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在利什曼原虫中,Hsp83 的优先翻译需要在 3'UTR 中存在热敏性富含嘧啶的元件,并涉及到 5'UTR 的扫描。

Preferential translation of Hsp83 in Leishmania requires a thermosensitive polypyrimidine-rich element in the 3' UTR and involves scanning of the 5' UTR.

机构信息

Department of Life Sciences, Ben Gurion University of the Negev, Beer Sheva 84105, Israel.

出版信息

RNA. 2010 Feb;16(2):364-74. doi: 10.1261/rna.1874710. Epub 2009 Dec 29.

Abstract

Heat shock proteins (HSPs) provide a useful system for studying developmental patterns in the digenetic Leishmania parasites, since their expression is induced in the mammalian life form. Translation regulation plays a key role in control of protein coding genes in trypanosomatids, and is directed exclusively by elements in the 3' untranslated region (UTR). Using sequential deletions of the Leishmania Hsp83 3' UTR (888 nucleotides [nt]), we mapped a region of 150 nt that was required, but not sufficient for preferential translation of a reporter gene at mammalian-like temperatures, suggesting that changes in RNA structure could be involved. An advanced bioinformatics package for prediction of RNA folding (UNAfold) marked the regulatory region on a highly probable structural arm that includes a polypyrimidine tract (PPT). Mutagenesis of this PPT abrogated completely preferential translation of the fused reporter gene. Furthermore, temperature elevation caused the regulatory region to melt more extensively than the same region that lacked the PPT. We propose that at elevated temperatures the regulatory element in the 3' UTR is more accessible to mediators that promote its interaction with the basal translation components at the 5' end during mRNA circularization. Translation initiation of Hsp83 at all temperatures appears to proceed via scanning of the 5' UTR, since a hairpin structure abolishes expression of a fused reporter gene.

摘要

热休克蛋白(HSPs)为研究双基因利什曼原虫的发育模式提供了一个有用的系统,因为它们在哺乳动物生活形式中表达。翻译调控在原生动物蛋白编码基因的控制中起着关键作用,并且仅由 3'非翻译区(UTR)中的元件指导。通过对利什曼 Hsp83 3'UTR(888 个核苷酸)进行连续缺失,我们定位了一个 150 个核苷酸的区域,该区域对于在哺乳动物样温度下优先翻译报告基因是必需的,但不是充分的,这表明 RNA 结构的变化可能与之相关。一个用于预测 RNA 折叠的高级生物信息学包(UNAfold)在一个高度可能的结构臂上标记了调控区域,该结构臂包括一个多嘧啶序列(PPT)。该 PPT 的突变完全废除了融合报告基因的优先翻译。此外,温度升高导致调控区域比缺乏 PPT 的相同区域更广泛地融化。我们提出,在高温下,3'UTR 中的调节元件更容易与促进其在 mRNA 环化过程中与 5'端基本翻译成分相互作用的介质相互作用。在所有温度下,Hsp83 的翻译起始似乎都通过 5'UTR 的扫描进行,因为发夹结构会使融合报告基因的表达被废除。

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