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Live-cell imaging to compare the transfection and gene silencing efficiency of calcium phosphate nanoparticles and a liposomal transfection agent

机译:活细胞成像以比较磷酸钙纳米颗粒和脂质体转染剂的转染和基因沉默效率

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摘要

The processing of DNA (for transfection) and short interfering RNA (siRNA; for gene silencing), introduced into HeLa cells by triple-shell calcium phosphate nanoparticles, was followed by live-cell imaging. For comparison, the commercial liposomal transfection agent Lipofectamine was used. The cells were incubated with these delivery systems, carrying either enhanced green fluorescent protein (eGFP)-encoding DNA or siRNA against eGFP. In the latter case, HeLa cells that stably expressed eGFP were used. The expression of eGFP started after 5 h in the case of nanoparticles and after 4 h in the case of Lipofectamine. The corresponding times for gene silencing were 5 h (nanoparticles) and immediately after incubation (Lipofectamine). The expression of eGFP was notably enhanced 2–3 h after cell division (mitosis). In general, the transfection and gene silencing efficiencies of the nanoparticles were lower than those of Lipofectamime, even at a substantially higher dose (factor 20) of nucleic acids. However, the cytotoxicity of the nanoparticles was lower than that of Lipofectamine, making them suitable vectors for in vivo application.
机译:由三层磷酸钙钙纳米粒子导入HeLa细胞的DNA(用于转染)和短干扰RNA(用于基因沉默)的处理,然后是活细胞成像。为了比较,使用市售脂质体转染剂Lipofectamine。将细胞与这些传递系统一起孵育,并携带编码增强型绿色荧光蛋白(eGFP)的DNA或针对eGFP的siRNA。在后一种情况下,使用稳定表达eGFP的HeLa细胞。在纳米颗粒的情况下,eGFP的表达在5µh之后开始,而在Lipofectamine的情况下,则在4µh之后开始表达。基因沉默的相应时间为5小时(纳米颗粒),孵育后立即进行(Lipofectamine)。细胞分裂(有丝分裂)后2–3 ofh,eGFP的表达显着增强。通常,即使在显着更高剂量(20倍的核酸)下,纳米颗粒的转染和基因沉默效率也比脂质转染酶低。但是,纳米颗粒的细胞毒性低于脂转染胺,因此使其成为体内应用的合适载体。

著录项

  • 期刊名称 NPG Open Access
  • 作者

    S Chernousova; M Epple;

  • 作者单位
  • 年(卷),期 -1(24),5
  • 年度 -1
  • 页码 282–289
  • 总页数 8
  • 原文格式 PDF
  • 正文语种
  • 中图分类
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