Effects of Mini-Dystrophin on Dystrophin-Deficient, Human Skeletal Muscle-Derived Cells

Meng, Jinhong; Counsell, John R.; Morgan, Jennifer E.

doi:10.3390/ijms21197168

“…Cell images were then used to extract the myotube area (MHC-positive area), and nuclei count (Figure 1C ), which was used to compute the fusion index (See Methods). As expected, the fusion index for the DMD donors (DMD #1 and DMD #4) was significantly lower compared to non-DMD donors (Non-DMD #1 and Non-DMD #3) (Meng et al, 2020 ).…”

Section: Characterizing Primary Donor Cells For Myoscreen Platformsupporting

confidence: 80%

Development and validation of a high throughput screening platform to enable target identification in skeletal muscle cells from Duchenne Muscular Dystrophy (DMD) patients

Hariharan,

Lorintiu,

Lee

et al. 2023

Preprint

0

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Duchenne muscular dystrophy (DMD) is a progressive and fatal muscle degenerating disease caused by dystrophin deficiency. Effective methods for drug discovery for the treatment of DMD requires systems to be physiologically relevant, scalable, and effective. To this end, the Myoscreen platform offers a scalable and physiologically relevant system for generating and characterizing patient-derived myotubes. Morphological profiling is a powerful technique involving the simultaneous measurement of hundreds of morphological parameters from fluorescence microscopy images and using machine learning to predict cellular activity. Here, we describe combining the Myoscreen platform and high dimensional morphological profiling to accurately predict a phenotype associated with the lack of Dystrophin expression in patient derived myotubes. Using this methodology, we evaluated a series of Dystrophin-associated protein complex (DAPC) candidates and identified that the combination of Utrophin and α- Sarcoglycan yielded highest morphological differences between DMD and non-DMD donors. Finally, we validated this methodology by knocking down Dystrophin expression in non-DMD cells as well as introducing Dystrophin expression in DMD cells. Knocking down Dystrophin in non- DMD cells shifted their morphological profile to one that is similar to DMD cells while introducing Dystrophin in DMD cells shifted their morphological profile towards non-DMD cells. In conclusion, we have developed a platform that accurately predicts the DMD disease phenotype in a disease relevant cell type. Ultimately this platform may have wide applications in the drug development process include identification of disease modifier genes, screening of novel therapeutic moieties, and as a potency assay for future therapeutics.

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“…Cell images were then used to extract the myotube area (MHC-positive area), and nuclei count (Figure 1C ), which was used to compute the fusion index (See Methods). As expected, the fusion index for the DMD donors (DMD #1 and DMD #4) was significantly lower compared to non-DMD donors (Non-DMD #1 and Non-DMD #3) (Meng et al, 2020 ).…”

Section: Characterizing Primary Donor Cells For Myoscreen Platformsupporting

confidence: 80%

Development and validation of a high throughput screening platform to enable target identification in skeletal muscle cells from Duchenne Muscular Dystrophy (DMD) patients

Hariharan,

Lorintiu,

Lee

et al. 2023

Preprint

0

View full text Add to dashboard Cite

Duchenne muscular dystrophy (DMD) is a progressive and fatal muscle degenerating disease caused by dystrophin deficiency. Effective methods for drug discovery for the treatment of DMD requires systems to be physiologically relevant, scalable, and effective. To this end, the Myoscreen platform offers a scalable and physiologically relevant system for generating and characterizing patient-derived myotubes. Morphological profiling is a powerful technique involving the simultaneous measurement of hundreds of morphological parameters from fluorescence microscopy images and using machine learning to predict cellular activity. Here, we describe combining the Myoscreen platform and high dimensional morphological profiling to accurately predict a phenotype associated with the lack of Dystrophin expression in patient derived myotubes. Using this methodology, we evaluated a series of Dystrophin-associated protein complex (DAPC) candidates and identified that the combination of Utrophin and α- Sarcoglycan yielded highest morphological differences between DMD and non-DMD donors. Finally, we validated this methodology by knocking down Dystrophin expression in non-DMD cells as well as introducing Dystrophin expression in DMD cells. Knocking down Dystrophin in non- DMD cells shifted their morphological profile to one that is similar to DMD cells while introducing Dystrophin in DMD cells shifted their morphological profile towards non-DMD cells. In conclusion, we have developed a platform that accurately predicts the DMD disease phenotype in a disease relevant cell type. Ultimately this platform may have wide applications in the drug development process include identification of disease modifier genes, screening of novel therapeutic moieties, and as a potency assay for future therapeutics.

show abstract

“… 25 We have previously reported that expression of minidystrophin in DMD muscle stem cells can adversely affect their proliferation and myogenic differentiation in vitro. 26 Therefore, it would be advantageous to use a muscle-specific promoter that drives transgene expression only in differentiated myotubes/myofibers and is small enough to fit into the lentiviral vector together with the large full-length DMD human cDNA.…”

Section: Introductionmentioning

confidence: 99%

Optimized lentiviral vector to restore full-length dystrophin via a cell-mediated approach in a mouse model of Duchenne muscular dystrophy

Meng

¹

,

Moore

²

,

Counsell

³

et al. 2022

Molecular Therapy - Methods & Clinical Development

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Effects of Mini-Dystrophin on Dystrophin-Deficient, Human Skeletal Muscle-Derived Cells

Cited by 6 publications

References 59 publications

Development and validation of a high throughput screening platform to enable target identification in skeletal muscle cells from Duchenne Muscular Dystrophy (DMD) patients

Development and validation of a high throughput screening platform to enable target identification in skeletal muscle cells from Duchenne Muscular Dystrophy (DMD) patients

Development and validation of a high throughput screening platform to enable target identification in skeletal muscle cells from Duchenne Muscular Dystrophy (DMD) patients

Optimized lentiviral vector to restore full-length dystrophin via a cell-mediated approach in a mouse model of Duchenne muscular dystrophy

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