Ex vivo gene transfer using adenovirus-mediated full-length dystrophin delivery to dystrophic muscles

Floyd, S. Steven; Clemens, Paula R.; Ontell, Martin P.; Kochanek, Stefan; Day, Charles S.; Yang, Jing; Hauschka, S. D.; Balkir, Levent; Morgan, J.E.; Moreland, Morey S.; Feero, Greg; Epperly, M.W.; Huard, Johnny

doi:10.1038/sj.gt.3300549

Cited by 82 publications

(35 citation statements)

References 64 publications

(108 reference statements)

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“…41 However, it is clear to us that the use of the adenoviral vector as well as the bacterial ␤-galactosidase to follow the fate Gene Therapy of the injected cells will trigger an immune response in long-term experiments. 42 In summary, we have (1) demonstrated the feasibility and survival of MDC injection into the bladder wall; (2) established improved detrusor contractility with MDC injection in a bladder injury model; (3) revealed the maturity of the ␤-galactosidase expressing myofibers in the injured bladder by demonstrating the presence of neuromuscular junctions based on the accumulation of AChRs in small segments of their membrane; and (4) demonstrated the possiblity of MDC differentiating into a smooth muscle lineage when injected into the bladder wall. We hypothesize that autologous MDC injections (muscle cells harvested from and cultured for a specific incontinence patient) can be used as a nonallergenic agent to improve bladder contractility.…”

Section: Figure 4 Physiological Improvement Of the Injured Bladder VImentioning

confidence: 99%

Muscle-derived cell-mediated ex vivo gene therapy for urological dysfunction

et al. 2002

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Section: Figure 4 Physiological Improvement Of the Injured Bladder VImentioning

confidence: 99%

Muscle-derived cell-mediated ex vivo gene therapy for urological dysfunction

et al. 2002

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“…To avoid this problem, ex vivo gene therapy approaches should be developed, and the in vitro engineering of dystrophic myoblasts for the expression of the therapeutic ␣2 chain gene is currently under investigation. 43,44 The understanding and control of premature cell death following injection should also be beneficial to overall transplantation results. Indeed, the success of myoblast transplantation has been recently improved by manipulating the immune response [40][41][42]44,45 or the biochemical adequacy between the donor cell and the recipient muscle 42 in other mouse models.…”

Section: Myoblasts As Versatile Candidates For In Vivo or Ex Vivo Resmentioning

confidence: 99%

Myoblast transplantations lead to the expression of the laminin α2 chain in normal and dystrophic (dy/dy) mouse muscles

et al. 1999

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Laminin-2 is part of the basement membrane of the skelmouse myoblast cell line in dy/dy muscles allows the etal muscle fibers. The laminin ␣2 chain is absent or drastiexpression of the murine laminin ␣2 chain; and (3) allocally reduced in a subgroup of congenital muscular dystransplantation of the D7 dystrophic dy/dy cell line allows trophy patients, and in the severely affected dystrophic the formation of new and hybrid muscle fibers in dy/dy dy/dy mouse. We previously reported that heterogenous muscle in the absence of laminin ␣2 chain expression. We primary mouse muscle cell cultures conferred laminin ␣2 conclude that normal myoblasts are able to restore the chain expression in dy/dy mice muscles upon cell transexpression of an extracellular skeletal muscle protein and plantation. In the present study we investigated whether that the absence of laminin-2 does not prevent transpure myoblast cell lines were able to confer laminin ␣2 planted muscle cells from participating in the formation of chain expression in vivo. We observed that: (1) xenomyofibers. Myoblasts are, therefore, attractive tools for transplantation of non-immortalized human myoblast in further exploration of gene complementation strategies in SCID mouse muscles allows human laminin ␣2 chain the animal models of congenital muscular dystrophy. expression; (2) allotransplantation of the permanent G8

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“…The feasibility of ex-vivo cell mediated gene transfer is being widely investigated (Pagel et al, 1995;Floyd et al, 1998). More recently, genetically engineered myoblast mediated FGF2 delivery for revasularization in a model of acute skin flap ischemia has been documented (Rinch et al, 2001).…”

Section: Introductionmentioning

confidence: 99%