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通过直接基因组测序鉴定拟南芥 MIR390a 前体加工缺陷突变体。

Identification of MIR390a precursor processing-defective mutants in Arabidopsis by direct genome sequencing.

机构信息

Molecular and Cellular Biology Program, Oregon State University, Corvallis, OR 97331, USA.

出版信息

Proc Natl Acad Sci U S A. 2010 Jan 5;107(1):466-71. doi: 10.1073/pnas.0913203107. Epub 2009 Dec 14.

Abstract

Transacting siRNA (tasiRNA) biogenesis in Arabidopsis is initiated by microRNA (miRNA) -guided cleavage of primary transcripts. In the case of TAS3 tasiRNA formation, ARGONAUTE7 (AGO7)-miR390 complexes interact with primary transcripts at two sites, resulting in recruitment of RNA-DEPENDENT RNA POLYMERASE6 for dsRNA biosynthesis. An extensive screen for Arabidopsis mutants with specific defects in TAS3 tasiRNA biogenesis or function was done. This yielded numerous ago7 mutants, one dcl4 mutant, and two mutants that accumulated low levels of miR390. A direct genome sequencing-based approach to both map and rapidly identify one of the latter mutant alleles was developed. This revealed a G-to-A point mutation (mir390a-1) that was calculated to stabilize a relatively nonpaired region near the base of the MIR390a foldback, resulting in misprocessing of the miR390/miR390* duplex and subsequent reduced TAS3 tasiRNA levels. Directed substitutions, as well as analysis of variation at paralogous miR390-generating loci (MIR390a and MIR390b), indicated that base pair properties and nucleotide identity within a region 4-6 bases below the miR390/miR390* duplex region contributed to the efficiency and accuracy of precursor processing.

摘要

拟南芥中转录的 siRNA(tasiRNA)生物发生是由 microRNA(miRNA)引导的初级转录物切割起始的。在 TAS3 tasiRNA 形成的情况下,ARGONAUTE7(AGO7)-miR390 复合物在两个位点与初级转录物相互作用,导致 RNA 依赖性 RNA 聚合酶 6 的募集以进行 dsRNA 生物合成。对 TAS3 tasiRNA 生物发生或功能有特定缺陷的拟南芥突变体进行了广泛筛选。这产生了许多 ago7 突变体、一个 dcl4 突变体和两个积累低水平 miR390 的突变体。开发了一种基于直接基因组测序的方法来定位和快速鉴定其中一个后者突变等位基因。这揭示了一个 G 到 A 的点突变(mir390a-1),该突变被计算为稳定 MIR390a 反向折叠底部附近相对未配对的区域,导致 miR390/miR390* 双链体的错误加工,随后 TAS3 tasiRNA 水平降低。定向取代以及对同源 miR390 生成基因座(MIR390a 和 MIR390b)的变异分析表明,在 miR390/miR390* 双链体区域下方 4-6 个碱基的区域内的碱基对特性和核苷酸同一性有助于前体加工的效率和准确性。

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