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Post-transcriptional Gene Silencing Induced by Short Interfering RNAs in Cultured Transgenic Plant Cells

机译:短干扰RNA在培养的转基因植物细胞中诱导的转录后基因沉默。

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Short interfering RNA (siRNA) is widely used for studying post-transcriptional gene silencing and holds great promise as a tool for both identifying function of novel genes and validating drug targets. Two siRNA fragments (siRNA-a and -b), which were designed against different specific areas of coding region of the same target green fluorescent protein (GFP) gene, were used to silence GFP expression in cultured gfp transgenic cells of rice (Oryza sativa L.; OS), cotton (Gossypium hirsutum L.; GH), Eraser fir [Abies fraseri (Pursh) Poir; AF], and Virginia pine (Pinus virginiana Mill.; PV). Differential gene silencing was observed in the bombarded transgenic cells between two siRNAs, and these results were consistent with the inactivation of GFP confirmed by laser scanning microscopy, Northern blot, and siRNA analysis in tested transgenic cell cultures. These data suggest that siRNA-mediated gene inactivation can be the siRNA specific in different plant species. These results indicate that siRNA is a highly specific tool for targeted gene knockdown and for establishing siRNA-mediated gene silencing, which could be a reliable approach for large-scale screening of gene function and drug target validation.
机译:短干扰RNA(siRNA)被广泛用于转录后基因沉默的研究,作为鉴定新基因功能和验证药物靶点的工具,具有广阔的前景。针对相同目标绿色荧光蛋白(GFP)基因编码区的不同特定区域设计的两个siRNA片段(siRNA-a和-b)用于沉默水稻培养的gfp转基因细胞(Oryza sativa)中GFP的表达L .; OS),棉花(Gossypium hirsutum L .; GH),橡皮擦[Abies fraseri(Pursh)Poir; AF]和弗吉尼亚松(Pinus virginiana Mill .; PV)。在两个siRNA轰击的转基因细胞中观察到差异的基因沉默,这些结果与在测试的转基因细胞培养物中通过激光扫描显微镜,Northern印迹和siRNA分析证实的GFP失活是一致的。这些数据表明,siRNA介导的基因失活可能是不同植物物种中特异的siRNA。这些结果表明,siRNA是用于靶向基因敲低和建立siRNA介导的基因沉默的高度特异性的工具,这可能是大规模筛选基因功能和药物靶标验证的可靠方法。

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