Stable transduction of myogenic cells with lentiviral vectors expressing a minidystrophin

Li, S; Kimura, En; Fall, Brent; Reyes, Morayma; Angello, John C.; Welikson, Robert E.; Hauschka, Stephen D.; Chamberlain, Jeffrey S.

doi:10.1038/sj.gt.3302505

Cited by 83 publications

(64 citation statements)

References 47 publications

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“…Our lentivirus construction recapitulates the transduction efficiency of previously tested and published lentivirus vectors [38,39]. We performed FACS analysis to determine the expression of GFP in infected CD133+ normal blood derived cells and we showed a percentage of 60.9% of GFP positive cells demonstrating a good efficiency of transduction as previously described [40,41] (Fig. 3B).…”

Section: Patient Phenotype and Genotype Descriptionmentioning

confidence: 99%

“…The PCR product woas digested with NheI and subcloned into pRRL-cPPT-hPGK-eGFP-WPRE vector. The transduction efficiency of lentiviral vectors containing eGFP and the dysferlin cassette was tested using the same multiplicity of infection as previously described [40,41]. Both lentiviral vectors showed the same transduction efficiency.…”

Section: Lentivector Carrying the Full-length Dysferlinmentioning

confidence: 99%

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Full‐length dysferlin expression driven by engineered human dystrophic blood derived CD133+ stem cells

et al. 2013

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The protein dysferlin is abundantly expressed in skeletal and cardiac muscles, where its main function is membrane repair. Mutations in the dysferlin gene are involved in two autosomal recessive muscular dystrophies: Miyoshi myopathy and limb‐girdle muscular dystrophy type 2B. Development of effective therapies remains a great challenge. Strategies to repair the dysferlin gene by skipping mutated exons, using antisense oligonucleotides (AONs), may be suitable only for a subset of mutations, while cell and gene therapy can be extended to all mutations. AON‐treated blood‐derived CD133+ stem cells isolated from patients with Miyoshi myopathy led to partial dysferlin reconstitution in vitro but failed to express dysferlin after intramuscular transplantation into scid/blAJ dysferlin null mice. We thus extended these experiments producing the full‐length dysferlin mediated by a lentiviral vector in blood‐derived CD133+ stem cells isolated from the same patients. Transplantation of engineered blood‐derived CD133+ stem cells into scid/blAJ mice resulted in sufficient dysferlin expression to correct functional deficits in skeletal muscle membrane repair. Our data suggest for the first time that lentivirus‐mediated delivery of full‐length dysferlin in stem cells isolated from Miyoshi myopathy patients could represent an alternative therapeutic approach for treatment of dysferlinopathies.

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Section: Patient Phenotype and Genotype Descriptionmentioning

confidence: 99%

Section: Lentivector Carrying the Full-length Dysferlinmentioning

confidence: 99%

Full‐length dysferlin expression driven by engineered human dystrophic blood derived CD133+ stem cells

et al. 2013

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“…Lentiviral vectors have been used to treat mdx mice locally restoring dystrophin expression at different efficiencies (Kobinger et al, 2003;Li et al, 2005). Kimura and colleagues showed that a lentivirus encoding μDys intramuscularly injected into 2 weeks old mdx 4cv mice could restore dystrophin in up to 400-1200 fibers in the tibialis anterior muscle.…”

Section: Lentiviral Vectorsmentioning

confidence: 99%

Duchenne Muscular Dystrophy: Therapeutic Approaches to Restore Dystrophin

Spitali¹,

Aartsma‐Rus²

2012

Muscular Dystrophy

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“…However key questions that need to be resolved before this approach could be used in DMD include the optimal vector configuration and the safety profile of the gene delivery methodology. Lentiviral vectors efficiently infect quiescent cells, including stem cells (S. Li et al, 2005) and give long-term, heritable, gene expression because they integrate into the host genome. Drawbacks with lentiviral vectors include possible gene silencing, or mutagenesis (Wilson & Cichutek, 2009), due to the site at which the virus inserts into the host genome.…”

Section: Genetic Modification Of Autologous Cellsmentioning

confidence: 99%

“…A lentiviral vector has been used to insert a 6.8 kb dystrophin mini gene (S. Li et al, 2005), to give rise to a shorter dystrophin protein in regenerated muscle fibers. While these engineered mini-dystrophins appear to retain most of the functional properties of full-length dystrophin, they nevertheless miss important domains, such as the nitric oxide synthase anchoring domain (Lai et al, 2009).…”

Section: Genetic Modification Of Autologous Cellsmentioning

confidence: 99%

Stem Cell Based Therapy for Muscular Dystrophies: Cell Types and Environmental Factors Influencing Their Efficacy

Morgan¹,

Alameddine²

2012

Muscular Dystrophy

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Stable transduction of myogenic cells with lentiviral vectors expressing a minidystrophin

Cited by 83 publications

References 47 publications

Full‐length dysferlin expression driven by engineered human dystrophic blood derived CD133+ stem cells

Full‐length dysferlin expression driven by engineered human dystrophic blood derived CD133+ stem cells

Duchenne Muscular Dystrophy: Therapeutic Approaches to Restore Dystrophin

Stem Cell Based Therapy for Muscular Dystrophies: Cell Types and Environmental Factors Influencing Their Efficacy

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