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莱茵衣藻叶绿体中petA转录本稳定性的顺式和反式作用决定因素的分子鉴定及功能

Molecular identification and function of cis- and trans-acting determinants for petA transcript stability in Chlamydomonas reinhardtii chloroplasts.

作者信息

Loiselay Christelle, Gumpel Nicola J, Girard-Bascou Jacqueline, Watson Adam T, Purton Saul, Wollman Francis-André, Choquet Yves

机构信息

UMR 7141 CNRS/UPMC, Institut de Biologie Physico-Chimique, 13 Rue Pierre et Marie Curie, F-75005 Paris, France.

出版信息

Mol Cell Biol. 2008 Sep;28(17):5529-42. doi: 10.1128/MCB.02056-07. Epub 2008 Jun 23.

Abstract

In organelles, the posttranscriptional steps of gene expression are tightly controlled by nucleus-encoded factors, most often acting in a gene-specific manner. Despite the molecular identification of a growing number of factors, their mode of action remains largely unknown. In the green alga Chlamydomonas reinhardtii, expression of the chloroplast petA gene, which codes for cytochrome f, depends on two specific nucleus-encoded factors. MCA1 controls the accumulation of the transcript, while TCA1 is required for its translation. We report here the cloning of MCA1, the first pentatricopeptide repeat protein functionally identified in this organism. By chloroplast transformation with modified petA genes, we investigated the function of MCA1 in vivo. We demonstrate that MCA1 acts on the very first 21 nucleotides of the petA 5' untranslated region to protect the whole transcript from 5'-->3' degradation but does not process the 5' end of the petA mRNA. MCA1 and TCA1 recognize adjacent targets and probably interact together for efficient expression of petA mRNA. MCA1, although not strictly required for translation, shows features of a translational enhancer, presumably by assisting the binding of TCA1 to its own target. Conversely, TCA1 participates to the full stabilization of the transcript through its interaction with MCA1.

摘要

在细胞器中,基因表达的转录后步骤受到核编码因子的严格控制,这些因子大多以基因特异性方式发挥作用。尽管已从分子层面鉴定出越来越多的因子,但其作用方式仍 largely unknown。在绿藻莱茵衣藻中,编码细胞色素f的叶绿体petA基因的表达依赖于两种特定的核编码因子。MCA1控制转录本的积累,而TCA1是其翻译所必需的。我们在此报告MCA1的克隆,它是在该生物体中功能上首次鉴定出的五肽重复蛋白。通过用修饰的petA基因进行叶绿体转化,我们在体内研究了MCA1的功能。我们证明,MCA1作用于petA 5'非翻译区的前21个核苷酸,以保护整个转录本免受5'→3'降解,但不处理petA mRNA的5'末端。MCA1和TCA1识别相邻靶点,可能共同相互作用以实现petA mRNA的高效表达。MCA1虽然不是翻译严格必需的,但显示出翻译增强子的特征,大概是通过协助TCA1与其自身靶点结合。相反,TCA1通过与MCA1相互作用参与转录本的完全稳定。

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