Evaluation of Existing Methods for Human Blood mRNA Isolation and Analysis for Large Studies

Anke Meyer; Federico Paroni; Kathrin Günther; Gitanjali Dharmadhikari; Wolfgang Ahrens; Sørge Kelm; Kathrin Maedler

doi:10.1371/journal.pone.0161778

Evaluation of Existing Methods for Human Blood mRNA Isolation and Analysis for Large Studies

PLoS One. 2016 Aug 30;11(8):e0161778. doi: 10.1371/journal.pone.0161778. eCollection 2016.

Authors

Anke Meyer¹, Federico Paroni¹, Kathrin Günther², Gitanjali Dharmadhikari¹, Wolfgang Ahrens², Sørge Kelm¹, Kathrin Maedler^{1

3}

Affiliations

¹ Centre for Biomolecular Interactions Bremen, University of Bremen, Bremen, Germany.
² Leibniz-Institute for Prevention Research and Epidemiology-BIPS, Bremen, Germany.
³ German Center for Diabetes Research (DZD) project partner, University of Bremen, Bremen, Germany.

Abstract

Aims: Prior to implementing gene expression analyses from blood to a larger cohort study, an evaluation to set up a reliable and reproducible method is mandatory but challenging due to the specific characteristics of the samples as well as their collection methods. In this pilot study we optimized a combination of blood sampling and RNA isolation methods and present reproducible gene expression results from human blood samples.

Methods: The established PAXgeneTM blood collection method (Qiagen) was compared with the more recent TempusTM collection and storing system. RNA from blood samples collected by both systems was extracted on columns with the corresponding Norgen and PAX RNA extraction Kits. RNA quantity and quality was compared photometrically, with Ribogreen and by Real-Time PCR analyses of various reference genes (PPIA, β-ACTIN and TUBULIN) and exemplary of SIGLEC-7.

Results: Combining different sampling methods and extraction kits caused strong variations in gene expression. The use of PAXgeneTM and TempusTM collection systems resulted in RNA of good quality and quantity for the respective RNA isolation system. No large inter-donor variations could be detected for both systems. However, it was not possible to extract sufficient RNA of good quality with the PAXgeneTM RNA extraction system from samples collected by TempusTM collection tubes. Comparing only the Norgen RNA extraction methods, RNA from blood collected either by the TempusTM or PAXgeneTM collection system delivered sufficient amount and quality of RNA, but the TempusTM collection delivered higher RNA concentration compared to the PAXTM collection system. The established Pre-analytix PAXgeneTM RNA extraction system together with the PAXgeneTM blood collection system showed lowest CT-values, i.e. highest RNA concentration of good quality. Expression levels of all tested genes were stable and reproducible.

Conclusions: This study confirms that it is not possible to mix or change sampling or extraction strategies during the same study because of large variations of RNA yield and expression levels.

Publication types

Comparative Study

MeSH terms

Blood Specimen Collection / methods*
Gene Expression Profiling / methods
Humans
Paired Box Transcription Factors / genetics*
Pilot Projects
RNA, Messenger / blood
RNA, Messenger / isolation & purification*
Reagent Kits, Diagnostic
Real-Time Polymerase Chain Reaction

Substances

Paired Box Transcription Factors
RNA, Messenger
Reagent Kits, Diagnostic

Grants and funding

This study was supported by ZF-funds from the University of Bremen (to AM), the ERC (260336-SIADIA; https://erc.europa.eu/) and the German Diabetes Center grant (DZD; https://www.dzd-ev.de/) from the BMBF (to KM). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.