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酵母毕赤酵母 Dicer 加工茎环 RNA 的结构和机制见解。

Structural and mechanistic insight into stem-loop RNA processing by yeast Pichia stipitis Dicer.

机构信息

Department of Biological Sciences and Centre for Bioimaging Sciences, National University of Singapore, Singapore, Singapore.

National University of Singapore (Suzhou) Research Institute, Suzhou, China.

出版信息

Protein Sci. 2021 Jun;30(6):1210-1220. doi: 10.1002/pro.4086. Epub 2021 Apr 28.

DOI:10.1002/pro.4086
PMID:33884665
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8138527/
Abstract

Dicer is a member of the ribonuclease III enzyme family and processes double-stranded RNA into small functional RNAs. The variation in the domain architecture of Dicer among different species whilst preserving its biological dicing function is intriguing. Here, we describe the structure and function of a novel catalytically active RNase III protein, a non-canonical Dicer (PsDCR1), found in budding yeast Pichia stipitis. The structure of the catalytically active region (the catalytic RNase III domain and double-stranded RNA-binding domain 1 [dsRBD1]) of DCR1 showed that RNaseIII domain is structurally similar to yeast RNase III (Rnt1p) but uniquely presents dsRBD1 in a diagonal orientation, forming a catalytic core made of homodimer and large RNA-binding surface. The second dsRNA binding domain at C-terminus, which is absent in Rnt1, enhances the RNA cleavage activity. Although the cleavage pattern of PsDCR1 anchors an apical loop similar to Rnt1, the cleavage activity depended on the sequence motif at the lower stem, not the apical loop, of hairpin RNA. Through RNA sequencing and RNA mutations, we showed that RNA cleavage by PsDCR1 is determined by the stem-loop structure of the RNA substrate, suggesting the possibility that stem-loop RNA-guided gene silencing pathway exists in budding yeast.

摘要

Dicer 是核糖核酸酶 III 酶家族的成员,可将双链 RNA 加工成具有功能的小 RNA。不同物种中 Dicer 的结构域架构存在差异,但仍保留其生物切割功能,这令人着迷。在这里,我们描述了新型催化活性 RNase III 蛋白(非典型 Dicer(PsDCR1))的结构和功能,该蛋白存在于出芽酵母毕赤酵母中。DCR1 的催化活性区域(催化 RNase III 结构域和双链 RNA 结合结构域 1(dsRBD1))的结构表明,RNaseIII 结构域在结构上与酵母 RNase III(Rnt1p)相似,但独特地以对角线方向呈现 dsRBD1,形成由同源二聚体和大 RNA 结合表面组成的催化核心。第二个位于 C 末端的双链 RNA 结合结构域在 Rnt1 中不存在,增强了 RNA 切割活性。尽管 PsDCR1 的切割模式锚定了类似于 Rnt1 的顶端环,但切割活性取决于发夹 RNA 较低茎部的序列基序,而不是顶端环。通过 RNA 测序和 RNA 突变,我们表明 PsDCR1 的 RNA 切割由 RNA 底物的茎环结构决定,这表明在出芽酵母中存在茎环 RNA 指导的基因沉默途径的可能性。

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