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Stabilizing of plasmid DNA in vivo by PEG-modified cationic gold nanoparticles and the gene expression assisted with electrical pulses

机译:PEG修饰的阳离子金纳米粒子在体内稳定质粒DNA并通过电脉冲辅助基因表达

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This study aimed to investigate the benefits of combining the use of PEG-modified cationic gold nanoparticles with electroporation for in vivo gene delivery. PEG-modified cationic gold nanoparticles were prepared by NaBH4 reduction of HAuCl4 in the presence of 2-aminoethanethiol and mPEG-SH. Zeta-potential of the particles was nearly neutral (+0.1 mV). After forming complexes with plasmid DNA at a w/w ratio of 8.4, nanoparticle complexes were 90 nm for at least 60 min and showed a negative zeta-potential. After intravenous injection of DNA-nanoparticle complexes, 20% of gold were detected in blood at 120 min after injection and 5% of DNA were observed in blood after 5 min, suggesting that PEG-modified nanoparticles were stably circulating in the blood flow, but some of the DNA bound to particles degraded during circulation. When electroporation was applied to a lobe of the liver following injection of DNA-nanoparticle complexes, significant gene expression was specifically observed in the pulsed lobe. We concluded that PEG-modified nanoparticles maintained DNA more stably in the blood flow than in the case of naked DNA and electroporation assisted in restricted gene expression of circulating DNA in limited areas of the liver. (c) 2006 Elsevier B.V. All rights reserved.
机译:这项研究旨在研究将PEG修饰的阳离子金纳米粒子与电穿孔结合用于体内基因递送的益处。在2-氨基乙硫醇和mPEG-SH的存在下,通过NaBH4还原HAuCl4制备PEG修饰的阳离子金纳米颗粒。颗粒的ζ电位几乎是中性的(+ 0.1mV)。与质粒DNA以8.4的w / w比形成复合物后,纳米粒子复合物在90 nm处至少作用60分钟,并显示出负的ζ电势。静脉内注射DNA-纳米颗粒复合物后,注射后120分钟在血液中检测到20%的金,5分钟后在血液中观察到5%的DNA,这表明PEG修饰的纳米颗粒在血流中稳定循环,但一些与颗粒结合的DNA在循环过程中会降解。注射DNA-纳米粒子复合物后,在肝叶上进行电穿孔时,在脉冲叶中特别观察到了显着的基因表达。我们得出的结论是,与裸露的DNA相比,PEG修饰的纳米粒子在血流中更稳定地维持DNA,而电穿孔则有助于在肝脏有限区域内限制循环DNA的基因表达。 (c)2006 Elsevier B.V.保留所有权利。

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