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Cis-acting elements and trans-acting factors for accurate translation of chloroplast psbA mRNAs: development of an in vitro translation system from tobacco chloroplasts.

机译:准确翻译叶绿体psbA mRNA的顺式作用元件和反式作用因子:从烟草叶绿体体外翻译系统的开发。

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摘要

Translational regulation is an important step of gene expression in chloroplasts. To analyze biochemical mechanisms of translational regulation unique to higher plant chloroplasts, an in vitro translation system has been developed from tobacco chloroplasts. Conditions for chloroplast extraction and the in vitro translation reaction have been optimized with a tobacco psbA-lacZ fusion mRNA. The in vitro system supports accurate translation of a variety of chloroplasts mRNAs. Using a series of mutant psbA mRNAs, we showed that three elements within the 5'-untranslated region of the mRNA are required for translation. Two of them are complementary to the 3'-terminus of chloroplast 16S rRNA (termed RBS1 and RBS2) and the other is an AU-rich sequence (UAAAUAAA) located between RBS1 and RBS2 and is termed the AU box. mRNA competition experiments using the in vitro translation reaction and gel mobility shift assays revealed the existence of a trans-acting factor(s) for translation and its possible interaction with the AU box. We propose a model for the initiation of psbA translation whereby RBS1 and RBS2 bind cooperatively to the 3'-end of 16S rRNA resulting in looping out of the AU box, which facilitates the interaction of a trans-acting factor(s).
机译:翻译调控是叶绿体中基因表达的重要步骤。为了分析高级植物叶绿体特有的翻译调控的生化机制,已经从烟草叶绿体开发了体外翻译系统。使用烟草psbA-lacZ融合mRNA优化了叶绿体提取条件和体外翻译反应。体外系统支持多种叶绿体mRNA的准确翻译。使用一系列的突变psbA mRNA,我们显示了在mRNA的5'-非翻译区域内的三个元素是翻译所必需的。它们中的两个与叶绿体16S rRNA的3'末端互补(称为RBS1和RBS2),另一个是位于RBS1和RBS2之间的富含AU的序列(UAAAUAAA),被称为AU盒。使用体外翻译反应和凝胶迁移率迁移分析的mRNA竞争实验揭示了翻译用反式作用因子的存在及其与AU盒的可能相互作用。我们提出了一个启动psbA翻译的模型,其中RBS1和RBS2协同结合到16S rRNA的3'末端,导致环出AU盒,这促进了反式作用因子的相互作用。

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