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拟南芥DNA促旋酶定位于叶绿体和线粒体。

Arabidopsis thaliana DNA gyrase is targeted to chloroplasts and mitochondria.

作者信息

Wall Melisa K, Mitchenall Lesley A, Maxwell Anthony

机构信息

Department of Biological Chemistry, John Innes Centre, Norwich Research Park, Colney, Norwich NR4 7UH, United Kingdom.

出版信息

Proc Natl Acad Sci U S A. 2004 May 18;101(20):7821-6. doi: 10.1073/pnas.0400836101. Epub 2004 May 10.

Abstract

DNA gyrase is the bacterial DNA topoisomerase (topo) that supercoils DNA by using the free energy of ATP hydrolysis. The enzyme, an A(2)B(2) tetramer encoded by the gyrA and gyrB genes, catalyses topological changes in DNA during replication and transcription, and is the only topo that is able to introduce negative supercoils. Gyrase is essential in bacteria and apparently absent from eukaryotes and is, consequently, an important target for antibacterial agents (e.g., quinolones and coumarins). We have identified four putative gyrase genes in the model plant Arabidopsis thaliana; one gyrA and three gyrB homologues. DNA gyrase protein A (GyrA) has a dual translational initiation site targeting the mature protein to both chloroplasts and mitochondria, and there are individual targeting sequences for two of the DNA gyrase protein B (GyrB) homologues. N-terminal fusions of the organellar targeting sequences to GFPs support the hypothesis that one enzyme is targeted to the chloroplast and another to the mitochondrion, which correlates with supercoiling activity in isolated organelles. Treatment of seedlings and cultured cells with gyrase-specific drugs leads to growth inhibition. Knockout of A. thaliana gyrA is embryo-lethal whereas knockouts in the gyrB genes lead to seedling-lethal phenotypes or severely stunted growth and development. The A. thaliana genes have been cloned in Escherichia coli and found to complement gyrase temperature-sensitive strains. This report confirms the existence of DNA gyrase in eukaryotes and has important implications for drug targeting, organelle replication, and the evolution of topos in plants.

摘要

DNA促旋酶是一种细菌DNA拓扑异构酶,它利用ATP水解产生的自由能使DNA超螺旋化。该酶是一种由gyrA和gyrB基因编码的A(2)B(2)四聚体,在复制和转录过程中催化DNA的拓扑变化,并且是唯一能够引入负超螺旋的拓扑异构酶。促旋酶在细菌中是必需的,而在真核生物中显然不存在,因此是抗菌剂(如喹诺酮类和香豆素类)的重要作用靶点。我们在模式植物拟南芥中鉴定出了四个假定的促旋酶基因;一个gyrA和三个gyrB同源物。DNA促旋酶蛋白A(GyrA)有一个双重翻译起始位点,可将成熟蛋白靶向到叶绿体和线粒体,并且两个DNA促旋酶蛋白B(GyrB)同源物有各自的靶向序列。将细胞器靶向序列与绿色荧光蛋白(GFP)进行N端融合,支持了一种酶靶向叶绿体而另一种酶靶向线粒体的假说,这与分离细胞器中的超螺旋活性相关。用促旋酶特异性药物处理幼苗和培养细胞会导致生长抑制。拟南芥gyrA基因敲除是胚胎致死的,而gyrB基因敲除会导致幼苗致死表型或严重发育迟缓和生长受阻。拟南芥基因已在大肠杆菌中克隆,并发现可互补促旋酶温度敏感菌株。本报告证实了真核生物中存在DNA促旋酶,这对药物靶向、细胞器复制以及植物中拓扑异构酶的进化具有重要意义。

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