methylation ,DNA Methylation ,Middle Aged ,medicine.disease ,Survival Analysis ,Molecular biology ,digestive system diseases ,Neoplasm Proteins ,DNA Repair Enzymes ,Real-time polymerase chain reaction ,DNA methylation ,Cancer research ,Immunohistochemistry ,Female ,Lymphoma, Large B-Cell, Diffuse ,Diffuse large B-cell lymphoma - Abstract
Aims: (1) To validate a quantitative real time methylation specific PCR assay (MethyLight) for the detection of O 6 -methylguanine-DNA methyltransferase (MGMT) gene methylation status (MS) in diffuse large B-cell lymphoma (DLBCL). (2) To determine the immunohistochemical (IHC) expression of the MGMT protein and correlate it with MS. Both IHC and MethyLight results were compared with patient’s outcome. Methods: 71 patients with primary nodal DLBCL were studied. MGMT immunoreactivity was detected using a specific monoclonal antibody. The MS of MGMT gene was analysed in 52/71 DLBCL using MethyLight. A selected subset of 40 DLBCL was also analysed using qualitative methylation-specific PCR (MSP). Statistical analysis of overall survival (OS), lymphoma-specific survival (LSS) and progression free survival (PFS) was performed according to IHC and MS results. Results: 19/71 DLBCLs (27%) were MGMT-negative at IHC; all were analysed, together with 33/52 MGMT-positive DLBCLs. MethyLight showed a better performance than MSP. There was a good correlation between the presence of MGMT expression and the unmethylated status; the absence of IHC expression was poorly correlated with the presence of methylation. Better OS, LSS and PFS was found in DLBCLs with MGMT gene methylation. DLBCLs not expressing MGMT at IHC showed a longer PFS. Conclusions: The quantitative real-time methylation-specific PCR assay for the detection of MGMT gene hypermethylation has been validated for the first time in DLBCL. Immunohistochemistry seems to represent an useful preliminary test to identify unmethylated cases; MS analysis may be performed in non-immunoreactive cases to identify truly methylated DLBCLs, which bear a better prognosis.
- Published
- 2009
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