Transformation of mammalian cells with an amplifiable dominant-acting gene.

Wigler, Michael; Perucho, Manuel; Kurtz, David T.; Dana, Sharon L.; Pellicer, Ángel Antonio Blasco; Axel, Richard; Silverstein, Saul

doi:10.1073/pnas.77.6.3567

Cited by 145 publications

(64 citation statements)

References 21 publications

(22 reference statements)

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“…Surprisingly, cultures cotransfected with pJM17 and cultures infected with adenovirus-2 produced similar amounts of AAV lacZ vector. pJM17 does produce extremely low levels of adenovirus when transfected into 293 cells in the presence or absence of AAV vector and helper plasmids (typically 5 × 10 6 cells transfected with 10 g of pJM17 by the calcium phosphate method 24 produce a total of 10 4 plaque forming units (p.f.u.)). This is due to an infrequent rearrangement of the circular genome that occurs in a small number of transfected cells.…”

Section: Resultsmentioning

confidence: 99%

Adeno-associated virus vectors can be efficiently produced without helper virus

et al. 1998

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The purpose of this work was to develop an efficient Therefore the minimum set of genes required to produce method for the production of adeno-associated virus (AAV) AAV helper activity equivalent to that provided by adenvectors in the absence of helper virus. The adenovirus ovirus infection consists of, or is a subset of, the following regions that mediate AAV vector replication were identified genes: the E4orf6 gene, the 72-M r , E2A protein gene, the and assembled into a helper plasmid. These included the VA RNA genes and the E1 region. AAV vector preparations VA, E2A and E4 regions. When this helper plasmid was made with adenovirus and by the helper virus-free method cotransfected into 293 cells, along with plasmids encoding were essentially indistinguishable with respect to particle the AAV vector, and rep and cap genes, AAV vector was density, particle to infectivity ratio, capsimer ratio and produced as efficiently as when using adenovirus infection efficiency of muscle transduction in vivo. Only AAV vector as a source of help. CMV-driven constructs expressing the preparations made by the helper virus-free method were E4orf6 and the 72-M r , E2A proteins were able to funcnot reactive with anti-adenovirus sera. tionally replace the E4 and E2A regions, respectively.

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Section: Resultsmentioning

confidence: 99%

Adeno-associated virus vectors can be efficiently produced without helper virus

et al. 1998

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“…The expression casette contained a CMV promoter, a chimeric intron composed of a CMV splice donor and a human globin splice acceptor site, human growth hormone polyadenylation sequence, and flanking AAV ITRs (inverted terminal repeats) (39).…”

Section: Construction Of Aav-aadc Plasmidmentioning

confidence: 99%

Convection-Enhanced Delivery of AAV Vector in Parkinsonian Monkeys; In Vivo Detection of Gene Expression and Restoration of Dopaminergic Function Using Pro-drug Approach

Bankiewicz

Eberling

Kohutnicka

et al. 2000

Experimental Neurology

379

236

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Using an approach that combines gene therapy with aromatic L-amino acid decarboxylase (AADC) gene and a pro-drug (L-dopa), dopamine, the neurotransmitter involved in Parkinson's disease, can be synthesized and regulated. Striatal neurons infected with the AADC gene by an adeno-associated viral vector can convert peripheral L-dopa to dopamine and may therefore provide a buffer for unmetabolized L-dopa. This approach to treating Parkinson's disease may reduce the need for L-dopa/carbidopa, thus providing a better clinical response with fewer side effects. In addition, the imbalance in dopamine production between the nigrostriatal and mesolimbic dopaminergic systems can be corrected by using AADC gene delivery to the striatum. We have also demonstrated that a fundamental obstacle in the gene therapy approach to the central nervous system, i.e., the ability to deliver viral vectors in sufficient quantities to the whole brain, can be overcome by using convection-enhanced delivery. Finally, this study demonstrates that positron emission tomography and the AADC tracer, 6-[ 18 F]fluoro-Lm-tyrosine, can be used to monitor gene therapy in vivo. Our therapeutic approach has the potential to restore dopamine production, even late in the disease process, at levels that can be maintained during continued nigrostriatal degeneration.

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“…For plasmid modification, "C-labelled MMS or MNU (Amersham, Bucks, England) in DMSO solution at the indicated concentrations were reacted with 2 pg of plasmid pHSV106 DNA [7,8] Mouse LTK-/aprtcells [9], maintained as monolayers in Dulbecco's modified Eagle's medium (Gibco) with 10% calf serum and antibiotics, were routinely passaged 1:3 once per week. 4 x lo5 mouse LTK-cells were seeded 24 h before transformation and transfections were carried out using the calcium phosphate-DNA coprecipitation technique [ 11.…”

Section: Methodsmentioning

confidence: 99%

DNA‐mediated gene transfer as an indicator of DNA damage and its repair by recipient cells

Ireland

Stewart

1987

FEBS Letters

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Preparations of plasmid containing the thymidine kinase gene (pHSV106) were treated with the alkylating agents methyl methanesulphonate or N-methyl-N-nitrosourea prior to transfection into thymidine kinasedeficient mouse L-cells using the DNA-calcium phosphate co-precipitation technique. Relative to transfection with unmodified plasmid, a reduced transformation efficiency was observed using alkylation-damaged plasmid, N-methyl-N-nitrosourea causing the greatest inhibition. Treatment of recipient cells with arabinosyl cytosine or dideoxythymidine during the expression period following transfection by the 'damaged' plasmid reduced transformation efficiency, suggesting that DNA repair 4-6 h post-transfection was required for gene expression.

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Transformation of mammalian cells with an amplifiable dominant-acting gene.

Cited by 145 publications

References 21 publications

Adeno-associated virus vectors can be efficiently produced without helper virus

Adeno-associated virus vectors can be efficiently produced without helper virus

Convection-Enhanced Delivery of AAV Vector in Parkinsonian Monkeys; In Vivo Detection of Gene Expression and Restoration of Dopaminergic Function Using Pro-drug Approach

DNA‐mediated gene transfer as an indicator of DNA damage and its repair by recipient cells

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