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Use of bicistronic vectors in combination with flow cytometry to screen for effective small interfering RNA target sequences.

机译:双顺反子载体与流式细胞仪结合使用以筛选有效的小干扰RNA靶序列。

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摘要

The efficacy and specificity of small interfering RNAs (siRNAs) are largely dependent on the siRNA sequence. Since only empirical strategies are currently available for predicting these parameters, simple and accurate methods for evaluating siRNAs are needed. To simplify such experiments, target genes are often tagged with reporters for easier readout. Here, we used a bicistronic vector expressing a target gene and green fluorescent protein (GFP) to create a system in which the effect of an siRNA sequence was reflected in the GFP expression level. Cells were transduced with the bicistronic vector, expression vectors for siRNA and red fluorescent protein (RFP). Flow cytometric analysis of the transduced cells revealed that siRNAs for the target gene silenced GFP from the bicistronic vector, but did not silence GFP transcribed without the target gene sequence. In addition, the mean fluorescence intensities of GFP on RFP-expressing cells correlated well with the target gene mRNA and protein levels. These results suggest that this flow cytometry-based method enables us to quantitatively evaluate the efficacy and specificity of siRNAs. Because of its simplicity and effectiveness, this method will facilitate the screening of effective siRNA target sequences, even in high-throughput applications.
机译:小干扰RNA(siRNA)的功效和特异性在很大程度上取决于siRNA序列。由于目前只有经验策略可用于预测这些参数,因此需要简单而准确的方法来评估siRNA。为了简化此类实验,通常将标靶基因标记有报告基因,以便于读出。在这里,我们使用表达靶基因和绿色荧光蛋白(GFP)的双顺反子载体创建了一个系统,其中siRNA序列的作用反映在GFP表达水平上。用双顺反子载体,siRNA表达载体和红色荧光蛋白(RFP)转导细胞。对转导细胞的流式细胞仪分析表明,目标基因的siRNA使双顺反子载体的GFP沉默,但没有使没有目标基因序列的GFP沉默。另外,在表达RFP的细胞上GFP的平均荧光强度与靶基因的mRNA和蛋白质水平很好地相关。这些结果表明,这种基于流式细胞仪的方法使我们能够定量评估siRNA的功效和特异性。由于其简单性和有效性,即使在高通量应用中,该方法也将有助于筛选有效的siRNA靶序列。

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