TY - JOUR T1 - Impact of RNA Extraction and Target Capture Methods on RNA Sequencing Using Formalin-Fixed, Paraffin Embedded Tissues JF - bioRxiv DO - 10.1101/656736 SP - 656736 AU - Christopher A. Hilker AU - Aditya V. Bhagwate AU - Jin Sung Jang AU - Jeffrey G Meyer AU - Asha A. Nair AU - Jaime I. Davila AU - Amber M. McDonald AU - Jennifer L. Winters AU - Rebecca N. Wehrs AU - Rory A. Jackson AU - Joshua A. Gorman AU - Mine S. Cicek AU - Andre M. Oliveira AU - E. Aubrey Thompson AU - Bruce W. Eckloff AU - Kevin C. Halling AU - Zhifu A. Sun AU - Jin Jen Y1 - 2019/01/01 UR - http://biorxiv.org/content/early/2019/05/31/656736.abstract N2 - Formalin fixed paraffin embedded (FFPE) tissues are commonly used biospecimen for clinical diagnosis. However, RNA degradation is extensive when isolated from FFPE blocks making it challenging for whole transcriptome profiling (RNA-seq). Here, we examined RNA isolation methods, quality metrics, and the performance of RNA-seq using different approaches with RNA isolated from FFPE and fresh frozen (FF) tissues. We evaluated FFPE RNA extraction methods using six different tissues and five different methods. The reproducibility and quality of the prepared libraries from these RNAs were assessed by RNA-seq. We next examined the performance and reproducibility of RNA-seq for gene expression profiling with FFPE and FF samples using targeted (Kinome capture) and whole transcriptome capture based sequencing. Finally, we assessed Agilent SureSelect All-Exon V6+UTR capture and the Illumina TruSeq RNA Access protocols for their ability to detect known gene fusions in FFPE RNA samples. Although the overall yield of RNA varied among extraction methods, gene expression profiles generated by RNA-seq were highly correlated (>90%) when the input RNA was of sufficient quality (≥DV200 30%) and quantity (≥ 100 ng). Using gene capture, we observed a linear relationship between gene expression levels for shared genes that were captured using either All-Exon or Kinome kits. Gene expression correlations between the two capture-based approaches were similar using RNA from FFPE and FF samples. However, TruSeq RNA Access protocol provided significantly higher exon and junction reads when compared to the SureSelect All-Exon capture kit and was more sensitive for fusion gene detection. Our study established pre and post library construction QC parameters that are essential to reproducible RNA-seq profiling using FFPE samples. We show that gene capture based NGS sequencing is an efficient and highly reproducible strategy for gene expression measurements as well as fusion gene detection. ER -