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首页> 外文期刊>National Academy Science Letters >RNAi (RNA Interference) Vectors for Functional Genomics Study in Plants
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RNAi (RNA Interference) Vectors for Functional Genomics Study in Plants

机译:用于植物功能基因组学研究的RNAi(RNA干扰)载体

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The discovery of RNA interference (RNAi) has revolutionized gene silencing for basic as well as applied studies. RNAi is a homology-dependent gene silencing mechanism, triggered by the introduction of double-stranded RNA (dsRNA) molecule. Since it can specifically suppress function of the targeted gene, the technique has been very useful in functional genomic studies. For efficient knock-down of the targeted gene, Gateway cloning based RNAi Silencing (pRISI) vector was developed. When a target gene-specific trigger fragment is cloned as inverted repeats in the pRISI vector, it produces a hairpin containing RNA transcribed from a CaMV35S (in case of pRISI-Ca) or from an ubiquitin (in case of pRISI-Ub) promoter. Function of the pRISI-Ca vector was confirmed by RNAi-mediated gene silencing experiment in Arabidopsis thaliana for At2g30350 gene which was found to be involved in repair of methylated DNA. A similar vector, pRISI-Ub was also developed for gene silencing studies in monocotyledonous plants. Its function was successfully demonstrated by transient suppression of GUS (UidA) gene co-bombarded with GUS-RNAi construct in wheat leaf. The vectors would be useful in rapid and easy preparation of RNAi constructs for reverse genetic studies for functional genomics in plants.
机译:RNA干扰(RNAi)的发现彻底改变了基因沉默的基础研究和应用研究。 RNAi是一种依赖同源性的基因沉默机制,可通过引入双链RNA(dsRNA)分子来触发。由于它可以特异性抑制靶基因的功能,因此该技术在功能基因组研究中非常有用。为了有效敲除靶基因,开发了基于Gateway克隆的RNAi沉默(pRISI)载体。当靶基因特异性触发片段以反向重复序列克隆到pRISI载体中时,它会产生一个发夹,该发夹含有从CaMV35S(对于pRISI-Ca而言)或从泛素(对于pRISI-Ub)启动子转录的RNA。通过RNAi介导的拟南芥At2g30350基因的基因沉默实验证实了pRISI-Ca载体的功能,该基因被发现与甲基化DNA的修复有关。还开发了类似的载体pRISI-Ub用于单子叶植物的基因沉默研究。通过瞬时抑制GUS(UidA)基因与小麦叶片中的GUS-RNAi构建体共同轰击,成功证明了其功能。该载体可用于快速简便地制备RNAi构建体,用于植物功能基因组学的反向遗传研究。

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