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拟南芥中一种微小RNA介导的串联反式作用小干扰RNA级联的生物信息学预测与实验验证

Bioinformatic prediction and experimental validation of a microRNA-directed tandem trans-acting siRNA cascade in Arabidopsis.

作者信息

Chen Ho-Ming, Li Yi-Hang, Wu Shu-Hsing

机构信息

Institute of Plant and Microbial Biology, Academia Sinica, Taipei 11529, Taiwan.

出版信息

Proc Natl Acad Sci U S A. 2007 Feb 27;104(9):3318-23. doi: 10.1073/pnas.0611119104. Epub 2007 Feb 20.

Abstract

Small RNAs play pivotal roles in regulating gene expression in higher eukaryotes. Among them, trans-acting siRNAs (ta-siRNAs) are a class of small RNAs that regulate plant development. The biogenesis of ta-siRNA depends on microRNA-targeted cleavage followed by the DCL4-mediated production of small RNAs phased in 21-nt increments relative to the cleavage site on both strands. To find TAS genes, we have used these characteristics to develop the first computational algorithm that allows for a comprehensive search and statistical evaluation of putative TAS genes from any given small RNA database. A search in Arabidopsis small RNA massively parallel signature sequencing (MPSS) databases with this algorithm revealed both known and previously unknown ta-siRNA-producing loci. We experimentally validated the biogenesis of ta-siRNAs from two PPR genes and the trans-acting activity of one of the ta-siRNAs. The production of ta-siRNAs from the identified PPR genes was directed by the cleavage of a TAS2-derived ta-siRNA instead of by microRNAs as was reported previously for TAS1a, -b, -c, TAS2, and TAS3 genes. Our results indicate the existence of a small RNA regulatory cascade initiated by miR173-directed cleavage and followed by the consecutive production of ta-siRNAs from two TAS genes.

摘要

小RNA在高等真核生物基因表达调控中发挥着关键作用。其中,反式作用小干扰RNA(ta-siRNA)是一类调控植物发育的小RNA。ta-siRNA的生物合成依赖于微小RNA靶向切割,随后由DCL4介导产生相对于切割位点在两条链上以21个核苷酸递增的小RNA。为了寻找TAS基因,我们利用这些特性开发了首个计算算法,该算法能够对来自任何给定小RNA数据库的假定TAS基因进行全面搜索和统计评估。使用该算法在拟南芥小RNA大规模平行签名测序(MPSS)数据库中进行搜索,发现了已知和先前未知的产生ta-siRNA的位点。我们通过实验验证了来自两个PPR基因的ta-siRNA的生物合成以及其中一个ta-siRNA的反式作用活性。从已鉴定的PPR基因产生ta-siRNA是由源自TAS2的ta-siRNA的切割所引导,而不是像先前报道的TAS1a、-b、-c、TAS2和TAS3基因那样由微小RNA引导。我们的结果表明存在一个由miR173引导切割起始,随后从两个TAS基因连续产生ta-siRNA的小RNA调控级联反应。

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