Andrey Korshunov1,2,3, Felix Sahm1,2,3, Olga Zheludkova4, Andrey Golanov5, Damian Stichel1,2, Daniel Schrimpf1,2, Marina Ryzhova6, Alexander Potapov5, Antje Habel1,2, Jochen Meyer1,2, Peter Lichter3,7, David T W Jones3,8, Andreas von Deimling1,2,3, Stefan M Pfister3,8,9, Marcel Kool3,8. 1. Clinical Cooperation Unit Neuropathology (G380), German Cancer Research Center and German Cancer Consortium, Heidelberg, Germany. 2. Department of Neuropathology, Heidelberg University Hospital, Heidelberg, Germany. 3. Hopp Children's Cancer Center at the National Center for Tumor Diseases Heidelberg, Heidelberg, Germany. 4. Department of Neuro-Oncology, Russian Scientific Center of Radiology, Moscow, Russia. 5. Department of Neuroradiology, NN Burdenko Neurosurgical Institute, Moscow, Russia. 6. Department of Neuropathology, NN Burdenko Neurosurgical Institute, Moscow, Russia. 7. Division of Molecular Genetics (B060), German Cancer Research Center and German Cancer Consortium, Heidelberg, Germany. 8. Division of Pediatric Neurooncology (B062), German Cancer Research Center and German Cancer Consortium, Heidelberg, Germany. 9. Department of Pediatric Hematology and Oncology, Heidelberg University Hospital, Heidelberg, Germany.
Abstract
BACKGROUND: Wingless-activated medulloblastoma (WNT MB) represents a well-characterized molecular variant accounting for 10-15% of all MB and is associated with a favorable clinical outcome. Patients with localized WNT MBs could benefit from de-intensification of combined treatment, which would require an accurate diagnosis of these tumors. However, despite the presence of molecular features related with a WNT MB signature (nuclear ß-catenin immunoexpression, CTNNB1 mutation, and monosomy 6), a prompt and reliable diagnostic verification of these tumors is not yet feasible. METHODS: In the current study, we analyzed 78 samples of WNT MB treated in a single institute through genome-wide DNA methylation and targeted next generation sequencing to elaborate an optimal method for WNT MB molecular verification. RESULTS: We found that DNA methylation profiling discloses significant advantages for molecular diagnostic of WNT MB. All other "routine" methods applied, such as ß-catenin immunohistochemistry, CTNNB1 mutation analysis, and detection of monosomy 6, failed to identify all WNT MB cases. Survival analysis revealed that application of a reduced radiotherapy protocol for WNT MB treatment had no influence on patients' survival. Only one patient died due to local relapse but recurrent tumor was pathologically and molecularly diagnosed as a secondary glioblastoma. CONCLUSIONS: DNA methylation analysis should be considered as a method of choice for further clinically relevant stratification of WNT MB and for correct diagnosis of the recurrent tumors. WNT MB patients with localized disease could benefit from treatment de-intensification.
BACKGROUND: Wingless-activated medulloblastoma (WNT MB) represents a well-characterized molecular variant accounting for 10-15% of all MB and is associated with a favorable clinical outcome. Patients with localized WNT MBs could benefit from de-intensification of combined treatment, which would require an accurate diagnosis of these tumors. However, despite the presence of molecular features related with a WNT MB signature (nuclear ß-catenin immunoexpression, CTNNB1 mutation, and monosomy 6), a prompt and reliable diagnostic verification of these tumors is not yet feasible. METHODS: In the current study, we analyzed 78 samples of WNT MB treated in a single institute through genome-wide DNA methylation and targeted next generation sequencing to elaborate an optimal method for WNT MB molecular verification. RESULTS: We found that DNA methylation profiling discloses significant advantages for molecular diagnostic of WNT MB. All other "routine" methods applied, such as ß-catenin immunohistochemistry, CTNNB1 mutation analysis, and detection of monosomy 6, failed to identify all WNT MB cases. Survival analysis revealed that application of a reduced radiotherapy protocol for WNT MB treatment had no influence on patients' survival. Only one patient died due to local relapse but recurrent tumor was pathologically and molecularly diagnosed as a secondary glioblastoma. CONCLUSIONS: DNA methylation analysis should be considered as a method of choice for further clinically relevant stratification of WNT MB and for correct diagnosis of the recurrent tumors. WNT MB patients with localized disease could benefit from treatment de-intensification.
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