RNA-Seq of human whole blood: Evaluation of globin RNA depletion on Ribo-Zero library method

Peripheral blood is a highly accessible biofluid providing a rich source of information about human physiology and health status. However, for studies of the blood transcriptome with RNA sequencing (RNA-Seq) techniques, high levels of hemoglobin mRNAs (hgbRNA) present in blood can occupy valuable se...

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Published inScientific reports Vol. 10; no. 1; p. 6271
Main Authors Harrington, Christina A., Fei, Suzanne S., Minnier, Jessica, Carbone, Lucia, Searles, Robert, Davis, Brett A., Ogle, Kimberly, Planck, Stephen R., Rosenbaum, James T., Choi, Dongseok
Format Journal Article
LanguageEnglish
Published London Nature Publishing Group UK 14.04.2020
Nature Publishing Group
Subjects
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38/91
45
631/1647/2017
631/337/2019
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Blood
Gene expression
Globins - genetics
Hemoglobin
Humanities and Social Sciences
Humans
Libraries
multidisciplinary
Peripheral blood
RNA - analysis
RNA-Seq
rRNA
Science
Science (multidisciplinary)
Specimen Handling - methods
Statistical analysis
Transcriptome
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Summary:Peripheral blood is a highly accessible biofluid providing a rich source of information about human physiology and health status. However, for studies of the blood transcriptome with RNA sequencing (RNA-Seq) techniques, high levels of hemoglobin mRNAs (hgbRNA) present in blood can occupy valuable sequencing space, impacting detection and quantification of non-hgbRNAs. In this study, we evaluated two methods for preparing ribosomal RNA (rRNA)-depleted sequencing libraries for RNA-Seq of whole blood, one of which is also designed to deplete hgbRNAs. Two experiments were performed: one evaluating library performance across 6 human blood samples and the other examining library reproducibility and performance in a two-subject subset. We find that addition of hgbRNA depletion to the rRNA-depletion protocol for library preparation from blood RNA effectively reduces highly abundant hgbRNA reads; however, it does not result in a statistically significant increase in differentially expressed genes in our patient-control study. Bioinformatic removal of globin gene counts in non-hgbRNA depleted libraries provides improvement in overall performance of these libraries. We conclude that use of a standard ribosomal RNA depletion method for library preparation coupled with bioinformatic removal of globin gene counts is sufficient for reproducible and sensitive measurement of both coding and noncoding RNAs in the blood transcriptome.
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ISSN:2045-2322
2045-2322
DOI:10.1038/s41598-020-62801-6