Transfection of airway epithelium by stable PEGylated poly-l-lysine DNA nanoparticles in vivo

Ziady, Assem-Galal; Gedeon, Christopher R.; Miller, Timothy J.; Quan, William; Payne, Jennifer M.; Hyatt, Susannah L.; Fink, Tamara L.; Muhammad, Osman; Oette, Sharon M.; Kowalczyk, Tomasz; Pasumarthy, Murali K.; Moen, Robert C.; Cooper, Mark J.; Davis, Pamela B.

doi:10.1016/j.ymthe.2003.07.007

Cited by 156 publications

(181 citation statements)

References 29 publications

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“…[36][37][38] The most successful cases occur after intranasal or intratracheal administration, when targeting airway epithelial cells. 3,5,9,39 Tissues containing nondividing cells (as in muscle) or slow mitotic cells (as in the liver) are very attractive targets because pDNA can remain for a long time inside the cells. 40 In relation to the relatively fast kinetics seen here, we do not exclude the possibility that the decrease in expression after 5-7 days may be indicative of toxicity.…”

Section: Discussionmentioning

confidence: 99%

“…For this purpose, DNA condensation is a recurrent requisite for this type of nonviral therapeutic approach. 5,[8][9][10][11][12] Bloomfield 13 has defined DNA condensation as the collapse of extended DNA chains into compact, orderly particles containing only one or a few molecules. Typically, this process results from a neutralization of the negative charges of the DNA phosphate groups with transition into the ordered phase that occurs when 90% of charges are neutralized.…”

Section: Introductionmentioning

confidence: 99%

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Fatty acid–spermine conjugates as DNA carriers for nonviral in vivo gene delivery

et al. 2009

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The lack of efficient in vivo gene delivery is a well-known shortcoming of nonviral delivery vectors, in particular of chemical vectors. We developed a series of novel nonviral carriers for plasmid-based in vivo gene delivery. This new transport device is based on the assembly of DNA plasmids with synthetic derivatives of naturally occurring moleculesfatty acid-spermine conjugates (or lipospermines). We tested the ability of these fatty acid conjugates to interact with plasmid DNA (pDNA) and found that they formed DNA nanocomplexes, which are protected from DNase I degradation. This protection was shown to directly correlate with the length of the aliphatic component. However, this increase in the length of the hydrocarbon chain resulted in increased toxicity. The cationic lipids used for transfection typically have a C 16 and C 18 hydrocarbon chain. Interestingly, toxicity studies, together with further characterization studies, suggested that the two most suitable candidates for in vivo delivery are those with the shortest hydrocarbon chain, butanoyl-and decanoylspermine. Morphological characterization of DNA nanocomplexes resulting from these lipospermines showed the formation of a homogenous population, with the diameter ranging approximately from 40 to 200 nm. Butanoylspermine was found to be the most promising carrier from this series, resulting in a significantly increased gene expression, in relation to naked plasmid, in both tissues herein targeted (dermis and M. tibialis anterior). Thus, we established a correlation between the in vitro properties of the ensuing DNA nanocarriers and their efficient in vivo gene expression.

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Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Fatty acid–spermine conjugates as DNA carriers for nonviral in vivo gene delivery

et al. 2009

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“…35 The luciferase expression achieved by our simple nonviral system approaches that of recombinant Sendai virus in the nose 36 and is comparable to that achieved with pDNA/PEI and pDNA/CK30PEG10K. 37 Unlike viral vectors, pDNA alone is not proinflammatory, especially when the CpG dinucleotides are eliminated. 38 It could therefore be repeatedly administered in the airway.…”

Section: Discussionmentioning

confidence: 66%

Mechanism of efficient transfection of the nasal airway epithelium by hypotonic shock

2005

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The main barrier to gene transfer in the airway epithelium is the low rate of apical endocytosis limiting naked DNA uptake. Deionized water is known to stimulate the exocytosis of numerous intracellular vesicles during hypotonic cell swelling, in order to expand plasma membrane and prevent cell lysis. This is followed by the phase of regulatory volume decrease (RVD), during which the excess plasma membrane is retrieved by intensive endocytosis. Here we show that the more hypotonic the DNA solution, the higher the transfection of the nasal tissue. P2 receptors are known to be involved in RVD and we demonstrate that some P2 agonists and a P2 antagonist impair transfection in a time-dependent manner. Our study strongly suggests that the nasal airway epithelial cells take up plasmid DNA in deionized water during RVD, within approximately half an hour. Our simple gene delivery system may constitute a promising method for respiratory tract gene therapy.

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“…The development and characterization of such second-generation complexes is in progress. 24 Also, our data suggest that re-engineering the plasmid DNA construct to eliminate promoters prone to silencing (eg, by substitution of a eukaryotic promoter) might well extend the duration of expression. Antibody responses to the complexes, when they occur, were low titer and did not prevent subsequent transfection with sec-R-targeted complexes.…”

Section: Discussionmentioning

confidence: 79%

Defining strategies to extend duration of gene expression from targeted compacted DNA vectors

et al. 2004

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Gene transfer complexes containing poly-L-lysine (poly-K) and DNA with ligands directed at the serpin enzyme complex receptor (sec-R) deliver reporter genes to receptor-bearing cells in vivo. Expression lasts for about 30 days, when complexes containing long-chain poly-K are used. Extending the duration of expression would be desirable if correction of genetic defects is the goal. To test whether the mechanism by which expression is extinguished was due to an immune response to the transgene, or the loss of the transgene, we conducted two experiments. In the first, we injected sec-Rtargeted lacZ complexes intravenously (i.v.) into mice genetically engineered to express this gene briefly during development. These mice, who should recognize the protein as 'self', also extinguished lacZ expression after 30 days. In a second experiment, we injected immunodeficient animals with sec-R-targeted human factor IX complexes. A similar temporal pattern of expression was observed in Rag-1 À/À mice, in whom expression also extinguished by 40 days. Moreover, factor IX plasmid DNA was detected in the lung and spleen 50 days after injection of complexes, suggesting that not all cells which had taken up the transgene had been destroyed. Thus, the host's immune response to the transgene may not account for the loss of reporter gene expression from these molecular conjugates. We further tested whether repeat administration of sec-R-targeted complexes will be limited by host immune responses. Mice were pre-dosed twice with sec-R-targeted complexes containing lacZ over a 40-day period. We then injected the animals i.v. with sec-R-targeted human factor IX complexes and measured gene expression and antibody production. Although 14 of 36 animals displayed low-titer antibodies to the ligand in targeted complex, expression levels were unaffected compared with virgin dosing. When the complexes were administered three times intranasally (n ¼ 10), no antibodies against the complex were detected in blood. Plasma from mice dosed with saline, nontargeted complex or naked DNA did not react with the ligand, ligand-poly K conjugate or targeted complex. All animals exhibiting human factor IX expression developed antibodies to that transgene by 21 days. Thus, at least three repeat administrations of sec-R-directed molecular conjugates are possible, provided that immune responses to the transgene itself are not limiting.

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Transfection of airway epithelium by stable PEGylated poly-l-lysine DNA nanoparticles in vivo

Cited by 156 publications

References 29 publications

Fatty acid–spermine conjugates as DNA carriers for nonviral in vivo gene delivery

Fatty acid–spermine conjugates as DNA carriers for nonviral in vivo gene delivery

Mechanism of efficient transfection of the nasal airway epithelium by hypotonic shock

Defining strategies to extend duration of gene expression from targeted compacted DNA vectors

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