mRNA therapy restores ureagenesis and corrects glutathione metabolism in argininosuccinic aciduria

Author:

Gurung Sonam,Timmermand Oskar V.,Perocheau Dany,Gil-Martinez Ana Luisa,Minnion Magdalena,Touramanidou Loukia,Fang Sherry,Messina Martina,Khalil Youssef,Barber Abigail R.,Edwards Richard S.,Finn Patrick F.,Cavedon Alex,Siddiqui Summar,Rice Lisa,Martini Paolo G.V.,Mills Philippa B.,Waddington Simon N.,Gissen Paul,Eaton Simon,Ryten Mina,Feelisch Martin,Frassetto Andrea,Witney Timothy H.,Baruteau Julien

Abstract

AbstractArgininosuccinate lyase (ASL) is a key enzyme integral to the hepatic urea cycle which is required for ammonia detoxification, and the citrulline-nitric oxide (NO) cycle for NO production. ASL deficient patients present with argininosuccinic aciduria (ASA), an inherited metabolic disease with hyperammonaemia and a chronic systemic phenotype with neurocognitive impairment and chronic liver disease. ASL deficiency as an inherited model of systemic NO deficiency, shows enhanced nitrosative and oxidative stress. Here, we describe the dysregulation of glutathione biosynthesis and upstream cysteine utilization in ASL-deficient patients and mice using targeted metabolomics andin vivopositron emission tomography (PET) imaging using (S)-4-(3-18F-fluoropropyl)-L-glutamate ([18F]FSPG). Upregulation of cysteine metabolism contrasted with glutathione depletion and down-regulated antioxidant pathways.hASLmRNA encapsulated in lipid nanoparticles corrected and rescued the neonatal and adult Asl-deficient mouse phenotypes, respectively, enhancing ureagenesis and glutathione metabolism and ameliorating chronic liver disease. We further present [18F]FSPG PET as a novel non-invasive diagnostic tool to assess liver disease and therapeutic efficacy in ASA. These findings support clinical translation of mRNA therapy for ASA.

Publisher

Cold Spring Harbor Laboratory

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