Literature DB >> 23327925

Blood cell mRNAs and microRNAs: optimized protocols for extraction and preservation.

Michael Eikmans1, Niels V Rekers, Jacqueline D H Anholts, Sebastiaan Heidt, Frans H J Claas.   

Abstract

Assessing messenger RNA (mRNA) and microRNA levels in peripheral blood cells may complement conventional parameters in clinical practice. Working with small, precious samples requires optimal RNA yields and minimal RNA degradation. Several procedures for RNA extraction and complementary DNA (cDNA) synthesis were compared for their efficiency. The effect on RNA quality of freeze-thawing peripheral blood cells and storage in preserving reagents was investigated. In terms of RNA yield and convenience, quality quantitative polymerase chain reaction signals per nanogram of total RNA and using NucleoSpin and mirVana columns is preferable. The SuperScript III protocol results in the highest cDNA yields. During conventional procedures of storing peripheral blood cells at -180°C and thawing them thereafter, RNA integrity is maintained. TRIzol preserves RNA in cells stored at -20°C. Detection of mRNA levels significantly decreases in degraded RNA samples, whereas microRNA molecules remain relatively stable. When standardized to reference targets, mRNA transcripts and microRNAs can be reliably quantified in moderately degraded (quality index 4-7) and severely degraded (quality index <4) RNA samples, respectively. We describe a strategy for obtaining high-quality and quantity RNA from fresh and stored cells from blood. The results serve as a guideline for sensitive mRNA and microRNA expression assessment in clinical material.

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Year:  2013        PMID: 23327925     DOI: 10.1182/blood-2012-06-438887

Source DB:  PubMed          Journal:  Blood        ISSN: 0006-4971            Impact factor:   22.113


  21 in total

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Review 5.  Gene Expression Signatures and the Spectrum of Coronary Artery Disease.

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Review 7.  The procurement, storage, and quality assurance of frozen blood and tissue biospecimens in pathology, biorepository, and biobank settings.

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8.  In vitro application of ribonucleases: comparison of the effects on mRNA and miRNA stability.

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Journal:  BMC Res Notes       Date:  2015-04-22

9.  Immune cell subsets and their gene expression profiles from human PBMC isolated by Vacutainer Cell Preparation Tube (CPT™) and standard density gradient.

Authors:  Christopher P Corkum; Danielle P Ings; Christopher Burgess; Sylwia Karwowska; Werner Kroll; Tomasz I Michalak
Journal:  BMC Immunol       Date:  2015-08-26       Impact factor: 3.615

10.  Methods to determine the transcriptomes of trypanosomes in mixtures with mammalian cells: the effects of parasite purification and selective cDNA amplification.

Authors:  Julius Mulindwa; Abeer Fadda; Clementine Merce; Enoch Matovu; John Enyaru; Christine Clayton
Journal:  PLoS Negl Trop Dis       Date:  2014-04-17
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