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对细胞器基因表达改变的核逆行反应核心模块的定义将GLK过表达体鉴定为gun突变体。

Definition of a core module for the nuclear retrograde response to altered organellar gene expression identifies GLK overexpressors as gun mutants.

作者信息

Leister Dario, Kleine Tatjana

机构信息

Lehrstuhl für Molekularbiologie der Pflanzen (Botanik), Department Biologie I, Ludwig-Maximilians-Universität, Planegg-Martinsried, Munich, Germany.

出版信息

Physiol Plant. 2016 Jul;157(3):297-309. doi: 10.1111/ppl.12431. Epub 2016 Apr 4.

DOI:10.1111/ppl.12431
PMID:26876646
Abstract

Retrograde signaling can be triggered by changes in organellar gene expression (OGE) induced by inhibitors such as lincomycin (LIN) or mutations that perturb OGE. Thus, an insufficiency of the organelle-targeted prolyl-tRNA synthetase PRORS1 in Arabidopsis thaliana activates retrograde signaling and reduces the expression of nuclear genes for photosynthetic proteins. Recently, we showed that mTERF6, a member of the so-called mitochondrial transcription termination factor (mTERF) family, is involved in the formation of chloroplast (cp) isoleucine-tRNA. To obtain further insights into its functions, co-expression analysis of MTERF6, PRORS1 and two other genes for organellar aminoacyl-tRNA synthetases was conducted. The results suggest a prominent role of mTERF6 in aminoacylation activity, light signaling and seed storage. Analysis of changes in whole-genome transcriptomes in the mterf6-1 mutant showed that levels of nuclear transcripts for cp OGE proteins were particularly affected. Comparison of the mterf6-1 transcriptome with that of prors1-2 showed that reduced aminoacylation of proline (prors1-2) and isoleucine (mterf6-1) tRNAs alters retrograde signaling in similar ways. Database analyses indicate that comparable gene expression changes are provoked by treatment with LIN, norflurazon or high light. A core OGE response module was defined by identifying genes that were differentially expressed under at least four of six conditions relevant to OGE signaling. Based on this module, overexpressors of the Golden2-like transcription factors GLK1 and GLK2 were identified as genomes uncoupled mutants.

摘要

逆行信号传导可由诸如林可霉素(LIN)等抑制剂诱导的细胞器基因表达(OGE)变化或扰乱OGE的突变引发。因此,拟南芥中靶向细胞器的脯氨酰 - tRNA合成酶PRORS1功能不足会激活逆行信号传导,并降低光合蛋白核基因的表达。最近,我们发现所谓的线粒体转录终止因子(mTERF)家族成员mTERF6参与叶绿体(cp)异亮氨酸 - tRNA的形成。为了进一步深入了解其功能,我们对MTERF6、PRORS1以及另外两个细胞器氨酰 - tRNA合成酶基因进行了共表达分析。结果表明mTERF6在氨酰化活性、光信号传导和种子储存中发挥着重要作用。对mterf6 - 1突变体全基因组转录组变化的分析表明,cp OGE蛋白的核转录本水平受到特别影响。将mterf6 - 1转录组与prors1 - 2的转录组进行比较发现,脯氨酸(prors1 - 2)和异亮氨酸(mterf6 - 1)tRNA的氨酰化减少以类似方式改变逆行信号传导。数据库分析表明,用LIN、去甲草净或强光处理会引发类似的基因表达变化。通过鉴定在与OGE信号传导相关的六个条件中的至少四个条件下差异表达的基因,定义了一个核心OGE反应模块。基于该模块,类Golden2转录因子GLK1和GLK2的过表达体被鉴定为基因组解偶联突变体。

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