Cell-mediated exon skipping normalizes dystrophin expression and muscle function in a new mouse model of Duchenne Muscular Dystrophy

Author:

Galli FrancescoORCID,Bragg Laricia,Rossi MairaORCID,Proietti Daisy,Perani LauraORCID,Bacigaluppi MarcoORCID,Tonlorenzi RossanaORCID,Sibanda Tendai,Caffarini Miriam,Talapatra AvraneelORCID,Santoleri Sabrina,Meregalli Mirella,Bano-Otalora BeatrizORCID,Bigot AnneORCID,Bozzoni IreneORCID,Bonini Chiara,Mouly Vincent,Torrente YvanORCID,Cossu GiulioORCID

Abstract

AbstractCell therapy for muscular dystrophy has met with limited success, mainly due to the poor engraftment of donor cells, especially in fibrotic muscle at an advanced stage of the disease. We developed a cell-mediated exon skipping that exploits the multinucleated nature of myofibers to achieve cross-correction of resident, dystrophic nuclei by the U7 small nuclear RNA engineered to skip exon 51 of the dystrophin gene. We observed that co-culture of genetically corrected human DMD myogenic cells (but not of WT cells) with their dystrophic counterparts at a ratio of either 1:10 or 1:30 leads to dystrophin production at a level several folds higher than what predicted by simple dilution. This is due to diffusion of U7 snRNA to neighbouring dystrophic resident nuclei. When transplanted into NSG-mdx-Δ51mice carrying a mutation of exon 51, genetically corrected human myogenic cells produce dystrophin at much higher level than WT cells, well in the therapeutic range, and lead to force recovery even with an engraftment of only 3–5%. This level of dystrophin production is an important step towards clinical efficacy for cell therapy.

Funder

UKRI | Medical Research Council

Wellcome Trust

Duchenne Parent Project

Publisher

Springer Science and Business Media LLC

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