Identification and validation of extracellular vesicle reference genes for the normalization of RT‐qPCR data

Extracellular vesicles (EVs) contain a plethora of biomolecules, including nucleic acids, with diverse diagnostic and therapeutic application potential. Although reverse transcription‐quantitative PCR (RT‐qPCR) is the most widely applied laboratory technique to evaluate gene expression, its applicab...

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Published inJournal of extracellular vesicles Vol. 13; no. 4; pp. e12421 - n/a
Main Authors Pinheiro, Cláudio, Guilbert, Niké, Lippens, Lien, Roux, Quentin, Boiy, Robin, Fischer, Suzanne, Van Dorpe, Sofie, De Craene, Bram, Berx, Geert, Boterberg, Tom, Sys, Gwen, Denys, Hannelore, Miinalainen, Ilkka, Mestdagh, Pieter, Vandesompele, Jo, De Wever, Olivier, Hendrix, An
Format Journal Article
LanguageEnglish
Published United States John Wiley and Sons Inc 01.04.2024
Wiley
Subjects
blood
Cell Line
Cells, Cultured
conditioned medium
exosomes
extracellular vesicles
Extracellular Vesicles - genetics
Extracellular Vesicles - metabolism
Humans
microvesicles
mRNA
protease
reference genes
Reverse Transcription
RNA - metabolism
RNase
snRNP Core Proteins - metabolism
tissue
urine
conditioned medium
protease
reference genes
extracellular vesicles
urine
exosomes
mRNA
tissue
microvesicles
blood
RNase
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Summary:Extracellular vesicles (EVs) contain a plethora of biomolecules, including nucleic acids, with diverse diagnostic and therapeutic application potential. Although reverse transcription‐quantitative PCR (RT‐qPCR) is the most widely applied laboratory technique to evaluate gene expression, its applicability in EV research is challenged by the lack of universal and stably present reference genes (RGs). In this study, we identify, validate and establish SNRPG, OST4, TOMM7 and NOP10 as RGs for the normalization of EV‐associated genes by RT‐qPCR. We show the stable presence of SNRPG, OST4, TOMM7 and NOP10 in multiple cell lines and their secreted EVs (n = 12) under different (patho)physiological conditions as well as in human‐derived biofluids (n = 3). Enzymatic treatments confirm the presence of SNRPG, OST4, TOMM7 and NOP10 inside EVs. In addition, the four EV‐associated RGs are stably detected in a size‐range of EV subpopulations. RefFinder analysis reveals that SNRPG, OST4, TOMM7 and NOP10 are more stable compared to RGs established specifically for cultured cells or tissues such as HMBS, YWHAZ, SDHA and GAPDH. In summary, we present four universal and stably present EV‐associated RGs to enable normalization and thus steer the implementation of RT‐qPCR for the analysis of EV‐associated RNA cargo for research or clinical applications.
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ISSN:2001-3078
2001-3078
DOI:10.1002/jev2.12421