Cas9 nickase-mediated contraction of CAG/CTG repeats at multiple disease loci

Author:

Murillo AlvaroORCID,Alpaugh MelanieORCID,Larin MeghanORCID,Randall Emma L.ORCID,Heraty LauraORCID,Durairaj Ruban RexORCID,Aston Alys N.ORCID,Taylor Alysha S.ORCID,Monteys Alex MasORCID,Stöberl NinaORCID,Heuchan Aeverie E. R.ORCID,Aeschlimann PascaleORCID,Bhattacharyya SoumyasreeORCID,Allen Nicholas D.ORCID,Puymirat JackORCID,Davidson Beverly L.ORCID,Cicchetti Francesca,Lelos Mariah,Dion VincentORCID

Abstract

AbstractExpanded CAG/CTG repeats cause at least 15 different neurodegenerative and neuromuscular diseases that all remain without an effective disease modifying treatment. Because the size of the repeat tract accounts for the majority of the variation in disease severity, contracting them presents an attractive therapeutic avenue. Here, we show that the CRISPR-Cas9 nickase targeting the CAG/CTG repeat itself leads to efficient contractions in Huntington’s disease patient-derived neurons and astrocytes, as well as in myotonic dystrophy type 1 patient-derived neurons. Using single-cell DNA sequencing, PCR-free whole genome sequencing, and targeted long-read sequencing of theHTTlocus, we found no off-target mutations above background in neurons and astrocytes. Furthermore, we delivered the Cas9 nickase and sgRNA stereotactically to a mouse model of Huntington’s disease using adeno-associated viruses, and found contractions accumulating in over half of the infected cells over a period of 5 months. We also found that the Cas9 nickase was prone to silencing, further improving the safety of the approach. Our results provide the proof of concept for using the Cas9 nickase to contract the repeat tract safely in multiple cell types and diseases.

Publisher

Cold Spring Harbor Laboratory

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