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Effective Silencing of Sry Gene with RNA Interference in Developing Mouse Embryos Resulted in Feminization of XY Gonad

机译:有效干扰沉默Sry基因与RNA干扰发展中的小鼠胚胎导致XY性腺女性化。

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摘要

Delivering siRNA or shRNA into the developing embryos is still a main challenge to use of RNAi in mammalian systems. Here we analyze several factors influencing RNAi-mediated silencing of Sry gene, which is a tightly controlled spatiotemporal expressed gene and only shortly expressed in developing mouse embryo gonad. A Sry gene-specific shRNAs expression vector (pSilencer4.1/Sry565) was constructed. The shRNA constructs were mixed with polyethylenimines (PEIs) to form a complex and then injected into pregnant mice though tail vein. Our results showed that Sry gene was downregulated significantly in developing embryos. Further study revealed that knocking-down of Sry expression resulted in feminization of gonad development in mouse embryos and the expression level of Sox9 and Wt1 gene was also significantly changed by downregulation of Sry. The transfection efficiency is associated with the amount of plasmid DNA injection, injection time, injection speed, and volume. Our studies suggest that transplacental RNAi could be implemented by tail vein injection of plasmid vector into pregnant mice.
机译:将siRNA或shRNA传递至发育中的胚胎仍然是在哺乳动物系统中使用RNAi的主要挑战。在这里,我们分析了几个影响RNAi介导的Sry基因沉默的因素,Sry基因是一个受到严格控制的时空表达基因,仅在发育中的小鼠胚胎性腺中短暂表达。构建了Sry基因特异性shRNAs表达载体(pSilencer4.1 / Sry565)。 shRNA构建体与聚乙烯亚胺(PEI)混合形成复合物,然后通过尾静脉注射到怀孕的小鼠中。我们的结果表明,Sry基因在发育中的胚胎中显着下调。进一步的研究表明,敲除Sry的表达会导致小鼠胚胎中性腺发育的女性化,而且Sry的下调也显着改变了Sox9和Wt1基因的表达水平。转染效率与质粒DNA注射量,注射时间,注射速度和体积有关。我们的研究表明,胎盘RNAi可以通过将尾巴的质粒载体注射到妊娠小鼠体内来实现。

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