Proof-of-Concept for Liquid Biopsy Disease Monitoring of MYC-Amplified Group 3 Medulloblastoma by Droplet Digital PCR

Author:

Stepien Natalia1ORCID,Senfter Daniel1,Furtner Julia23,Haberler Christine4ORCID,Dorfer Christian5ORCID,Czech Thomas5ORCID,Lötsch-Gojo Daniela5,Mayr Lisa1ORCID,Hedrich Cora1,Baumgartner Alicia1ORCID,Aliotti-Lippolis Maria1,Schned Hannah1,Holler Johannes1,Bruckner Katharina1ORCID,Slavc Irene1ORCID,Azizi Amedeo A.1ORCID,Peyrl Andreas1ORCID,Müllauer Leonhard6ORCID,Madlener Sibylle1,Gojo Johannes1ORCID

Affiliation:

1. Department of Pediatrics and Adolescent Medicine, Comprehensive Center for Pediatrics and Comprehensive Cancer Center, Medical University of Vienna, 1090 Vienna, Austria

2. Division of Neuroradiology and Musculoskeletal Radiology, Department of Biomedical Imaging and Image-Guided Therapy, Medical University of Vienna, 1090 Vienna, Austria

3. Research Center for Medical Image Analysis and Artificial Intelligence (MIAAI), Faculty of Medicine and Dentistry, Danube Private University, 3500 Krems-Stein, Austria

4. Division of Neuropathology and Neurochemistry, Department of Neurology, Medical University of Vienna, 1090 Vienna, Austria

5. Department of Neurosurgery, Medical University of Vienna, 1090 Vienna, Austria

6. Department of Pathology, Medical University of Vienna, 1090 Vienna, Austria

Abstract

Background: Liquid biopsy diagnostic methods are an emerging complementary tool to imaging and pathology techniques across various cancer types. However, there is still no established method for the detection of molecular alterations and disease monitoring in MB, the most common malignant CNS tumor in the pediatric population. In the presented study, we investigated droplet digital polymerase chain reaction (ddPCR) as a highly sensitive method for the detection of MYC amplification in bodily fluids of group 3 MB patients. Methods: We identified a cohort of five MYC-amplified MBs by methylation array and FISH. Predesigned and wet-lab validated probes for ddPCR were used to establish the detection method and were validated in two MYC-amplified MB cell lines as well as tumor tissue of the MYC-amplified cohort. Finally, a total of 49 longitudinal CSF samples were analyzed at multiple timepoints during the course of the disease. Results: Detection of MYC amplification by ddPCR in CSF showed a sensitivity and specificity of 90% and 100%, respectively. We observed a steep increase in amplification rate (AR) at disease progression in 3/5 cases. ddPCR was proven to be more sensitive than cytology for the detection of residual disease. In contrast to CSF, MYC amplification was not detectable by ddPCR in blood samples. Conclusions: ddPCR proves to be a sensitive and specific method for the detection of MYC amplification in the CSF of MB patients. These results warrant implementation of liquid biopsy in future prospective clinical trials to validate the potential for improved diagnosis, disease staging and monitoring.

Funder

Oncomine Clinical Research Grant 2020

“FWF der Wissenschaftsfonds”

OeNB Jubiläumsfonds

Physician Researcher Pathway Scholarships of the Medical University of Vienna

“Medizinisch-Wissenschaftlichen Fonds des Bürgermeisters der Bundeshauptstadt Wien”

CCP Starter Grant 2020

“Verein unser_kind”

”Forschungsgesellschaft für Cerebrale Tumore”

Publisher

MDPI AG

Subject

Cancer Research,Oncology

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