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Intravital Fluorescence Imaging of Small Interfering RNA–Mediated Gene Repression in a Dual Reporter Melanoma Xenograft Model

机译:小报告RNA黑色素瘤异种移植模型中的小干扰RNA介导的基因抑制的玻璃体内荧光成像。

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摘要

Development of RNA interference (RNAi)-based therapeutics has been hampered by the lack of effective and efficient means of delivery. Reliable model systems for screening and optimizing delivery of RNAi-based agents in vivo are crucial for preclinical research aimed at advancing nucleic acid-based therapies. We describe here a dual fluorescent reporter xenograft melanoma model prepared by intradermal injection of human A375 melanoma cells expressing tandem tomato fluorescent protein (tdTFP) containing a small interfering RNA (siRNA) target site as well as enhanced green fluorescent protein (EGFP), which is used as a normalization control. Intratumoral injection of a siRNA specific to the incorporated siRNA target site, complexed with a cationic lipid that has been optimized for in vivo delivery, resulted in 65%±11% knockdown of tdTFP relative to EGFP quantified by in vivo imaging and 68%±10% by reverse transcription–quantitative polymerase chain reaction. No effect was observed with nonspecific control siRNA treatment. This model provides a platform on which siRNA delivery technologies can be screened and optimized in vivo.
机译:由于缺乏有效的传递手段,阻碍了基于RNA干扰(RNAi)疗法的开发。用于筛选和优化体内基于RNAi的药物的可靠模型系统对于旨在推进基于核酸的疗法的临床前研究至关重要。我们在这里描述了一种双重荧光报告基因异种移植物黑色素瘤模型,该模型是通过皮内注射人A375黑色素瘤细胞而制备的,该细胞表达了含有小的干扰RNA(siRNA)目标位点以及增强型绿色荧光蛋白(EGFP)的串联番茄荧光蛋白(tdTFP)。用作规范化控件。瘤内注射对掺入的siRNA靶位点特异的siRNA,并与已针对体内递送进行优化的阳离子脂质复合,相对于通过体内成像定量的EGFP,tdTFP的敲除率达到65%±11% %通过逆转录定量聚合酶链反应。用非特异性对照siRNA处理未观察到效果。该模型提供了一个平台,可在其中筛选和优化siRNA体内递送技术。

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