Nucleofection of muscle-derived stem cells and myoblasts with ϕC31 integrase: stable expression of a full-length-dystrophin fusion gene by human myoblasts

Quenneville, Simon; Chapdelaine, Pierre; Rousseau, Joël; Beaulieu, Jean; Caron, Nicolas; Skuk, Daniel; Mills, Philippe; Olivares, Eric C.; Calos, Michèle P.; Tremblay, Jacques P.

doi:10.1016/j.ymthe.2004.05.034

Cited by 74 publications

(58 citation statements)

References 31 publications

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“…15,22 In our previous experiments, these methods were shown to be very efficient for the MPC transfection and stable gene expression in vitro. 11 The present work was carried out to verify whether the gene transfected with this method could be expressed in vivo.…”

Section: Discussionmentioning

confidence: 99%

“…As very low-transfection levels were observed in the preliminary experiments of nucleofection with the fulllength dystrophin transgene, 11 intermediate experiments using a truncated version of the dystrophin cDNA were carried out. This so-called MDys was fused with eGFP 18 and an attB sequence was also added in the plasmid to produce the p-attB-CMV-eGFP-MDys.…”

Section: Mini-dystrophin Gene Expression In MDX Muscle Fibersmentioning

confidence: 99%

“…The plasmid pattB-CMV-eGFP-Dys has been described previously. 11 The pattB-MCK-eGFP-Dys was produced using the same restriction sites (NdeI and AgeI) as described for pattB-MCK-eGFP-MDys. Figure 1 shows most of the constructs.…”

Section: Plasmidsmentioning

confidence: 99%

“…9,10 Recently, the Amaxa Corporation developed the nucleofection method, which allowed us to deliver not only eGFP but also the full-length dystrophin fused with eGFP into human primary MPCs. 11 Stable expressions of these transgenes were then obtained with the phiC31 integrase system. In this system, sequences called 'attB' and 'attP' are recognized and recombined by the integrase.…”

Section: Introductionmentioning

confidence: 99%

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Dystrophin expression in host muscle following transplantation of muscle precursor cells modified with the phiC31 integrase

et al. 2006

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Duchenne muscular dystrophy (DMD) is the most severe muscular dystrophy. It is caused by the absence of dystrophin in muscle fibers. The autologous transplantation of genetically corrected muscle precursor cells (MPCs) is a possible cure for DMD. A non-viral method of genetic modification was tested in this study. The co-transfection (nucleofection) of a phiC31 integrase and a transgene expressing plasmid in MPCs led to an increased stable expression in vitro. The stable expression of a small transgene (eGFP) in muscle fibers was initially demonstrated following the transplantation of the genetically modified cells. The stable expression of a truncated version of dystrophin as well as the full-length dystrophin fused with eGFP was then demonstrated in MPCs obtained from an mdx mice. The transplantation of these cells led not only to the expression of these fusion proteins in muscle fibers but also to the reconstitution of the dystrophin complex. Human MPCs were also genetically modified with a plasmid coding for the fulllength human dystrophin gene fused with eGFP and transplanted in severe combined immuno deficient mice leading to the expression of eGFP dystrophin in muscle fibers. This work indicates that cell transplantation after correction of MPCs with phiC31 integrase is a possible approach to treat DMD.

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Section: Discussionmentioning

confidence: 99%

Section: Mini-dystrophin Gene Expression In MDX Muscle Fibersmentioning

confidence: 99%

Section: Plasmidsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Dystrophin expression in host muscle following transplantation of muscle precursor cells modified with the phiC31 integrase

et al. 2006

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“…As the PCR analysis indicated the presence of the expected amplicon size, the nucleofection of infected human myoblasts was made as previously described. 43 In brief, 5 mg of plasmid MGNs RAG1 or I-SceI was introduced by nucleofection within the infected human myoblasts containing the corresponding specific target. Nucleofector solution adult (NHDF-adult) has been used and the nucleofector apparatus (AMAXA Inc., Amaxa Nucleofector System, Lonza Walkerrsville Inc., Walkersville, MD, USA) was set to program P-022 according to the Amaxa protocol.…”

Section: Electroporationmentioning

confidence: 99%

Meganucleases can restore the reading frame of a mutated dystrophin

et al. 2010

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Mutations in Duchenne muscular dystrophy (DMD) are either inducing a nonsense codon or a frameshift. Meganucleases (MGNs) can be engineered to induce double-strand breaks (DSBs) at specific DNA sequences. These breaks are repaired by homologous recombination or by non-homologous end joining (NHEJ), which results in insertions or deletions (indels) of a few base pairs. To verify whether MGNs could be used to restore the normal reading frame of a dystrophin gene with a frameshift mutation, we inserted in a plasmid coding for the dog m-dystrophin sequences containing a MGN target. The number of base pairs in these inserted sequences changed the reading frame. One of these modified target m-dystrophin plasmids and an appropriate MGN were then transfected in 293FT cells. The MGN induced micro-deletion or micro-insertion in the m-dystrophin that restored dystrophin expression. MGNs also restored m-dystrophin expression in myoblasts in vitro and in muscle fibers in vivo. The mutation of the targeted m-dystrophin was confirmed by PCR amplification followed by digestion with the Surveyor enzyme and by cloning and sequencing of the amplicons. These experiments are thus a proof of principle that MGNs that are adequately engineered to target appropriate sequences in the human dystrophin gene should be able to restore the normal reading frame of that gene in DMD patients with an out-of-frame deletion. New MGNs engineered to target a sequence including or near nonsense mutation could also be used to delete it.

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PhiC31 Integrase for Modification of Stem Cells

Jung

Calos

2009

Emerging Technology Platforms for Stem Cells

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Nucleofection of muscle-derived stem cells and myoblasts with ϕC31 integrase: stable expression of a full-length-dystrophin fusion gene by human myoblasts

Cited by 74 publications

References 31 publications

Dystrophin expression in host muscle following transplantation of muscle precursor cells modified with the phiC31 integrase

Dystrophin expression in host muscle following transplantation of muscle precursor cells modified with the phiC31 integrase

Meganucleases can restore the reading frame of a mutated dystrophin

PhiC31 Integrase for Modification of Stem Cells

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