Literature DB >> 8932437

The influence of sodium glycocholate and other additives on the in vivo transfection of plasmid DNA in the lungs.

D J Freeman1, R W Niven.   

Abstract

PURPOSE: A plasmid containing the luciferase 'marker' cDNA was constructed to test non viral gene delivery formulations in vivo.
METHODS: A scale up procedure was devised to produce up to gram quantities of plasmid. Sufficient quantities were generated to process and test the DNA with various additives and to generate a spray-dried powder formulation of the plasmid. Male Sprague-Dawley rats (250 g) were intratracheally instilled with 200-250 microl of solution containing 200 microg plasmid +/- lipid [DC Chol:DOPE 1:1 molar (2mg/kg)] growth factors [KGF (10 mg/kg), EGF (5 mg/kg)], permeation enhancers [sodium glycocholate (0.01 to 10% w/v)), sodium deoxycholate (1% w/v), beta-cyclodextrin (1% w/v)], surfactant [Tween 80 (1% w/v)], a mucolytic [N-acetylcysteine (10% w/v)] and positively charged synthetic polymers [PVAVAM 6 and 14%]. Animals were sacrificed 24 hr post-dose and the lungs were assayed for luciferase using a chemiluminescent assay.
RESULTS: The relative ability of the materials to promote luciferase production in the lungs was permeation enhancer >> DNA alone > or = lipid, mucolytic, surfactant, growth factor > polymer. Protein production in the lungs ranged from 10 times below the DNA control (approximately 16 pg) using the polymers (approximately 1.5 pg) to approximately 125 times greater than the control using the permeation enhancer (approximately 2050 pg). The transfection capabilities of the majority of additives was low. The enhancing effects of sodium glycocholate were dose-dependent and perhaps associated with the critical micelle concentration. Although the bile salt was the most successful of the tested compounds, it resulted in significant mortality when used at concentrations greater than 1% w/v.
CONCLUSIONS: The results suggest that transfection can be significantly enhanced by additives such as NaGC but some toxicity may be unavoidable.

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Year:  1996        PMID: 8932437     DOI: 10.1023/a:1016078728202

Source DB:  PubMed          Journal:  Pharm Res        ISSN: 0724-8741            Impact factor:   4.200


  21 in total

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4.  Use of 2-hydroxypropyl-beta-cyclodextrin as a solubilizing and stabilizing excipient for protein drugs.

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5.  Systemic absorption and activity of recombinant consensus interferons after intratracheal instillation and aerosol administration.

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6.  Retinoic acid stimulates mouse lung development by a mechanism involving epithelial-mesenchymal interaction and regulation of epidermal growth factor receptors.

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7.  A novel cationic liposome reagent for efficient transfection of mammalian cells.

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8.  Suppression of in vivo tumorigenicity of human lung cancer cells by retrovirus-mediated transfer of the human tumor necrosis factor-alpha cDNA.

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9.  Import of firefly luciferase into mammalian peroxisomes in vivo requires nucleoside triphosphates.

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5.  Design and evaluation of thioalkylated mannose-modified dendrimer (G3)/α-cyclodextrin conjugates as antigen-presenting cell-selective siRNA carriers.

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6.  Safety Assessment of Formulation Vehicles Following Intravitreal Administration in Rabbits.

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Review 7.  Cyclodextrins in non-viral gene delivery.

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Review 8.  Polymers for DNA delivery.

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  8 in total

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