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High-Throughput Construction of Intron-Containing Hairpin RNA Vectors for RNAi in Plants

机译:植物中RNAi的含内含子发夹RNA载体的高通量构建

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摘要

With the wide use of double-stranded RNA interference (RNAi) for the analysis of gene function in plants, a high-throughput system for making hairpin RNA (hpRNA) constructs is in great demand. Here, we describe a novel restriction-ligation approach that provides a simple but efficient construction of intron-containing hpRNA (ihpRNA) vectors. The system takes advantage of the type IIs restriction enzyme BsaI and our new plant RNAi vector pRNAi-GG based on the Golden Gate (GG) cloning. This method requires only a single PCR product of the gene of interest flanked with BsaI recognition sequence, which can then be cloned into pRNAi-GG at both sense and antisense orientations simultaneously to form ihpRNA construct. The process, completed in one tube with one restriction-ligation step, produced a recombinant ihpRNA with high efficiency and zero background. We demonstrate the utility of the ihpRNA constructs generated with pRNAi-GG vector for the effective silencing of various individual endogenous and exogenous marker genes as well as two genes simultaneously. This method provides a novel and high-throughput platform for large-scale analysis of plant functional genomics.
机译:随着双链RNA干扰(RNAi)在植物基因功能分析中的广泛应用,对制备发夹RNA(hpRNA)构建体的高通量系统的需求很大。在这里,我们描述了一种新型的限制性连接方法,该方法提供了一个简单而有效的含内含子hpRNA(ihpRNA)载体的构建方法。该系统利用II型限制酶BsaI和基于金门(GG)克隆的新植物RNAi载体pRNAi-GG。该方法仅需要侧翼为BsaI识别序列的目标基因的单个PCR产物,然后可以同时以有义和反义方向将其克隆到pRNAi-GG中以形成ihpRNA构建体。该过程在一个试管中完成,只需一个限制性连接步骤,就可以生产出高效且零背景的重组ihpRNA。我们证明了用pRNAi-GG载体产生的ihpRNA构建体的效用,可同时有效沉默各种个体内源性和外源性标记基因以及两个基因。该方法为大规模分析植物功能基因组学提供了一种新颖且高通量的平台。

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