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拟南芥中铝依赖性的根生长抑制是由AtATR调控的细胞周期停滞引起的。

Aluminum-dependent root-growth inhibition in Arabidopsis results from AtATR-regulated cell-cycle arrest.

作者信息

Rounds Megan A, Larsen Paul B

机构信息

Department of Biochemistry, University of California, Riverside, California 92521, USA.

出版信息

Curr Biol. 2008 Oct 14;18(19):1495-500. doi: 10.1016/j.cub.2008.08.050. Epub 2008 Oct 2.

DOI:10.1016/j.cub.2008.08.050
PMID:18835170
Abstract

Aluminum (Al) toxicity is a global problem severely limiting agricultural productivity in acid-soil regions comprising upwards of 50% of the world's arable land [1, 2]. Although Al-exclusion mechanisms have been intensively studied [3-9], little is known about tolerance to internalized Al, which is predicted to be mechanistically complex because of the plethora of predicted cellular targets for Al(3+)[2, 10]. An Arabidopsis mutant with Al hypersensitivity, als3-1, was found to represent a lesion in a phloem and root-tip-localized factor similar to the bacterial ABC transporter ybbm, with ALS3 likely responsible for Al transfer from roots to less-sensitive tissues [10-12]. To identify mutations that enhance mechanisms of Al resistance or tolerance, a suppressor screen for mutants that mask the Al hypersensitivity of als3-1 was performed [13]. Two allelic suppressors conferring increased Al tolerance were found to represent dominant-negative mutations in a factor required for monitoring DNA integrity, AtATR[14-17]. From this work, Al-dependent root-growth inhibition primarily arises from DNA damage coupled with AtATR-controlled blockage of cell-cycle progression and terminal differentiation because of loss of the root-quiescent center, with mutations that prevent response to this damage resulting in quiescent-center maintenance and sustained vigorous growth in an Al-toxic environment.

摘要

铝(Al)毒性是一个全球性问题,严重限制了占世界可耕地面积50%以上的酸性土壤地区的农业生产力[1,2]。尽管对铝排斥机制已进行了深入研究[3-9],但对于内化铝的耐受性却知之甚少,由于预测铝离子(Al3+)有大量的细胞靶点,预计其机制很复杂[2,10]。一个对铝过敏的拟南芥突变体als3-1,被发现是一种在韧皮部和根尖定位的因子中存在损伤,该因子类似于细菌ABC转运蛋白ybbm,ALS3可能负责将铝从根部转移到敏感性较低的组织[10-12]。为了鉴定增强铝抗性或耐受性机制的突变,对掩盖als3-1铝超敏性的突变体进行了抑制子筛选[13]。发现两个赋予更高铝耐受性的等位抑制子代表了监测DNA完整性所需因子AtATR中的显性负突变[14-17]。从这项工作可知,铝依赖性根生长抑制主要源于DNA损伤,以及由于根静止中心丧失导致的AtATR控制的细胞周期进程和终末分化阻滞,而阻止对这种损伤作出反应的突变会导致静止中心维持,并在铝毒性环境中持续旺盛生长。

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