Long-term efficient gene delivery using polyethylenimine with modified Tat peptide. Yamano, S., Dai, J., Hanatani, S., Haku, K., Yamanaka, T., Ishioka, M., Takayama, T., Yuvienco, C., Khapli, S., Moursi, A., M., & Montclare, J., K. Biomaterials, 35(5):1705-1715, 2014.
abstract   bibtex   
Polyethylenimine (PEI), a cationic polymer, has been widely studied and shown great promise as an efficient gene delivery vehicle. Likewise, the HIV-1 Tat peptide, a cell-permeable peptide, has been successfully used for intracellular gene delivery. To improve the favorable properties of these two vectors, we combine PEI with the modified Tat peptide sequence bearing histidine and cysteine residues (mTat). Invitro mTat/PEI-mediated transfection was evaluated by luciferase expression plasmid in two cell types. mTat/PEI produced significant improvement (≈5-fold) in transfection efficiency of both cell lines with little cytotoxicity when compared to mTat alone, PEI alone, or four commercial reagents. The particle size of mTat/PEI/DNA complex was significantly smaller than mTat or PEI alone, and it was correlated with higher transfection efficiency. Filipin III, an inhibitor of caveolae-mediated endocytosis, significantly inhibited mTat/PEI transfection. In contrast, chlorpromazine, an inhibitor of clathrin-mediated endocytosis, did not. This suggested caveolae-mediated endocytosis as the transfection mechanism. Furthermore, the results of invivo studies showed that animals administered mTat/PEI/DNA intramuscularly had significantly higher and longer luciferase expression (≈7 months) than those with mTat/DNA, PEI/DNA, or DNA alone, without any associated toxicity. The combination of mTat with PEI could significantly improve transfection efficiency, expanding the potential use as a non-viral gene vector both invitro and invivo. © 2013 Elsevier Ltd.
@article{
 title = {Long-term efficient gene delivery using polyethylenimine with modified Tat peptide},
 type = {article},
 year = {2014},
 identifiers = {[object Object]},
 keywords = {Gene delivery,Non-viral vector,Plasmid DNA,Polyethylenimine,Tat peptide,Transfection},
 pages = {1705-1715},
 volume = {35},
 id = {63c7cbbd-b10a-3413-a522-290c1616f239},
 created = {2015-12-14T19:51:28.000Z},
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 last_modified = {2017-03-14T12:30:08.401Z},
 read = {false},
 starred = {false},
 authored = {true},
 confirmed = {true},
 hidden = {false},
 citation_key = {Yamano2014},
 private_publication = {false},
 abstract = {Polyethylenimine (PEI), a cationic polymer, has been widely studied and shown great promise as an efficient gene delivery vehicle. Likewise, the HIV-1 Tat peptide, a cell-permeable peptide, has been successfully used for intracellular gene delivery. To improve the favorable properties of these two vectors, we combine PEI with the modified Tat peptide sequence bearing histidine and cysteine residues (mTat). Invitro mTat/PEI-mediated transfection was evaluated by luciferase expression plasmid in two cell types. mTat/PEI produced significant improvement (≈5-fold) in transfection efficiency of both cell lines with little cytotoxicity when compared to mTat alone, PEI alone, or four commercial reagents. The particle size of mTat/PEI/DNA complex was significantly smaller than mTat or PEI alone, and it was correlated with higher transfection efficiency. Filipin III, an inhibitor of caveolae-mediated endocytosis, significantly inhibited mTat/PEI transfection. In contrast, chlorpromazine, an inhibitor of clathrin-mediated endocytosis, did not. This suggested caveolae-mediated endocytosis as the transfection mechanism. Furthermore, the results of invivo studies showed that animals administered mTat/PEI/DNA intramuscularly had significantly higher and longer luciferase expression (≈7 months) than those with mTat/DNA, PEI/DNA, or DNA alone, without any associated toxicity. The combination of mTat with PEI could significantly improve transfection efficiency, expanding the potential use as a non-viral gene vector both invitro and invivo. © 2013 Elsevier Ltd.},
 bibtype = {article},
 author = {Yamano, Seiichi and Dai, Jisen and Hanatani, Shigeru and Haku, Ken and Yamanaka, Takuto and Ishioka, Mika and Takayama, Tadahiro and Yuvienco, Carlo and Khapli, Sachin and Moursi, Amr M. and Montclare, Jin K.},
 journal = {Biomaterials},
 number = {5}
}
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