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A CRISPR-Cas9-based reporter system for single-cell detection of extracellular vesicle-mediated functional transfer of RNA.

Olivier G de Jong ,
Daniel E Murphy ,
Imre Mäger ,
Eduard Willms ,
Antonio Garcia-Guerra ,
Jerney J Gitz-Francois ,
Juliet Lefferts ,
Dhanu Gupta ,
Sander C Steenbeek ,
Jacco van Rheenen ,
Samir El Andaloussi ,
Raymond M Schiffelers ,
Matthew J A Wood ,
Pieter Vader

Abstract

Extracellular vesicles (EVs) form an endogenous transport system for intercellular transfer of biological cargo, including RNA, that plays a pivotal role in physiological and pathological processes. Unfortunately, whereas biological effects of EV-mediated RNA transfer are abundantly studied, regulatory pathways and mechanisms remain poorly defined due to a lack of suitable readout systems. Here, we describe a highly-sensitive CRISPR-Cas9-based reporter system that allows direct functional study of EV-mediated transfer of small non-coding RNA molecules at single-cell resolution. Using this CRISPR operated stoplight system for functional intercellular RNA exchange (CROSS-FIRE) we uncover various genes involved in EV subtype biogenesis that play a regulatory role in RNA transfer. Moreover we identify multiple genes involved in endocytosis and intracellular membrane trafficking that strongly regulate EV-mediated functional RNA delivery. Altogether, this approach allows the elucidation of regulatory mechanisms in EV-mediated RNA transfer at the level of EV biogenesis, endocytosis, intracellular trafficking, and RNA delivery.

More about this publication

Nature communications

Volume 11
Issue nr. 1
Pages 1113
Publication date 28-02-2020

Full text links

Publisher website (DOI) 10.1038/s41467-020-14977-8
Europe PubMed Central 32111843
Pubmed 32111843

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