Overcoming the Challenges of High Quality RNA Extraction from Core Needle Biopsy
Hanne Locy,
Rohann J.M. Correa,
Dorien Autaers,
Ann Schiettecatte,
Jan Jonckheere,
Wim Waelput,
Louise Cras,
Stefanie Brock,
Stefaan Verhulst,
Keith Kwan,
Marian Vanhoeij,
Kris Thielemans,
Karine Breckpot
Affiliations
Hanne Locy
Laboratory for Molecular and Cellular Therapy, Department of Biomedical Sciences, Vrije Universiteit Brussel (VUB), Laarbeeklaan 103/E, B-1090 Brussels, Belgium
Rohann J.M. Correa
Department of Radiation Oncology, London Regional Cancer Program, London Health Sciences Centre, 800 Commisioners Road East, London, ON N6A 4G5, Canada
Dorien Autaers
Laboratory for Molecular and Cellular Therapy, Department of Biomedical Sciences, Vrije Universiteit Brussel (VUB), Laarbeeklaan 103/E, B-1090 Brussels, Belgium
Ann Schiettecatte
Department of Radiology, Universitair Ziekenhuis Brussel (UZ Brussel), Laarbeeklaan 101, B-1090 Brussels, Belgium
Jan Jonckheere
Department of Radiology, Universitair Ziekenhuis Brussel (UZ Brussel), Laarbeeklaan 101, B-1090 Brussels, Belgium
Wim Waelput
Department of Anatomo-Pathology, UZ Brussel, Laarbeeklaan 101, B-1090 Brussels, Belgium
Louise Cras
Department of Anatomo-Pathology, UZ Brussel, Laarbeeklaan 101, B-1090 Brussels, Belgium
Stefanie Brock
Department of Anatomo-Pathology, UZ Brussel, Laarbeeklaan 101, B-1090 Brussels, Belgium
Stefaan Verhulst
Liver Cell Biology Research Group, Department of Biomedical Sciences, VUB, Laarbeeklaan 103/D, B-1090 Brussels, Belgium
Keith Kwan
Department of Pathology and Laboratory Medicine, Western University, London, ON N6A 3K7, Canada
Marian Vanhoeij
Department of Surgery, UZ Brussel, Laarbeeklaan 101, B-1090 Brussels, Belgium
Kris Thielemans
Laboratory for Molecular and Cellular Therapy, Department of Biomedical Sciences, Vrije Universiteit Brussel (VUB), Laarbeeklaan 103/E, B-1090 Brussels, Belgium
Karine Breckpot
Laboratory for Molecular and Cellular Therapy, Department of Biomedical Sciences, Vrije Universiteit Brussel (VUB), Laarbeeklaan 103/E, B-1090 Brussels, Belgium
The use of gene expression profiling (GEP) in cancer management is rising, as GEP can be used for disease classification and diagnosis, tailoring treatment to underlying genetic determinants of pharmacological response, monitoring of therapy response, and prognosis. However, the reliability of GEP heavily depends on the input of RNA in sufficient quantity and quality. This highlights the need for standard procedures to ensure best practices for RNA extraction from often small tumor biopsies with variable tissue handling. We optimized an RNA extraction protocol from fresh-frozen (FF) core needle biopsies (CNB) from breast cancer patients and from formalin-fixed paraffin-embedded (FFPE) tissue when FF CNB did not yield sufficient RNA. Methods to avoid ribonucleases andto homogenize or to deparaffinize tissues and the impact of tissue composition on RNA extraction were studied. Additionally, RNA’s compatibility with the nanoString nCounter® technology was studied. This technology platform enables GEP using small RNA fragments. After optimization of the protocol, RNA of high quality and sufficient quantity was obtained from FF CNB in 92% of samples. For the remaining 8% of cases, FFPE material prepared by the pathology department was used for RNA extraction. Both resulting RNA end products are compatible with the nanoString nCounter® technology.
