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首页> 外文期刊>Human gene therapy >Gene gun bombardment with DNA-coated gold particles is a potential alternative to hydrodynamics-based transfection for delivering genes into superficial hepatocytes.
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Gene gun bombardment with DNA-coated gold particles is a potential alternative to hydrodynamics-based transfection for delivering genes into superficial hepatocytes.

机译:基因枪轰击用涂有DNA的金颗粒轰击是将基因传递到浅表肝细胞中的基于水动力学的转染的潜在替代方法。

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Although in vivo nonviral gene delivery to the liver is critical for hepatic gene therapy, there are a number of technical obstacles. Enhanced green fluorescent protein (EGFP)-encoding DNA was coated onto gold particles (gold-DNA), dissolved in phosphate-buffered saline (pure DNA), and prepared as a polymer adjuvant (jetPEI)-galactosidase solution (polymer-DNA). Murine liver transfection was attempted by nonviral approaches, which included hydrodynamics-based transfection (HBT) of pure DNA, transport and transhepatic injection of polymer-DNA, and gene gun bombardment with pure DNA, gold-DNA, and polymer-DNA. Only HBT and gene gun bombardment yielded significant numbers of EGFP(+) hepatocytes. With the exception of the edge of the liver, HBT had a whole-liver transfection rate of 20% under optimized conditions. HBT resulted in marked hepatic infarctions, most prominently at the edge of the liver. For gene gun bombardment, the transfection rate was pressure dependent and limited to 15% for gold-DNA. Triple or quadruple bombardment at 30 psi resulted in a transfection rate comparable to that of a single bombardment at higher pressure, but was associated with minimal scattered hepatic necrosis. The EGFP(+) hepatocytes were located mainly in the superficial layers. We conclude that both HBT and gene gun bombardment yielded efficient murine hepatocyte transfection in vivo. Severe hepatic infarction impedes foreign gene expression in the superficial hepatocytes after HBT. Repeated bombardment with gold-DNA, using an accelerated particle gene gun at 30 psi, is a potential alternative to HBT for delivering genes to superficial hepatocytes in vivo, although gold-related hepatic necrosis is a persistent problem.
机译:尽管体内非病毒基因向肝脏的递送对于肝基因治疗至关重要,但存在许多技术障碍。将编码增强型绿色荧光蛋白(EGFP)的DNA包被在金颗粒(金DNA)上,溶解在磷酸盐缓冲液(纯DNA)中,并制成聚合物佐剂(jetPEI)-半乳糖苷酶溶液(聚合物-DNA)。通过非病毒方法尝试了鼠肝转染,包括纯DNA的基于流体动力学的转染(HBT),聚合物-DNA的转运和肝移植以及纯DNA,金-DNA和聚合物-DNA的基因枪轰击。仅HBT和基因枪轰击产生大量EGFP(+)肝细胞。在最佳条件下,除肝脏边缘外,HBT的全肝转染率为20%。 HBT导致明显的肝梗塞,最明显的是在肝边缘。对于基因枪轰击,转染率取决于压力,对于金DNA,转染率限制为15%。 30 psi的三倍或四倍轰击产生的转染率与高压下单次轰击的转染率相当,但与最小的散布性肝坏死有关。 EGFP(+)肝细胞主要位于浅层。我们得出的结论是,HBT和基因枪轰击均可在体内产生有效的鼠肝细胞转染。严重肝梗塞会阻止HBT后浅表肝细胞中外源基因的表达。尽管与金有关的肝坏死是一个长期存在的问题,但使用30 psi的加速粒子基因枪对金DNA的反复轰击是将HBT传递到体内浅表肝细胞的一种潜在替代HBT的方法。

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