Antibody-mediated enzyme replacement therapy targeting both lysosomal and cytoplasmic glycogen in Pompe disease

Yi, Haiqing; Sun, Tao; Armstrong, Dustin D.; Borneman, Scott; Yang, Chunyu; Austin, Stephanie; Kishnani, Priya S.; Sun, Baodong

doi:10.1007/s00109-017-1505-9

Cited by 26 publications

(14 citation statements)

References 36 publications

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“…This antibody-enzyme fusion (AEF) strategy has proven successful for the replacement of a cytosolic enzyme and rescue of X-linked myotubular myopathy in mice (Lawlor et al, 2013). A Fab-GAA fusion has similar efficacy to reduce glycogen in Pompe mice with the additional advantage of targeting both lysosomal and cytosolic glycogen and is now in Phase 1/2 clinical trials (Valerion Therapeutics, 2016;Yi et al, 2017). Rather than utilizing the AEF platform to deliver a replacement enzyme, we generated an AEF designed to penetrate cells and degrade pathogenic LBs.…”

Section: Introductionmentioning

confidence: 99%

Targeting Pathogenic Lafora Bodies in Lafora Disease Using an Antibody-Enzyme Fusion

et al. 2019

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Section: Introductionmentioning

confidence: 99%

Targeting Pathogenic Lafora Bodies in Lafora Disease Using an Antibody-Enzyme Fusion

et al. 2019

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“…While the glycogen in some GSDs is of normal structure like in Pompe disease, other GSDs such as Cori disease and Andersen disease are characterized by polyglucosans, like LD (7). Two AEF drugs (VAL-0417 and Fab-GAA) have now been shown to target, respectively, cytosolic polyglucosan (the present study) and normal glycogen in both the cytosol and lysosome (47). These drugs could be repurposed and/or modified to target glycogen in other GSDs.…”

Section: Discussionmentioning

confidence: 63%

“…In the first study, the deficient lipid phosphatase myotubularin fused to an Fv fragment was delivered by intramuscular injection and improved muscle function in a mouse model of myotubular myopathy (46). In the second, a Fab fragment fused to GAA delivered intravenously reduced glycogen load and alleviated pathology in GAA-deficient mice (47). These two studies illustrate that enzyme replacement therapy, which can be problematic for cytosolic enzymes, can be enhanced by fusion of the replacement enzyme with a cell-penetrating antibody fragment.…”

Section: Discussionmentioning

confidence: 99%

Targeting pathogenic Lafora bodies in Lafora disease using an antibody-enzyme fusion

Brewer

Uittenbogaard

Austin

et al. 2019

Preprint

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One Sentence Summary: An antibody-enzyme fusion delivering an amylase degrades the toxic polyglucosan bodies that cause Lafora disease, a fatal childhood epilepsy.Abstract: Lafora disease (LD) is a fatal childhood epilepsy and a non-classical glycogen storage disorder with no effective therapy or cure. LD is caused by recessive mutations in the EPM2A or EPM2B genes that encode the glycogen phosphatase laforin and an E3 ubiquitin ligase malin, respectively. A hallmark of LD is the intracellular accumulation of abnormal and insoluble α linked polysaccharide deposits known as Lafora bodies (LBs) in several tissues, including most regions of the brain. In mouse models of LD, genetic reduction of glycogen synthesis eliminates LB formation and rescues the neurological phenotype. Since multiple groups have confirmed that neurodegeneration and epilepsy result from LB accumulation, a major focus in the field has shifted toward the development of therapies that reduce glycogen synthesis or target LBs for degradation with the goal of treating LD. Herein, we identify the optimal enzymes for degrading LBs, and we develop a novel therapeutic agent by fusing human pancreatic α -amylase to a cellpenetrating antibody fragment. This antibody-enzyme fusion (VAL-0417) degrades LBs in vitro, shows robust cellular uptake, and significantly reduces the LB load in vivo in Epm2a-/-mice. VAL-0417 is a promising therapeutic for the treatment of LD and a putative precision therapy for an intractable epilepsy. Antibody-enzyme fusions represent a new class of antibody-based drugs that could be utilized to treat glycogen storage disorders and other diseases. The progressive myoclonic epilepsies (PMEs) are a group of inherited disorders characterized by recurrent seizures, myoclonus, and progressive neurological decline. There are currently no treatments for PMEs, and anti-epilepsy drugs are palliative at best (1). Lafora disease (LD; epilepsy, progressive myoclonus type 2, EPM2) is a severe form of PME that typically manifests with tonic-clonic seizures and myoclonic jerks in the early teen years followed by rapid neurological deterioration, increasingly severe and frequent epileptic episodes, dementia and death within ten years of onset (OMIM: 254780). LD is caused by mutations in the EPM2A or EPM2B genes that encode laforin, a glycogen phosphatase, and malin, an E3 ubiquitin ligase that ubiquitinates enzymes involved in glycogen metabolism (reviewed in (2)). LD is distinguishable from other PMEs by the presence of cytosolic polysaccharide inclusions known as Lafora bodies (LBs) most notably in the brain, where they are found in neuronal cell bodies and dendrites and astrocytic processes, and in other tissues such as muscle, heart, and liver (3-5). Among the PMEs LD is uniquely considered a non-classical glycogen storage disease (GSD) (6, 7). Independent studies from multiple groups demonstrate that Epm2a-/-and Epm2b-/-mice recapitulate disease symptoms with respect to LB formation, neurodegeneration, neurological impairments, and susceptibil...

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“…This monoclonal anti-DNA antibody were shown to penetrate living cells and move to the nucleus through the equilibrative nucleoside transporter 2 (ENT2) [113][114][115]. Experiments in cultured L6 myoblasts and fibroblasts derived from Pompe disease patients as well as in vivo studies in KO mice suggested a potential benefit of this fusion protein [116]. However, in our experience, VAL-1221 in KO mice did not show any improvement in muscle glycogen content (unpublished data).…”

Section: Next-generation Ertmentioning

confidence: 80%

Pompe Disease: New Developments in an Old Lysosomal Storage Disorder

Meena

Raben

2020

Biomolecules

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Pompe disease, also known as glycogen storage disease type II, is caused by the lack or deficiency of a single enzyme, lysosomal acid alpha-glucosidase, leading to severe cardiac and skeletal muscle myopathy due to progressive accumulation of glycogen. The discovery that acid alpha-glucosidase resides in the lysosome gave rise to the concept of lysosomal storage diseases, and Pompe disease became the first among many monogenic diseases caused by loss of lysosomal enzyme activities. The only disease-specific treatment available for Pompe disease patients is enzyme replacement therapy (ERT) which aims to halt the natural course of the illness. Both the success and limitations of ERT provided novel insights in the pathophysiology of the disease and motivated the scientific community to develop the next generation of therapies that have already progressed to the clinic.

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Antibody-mediated enzyme replacement therapy targeting both lysosomal and cytoplasmic glycogen in Pompe disease

Cited by 26 publications

References 36 publications

Targeting Pathogenic Lafora Bodies in Lafora Disease Using an Antibody-Enzyme Fusion

Targeting Pathogenic Lafora Bodies in Lafora Disease Using an Antibody-Enzyme Fusion

Targeting pathogenic Lafora bodies in Lafora disease using an antibody-enzyme fusion

Pompe Disease: New Developments in an Old Lysosomal Storage Disorder

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