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AtIREG2编码一种液泡膜转运蛋白,参与拟南芥根中依赖铁的镍解毒过程。

AtIREG2 encodes a tonoplast transport protein involved in iron-dependent nickel detoxification in Arabidopsis thaliana roots.

作者信息

Schaaf Gabriel, Honsbein Annegret, Meda Anderson R, Kirchner Silvia, Wipf Daniel, von Wirén Nicolaus

机构信息

Institut für Pflanzenernährung, Universität Hohenheim, 70593 Stuttgart, Germany.

出版信息

J Biol Chem. 2006 Sep 1;281(35):25532-40. doi: 10.1074/jbc.M601062200. Epub 2006 Jun 21.

DOI:10.1074/jbc.M601062200
PMID:16790430
Abstract

Iron acquisition in Arabidopsis depends mainly on AtIRT1, a Fe2+ transporter in the plasma membrane of root cells. However, substrate specificity of AtIRT1 is low, leading to an excess accumulation of other transition metals in iron-deficient plants. In the present study we describe AtIREG2 as a nickel transporter at the vacuolar membrane that counterbalances the low substrate specificity of AtIRT1 and possibly other iron transport systems in iron-deficient root cells. AtIREG2 is co-regulated with AtIRT1 by the transcription factor FRU/FIT1, encodes a membrane protein, which has 10 putative transmembrane domains and shares homology with vertebrate Fe2+ exporters. Heterologous expression of AtIREG2 in various yeast mutants, however, did not demonstrate an iron transport function. Instead, expression in wild-type and nickel-sensitive cot1 yeast cells conferred enhanced tolerance to elevated concentrations of nickel at acidic pH. A role in vacuolar substrate transport was further supported by localization of AtIREG2-GFP fusion proteins to the tonoplast in Arabidopsis suspension cells and root cells of intact plants. Transgenic plants overexpressing AtIREG2 showed an increased tolerance to elevated concentrations of nickel, whereas T-DNA insertion lines lacking AtIREG2 expression were more sensitive to nickel, particularly under iron deficiency, and accumulated less nickel in roots. We therefore propose a role of AtIREG2 in vacuolar loading of nickel under iron deficiency and thus identify it as a novel component in the iron deficiency stress response.

摘要

拟南芥中铁的获取主要依赖于AtIRT1,它是根细胞质膜上的一种Fe2+转运蛋白。然而,AtIRT1的底物特异性较低,导致缺铁植物中其他过渡金属过量积累。在本研究中,我们将AtIREG2描述为液泡膜上的一种镍转运蛋白,它可以平衡缺铁根细胞中AtIRT1以及可能其他铁转运系统较低的底物特异性。AtIREG2与AtIRT1受转录因子FRU/FIT1共同调控,编码一种膜蛋白,该蛋白有10个假定的跨膜结构域,与脊椎动物的Fe2+输出蛋白具有同源性。然而,AtIREG2在各种酵母突变体中的异源表达并未显示出铁转运功能。相反,在野生型和对镍敏感的cot1酵母细胞中的表达赋予了细胞在酸性pH条件下对高浓度镍更强的耐受性。AtIREG2-GFP融合蛋白定位于拟南芥悬浮细胞和完整植株根细胞的液泡膜,这进一步支持了其在液泡底物转运中的作用。过表达AtIREG2的转基因植物对高浓度镍的耐受性增强,而缺乏AtIREG2表达的T-DNA插入系对镍更敏感,尤其是在缺铁条件下,并且根部积累的镍更少。因此,我们提出AtIREG2在缺铁条件下参与镍的液泡装载,从而将其鉴定为缺铁胁迫反应中的一个新成分。

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