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Systemic AAV8-mediated delivery of a functional copy of muscle glycogen phosphorylase (Pygm) ameliorates disease in a murine model of McArdle disease.

Hum Mol Genet. 2020; 
McNamara EL,, Taylor RL,, Clayton JS,, Goullee H,, Dilworth KL, Pinós T,, Brull A, Alexander IE,, Lisowski L,,, Ravenscroft G,, Laing NG,, Nowak KJ,,.
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PCR Cloning and Subcloning 292 Materials and Methods 293 AAV8 construct design and virus production 294 The mouse Pygm cDNA sequence with a potent, synthetic skeletal muscle specific promoter, triple 295 muscle creatine kinase (tMCK)47, was designed in silico and subsequently custom synthesised by 296 GenScript....1 using a TOPO TA cloning kit (Thermo 334 Fisher, USA), or purchased directly from GenScript (USA). Get A Quote

摘要

McArdle disease is a disorder of carbohydrate metabolism that causes painful skeletal muscle cramps and skeletal muscle damage leading to transient myoglobinuria and increased risk of kidney failure. McArdle disease is caused by recessive mutations in the muscle glycogen phosphorylase (PYGM) gene leading to absence of PYGM enzyme in skeletal muscle and preventing access to energy from muscle glycogen stores. There is currently no cure for McArdle disease. Using a preclinical animal model, we aimed to identify a clinically translatable and relevant therapy for McArdle disease. We evaluated the safety and efficacy of recombinant adeno-associated virus serotype 8 (rAAV8) to treat a murine model of McArdle disease ... More

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