NormQ: RNASeq normalization based on RT-qPCR derived size factors

Ravindra Naraine; Pavel Abaffy; Monika Sidova; Silvie Tomankova; Kseniia Pocherniaieva; Ondrej Smolik; Mikael Kubista; Martin Psenicka; Radek Sindelka

doi:10.1016/j.csbj.2020.05.010

NormQ: RNASeq normalization based on RT-qPCR derived size factors

Comput Struct Biotechnol J. 2020 May 14:18:1173-1181. doi: 10.1016/j.csbj.2020.05.010. eCollection 2020.

Authors

Ravindra Naraine¹, Pavel Abaffy¹, Monika Sidova¹, Silvie Tomankova¹, Kseniia Pocherniaieva², Ondrej Smolik^{1

3}, Mikael Kubista¹, Martin Psenicka², Radek Sindelka¹

Affiliations

¹ Laboratory of Gene Expression, Institute of Biotechnology of the Czech Academy of Sciences - BIOCEV, Prumyslova 595, Vestec 252 50, Czech Republic.
² University of South Bohemia in Ceske Budejovice, Faculty of Fisheries and Protection of Waters, South Bohemian Research Center of Aquaculture and Biodiversity of Hydrocenoses, Research Institute of Fish Culture and Hydrobiology, Vodnany, Czech Republic.
³ Department of Cell Biology, Faculty of Science, Charles University, Prague, Czech Republic.

Abstract

The merit of RNASeq data relies heavily on correct normalization. However, most methods assume that the majority of transcripts show no differential expression between conditions. This assumption may not always be correct, especially when one condition results in overexpression. We present a new method (NormQ) to normalize the RNASeq library size, using the relative proportion observed from RT-qPCR of selected marker genes. The method was compared against the popular median-of-ratios method, using simulated and real-datasets. NormQ produced more matches to differentially expressed genes in the simulated dataset and more distribution profile matches for both simulated and real datasets.

Keywords: DESeq; Median-of-ratios; Normalization; RNASeq; TOMOSeq; Transcriptomics.