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Study on the efficiency of dsRNAs with increasing length in RNA-based silencing of the Fusarium CYP51 genes

机译:基于RNA CYP51基因RNA的沉默效率随着DSRNA效率的研究

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Previously, we have demonstrated that transgenic Arabidopsis and barley plants, expressing a 791 nucleotide (nt) dsRNA (CYP3RNA) that targets all three CYP51 genes (FgCYP51A, FgCYP51B, FgCYP51C) in Fusarium graminearum (Fg), inhibited fungal infection via a process designated as host-induced gene silencing (HIGS). More recently, we have shown that spray applications of CYP3RNA also protect barley from fungal infection via a process termed spray-induced gene silencing (SIGS). Thus, RNAi technology may have the potential to revolutionize plant protection in agriculture. Therefore, successful field application will require optimization of RNAi design necessary to maximize the efficacy of the RNA silencing construct for making RNAi-based strategies a realistic and sustainable approach in agriculture. Previous studies indicate that silencing is correlated with the number of siRNAs generated from a dsRNA precursor. To prove the hypothesis that silencing efficiency is correlated with the number of siRNAs processed out of the dsRNA precursor, we tested in a HIGS and SIGS approach dsRNA precursors of increasing length ranging from 400 nt to 1500 nt to assess gene silencing efficiency of individual FgCYP51 genes. Concerning HIGS-mediated disease control, we found that there is no significant correlation between the length of the dsRNA precursor and the reduction of Fg infection on CYP51-dsRNA-expressing Arabidopsis plants. Importantly and in clear contrast to HIGS, we measured a decrease in SIGS-mediated Fg disease resistance that significantly correlates with the length of the dsRNA construct that was sprayed, indicating that the size of the dsRNA interferes with a sufficient uptake of dsRNAs by the fungus.
机译:以前,我们已经证明了转基因拟南芥和大麦植物,表达靶向镰刀酸镰刀菌(FG)的所有三种CYP51基因(FGCOP51A,FGCOP51B,FGCOP51B,FGCOP51B,FGCOP51C),通过指定的方法抑制真菌感染作为宿主诱导的基因沉默(HIGS)。最近,我们已经表明,Cyp3RNA的喷涂应用还通过被称为喷雾诱导的基因沉默(SIG)的过程保护大麦免受真菌感染。因此,RNAI技术可能有可能彻底改变农业的植物保护。因此,成功的现场应用将需要优化RNAi设计,以最大限度地提高RNA沉默构建的效果,以使RNAi的战略成为农业的现实和可持续的方法。以前的研究表明,沉默与从DSRNA前体产生的SIRNA的数量相关。为了证明沉默效率与从DSRNA前体中加工的SIRNA的数量相关的假设,我们在HIGS和SIGs中测试了DsRNA前体,其增加的长度为400nt至1500nt以评估单个FGCYP51基因的基因沉默效率。关于HIGS介导的疾病控制,我们发现DSRNA前体的长度与CYP51-DSRNA表达拟南芥植物的FG感染之间没有显着相关性。重要的是,与Higs透明形成对比,我们测量了SIG介导的FG疾病抗性的降低,与喷射的DSRNA构建体的长度显着相关,表明DSRNA的大小干扰真菌的足够摄取的DSRNA 。

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