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一种细胞核编码的叶绿体磷蛋白调控莱茵衣藻光系统I亚基PsaC的表达。

A Nucleus-Encoded Chloroplast Phosphoprotein Governs Expression of the Photosystem I Subunit PsaC in Chlamydomonas reinhardtii.

作者信息

Douchi Damien, Qu Yujiao, Longoni Paolo, Legendre-Lefebvre Linnka, Johnson Xenie, Schmitz-Linneweber Christian, Goldschmidt-Clermont Michel

机构信息

Department of Botany and Plant Biology and Department of Molecular Biology, University of Geneva, 1211 Geneva 4, Switzerland.

Institute of Biology, Molecular Genetics, Humboldt University of Berlin, D-10115 Berlin, Germany.

出版信息

Plant Cell. 2016 May;28(5):1182-99. doi: 10.1105/tpc.15.00725. Epub 2016 Apr 25.

Abstract

The nucleo-cytoplasmic compartment exerts anterograde control on chloroplast gene expression through numerous proteins that intervene at posttranscriptional steps. Here, we show that the maturation of psaC mutant (mac1) of Chlamydomonas reinhardtii is defective in photosystem I and fails to accumulate psaC mRNA. The MAC1 locus encodes a member of the Half-A-Tetratricopeptide (HAT) family of super-helical repeat proteins, some of which are involved in RNA transactions. The Mac1 protein localizes to the chloroplast in the soluble fraction. MAC1 acts through the 5' untranslated region of psaC transcripts and is required for their stability. Small RNAs that map to the 5'end of psaC RNA in the wild type but not in the mac1 mutant are inferred to represent footprints of MAC1-dependent protein binding, and Mac1 expressed in bacteria binds RNA in vitro. A coordinate response to iron deficiency, which leads to dismantling of the photosynthetic electron transfer chain and in particular of photosystem I, also causes a decrease of Mac1. Overexpression of Mac1 leads to a parallel increase in psaC mRNA but not in PsaC protein, suggesting that Mac1 may be limiting for psaC mRNA accumulation but that other processes regulate protein accumulation. Furthermore, Mac 1 is differentially phosphorylated in response to iron availability and to conditions that alter the redox balance of the electron transfer chain.

摘要

核质区室通过众多干预转录后步骤的蛋白质对叶绿体基因表达施加正向控制。在此,我们表明莱茵衣藻的psaC突变体(mac1)在光系统I中成熟存在缺陷,且无法积累psaC mRNA。MAC1基因座编码超螺旋重复蛋白的半A-四肽(HAT)家族成员,其中一些成员参与RNA相关事务。Mac1蛋白定位于叶绿体的可溶性部分。MAC1通过psaC转录本的5'非翻译区发挥作用,并且是其稳定性所必需的。在野生型中可映射到psaC RNA 5'端但在mac1突变体中不存在的小RNA被推断代表MAC1依赖性蛋白结合的足迹,并且在细菌中表达的Mac1在体外与RNA结合。对铁缺乏的协同反应会导致光合电子传递链,特别是光系统I的拆解,这也会导致Mac1减少。Mac1的过表达导致psaC mRNA平行增加,但PsaC蛋白没有增加,这表明Mac1可能是psaC mRNA积累的限制因素,但其他过程调节蛋白质积累。此外,Mac1会根据铁的可用性以及改变电子传递链氧化还原平衡的条件发生差异磷酸化。

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