Identifying stably expressed genes from multiple RNA-Seq data sets.

PeerJ

Department of Statistics, Oregon State University, Corvallis, OR, United States; Molecular and Cellular Biology Graduate Program, Oregon State University, Corvallis, OR, United States of America.

Published: December 2016

We examined RNA-Seq data on 211 biological samples from 24 different Arabidopsis experiments carried out by different labs. We grouped the samples according to tissue types, and in each of the groups, we identified genes that are stably expressed across biological samples, treatment conditions, and experiments. We fit a Poisson log-linear mixed-effect model to the read counts for each gene and decomposed the total variance into between-sample, between-treatment and between-experiment variance components. Identifying stably expressed genes is useful for count normalization and differential expression analysis. The variance component analysis that we explore here is a first step towards understanding the sources and nature of the RNA-Seq count variation. When using a numerical measure to identify stably expressed genes, the outcome depends on multiple factors: the background sample set and the reference gene set used for count normalization, the technology used for measuring gene expression, and the specific numerical stability measure used. Since differential expression (DE) is measured by relative frequencies, we argue that DE is a relative concept. We advocate using an explicit reference gene set for count normalization to improve interpretability of DE results, and recommend using a common reference gene set when analyzing multiple RNA-Seq experiments to avoid potential inconsistent conclusions.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC5178351PMC
http://dx.doi.org/10.7717/peerj.2791DOI Listing

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