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水稻谷胱甘肽过氧化物酶 1 介导的 bZIP68 氧化正向调控非依赖 ABA 的渗透胁迫信号。

Rice GLUTATHIONE PEROXIDASE1-mediated oxidation of bZIP68 positively regulates ABA-independent osmotic stress signaling.

机构信息

Laboratory Center of Life Sciences, College of Life Sciences, Nanjing Agricultural University, Nanjing 210095, PR China.

Institute for Biology and Biotechnology of Plants, University of Muenster, 48149 Muenster, Germany.

出版信息

Mol Plant. 2022 Apr 4;15(4):651-670. doi: 10.1016/j.molp.2021.11.006. Epub 2021 Nov 15.

Abstract

Osmotic stress caused by drought and high salinity is a significant environmental threat that limits plant growth and agricultural yield. Redox regulation plays an important role in plant stress responses, but the mechanisms by which plants perceive and transduce redox signals are still underexplored. Here, we report a critical function for the thiol peroxidase GPX1 in osmotic stress response in rice, where it serves as a redox sensor and transducer. GPX1 is quickly oxidized upon exposure to osmotic stress and forms an intramolecular disulfide bond, which is required for the activation of bZIP68, a VRE-like basic leucine zipper (bZIP) transcription factor involved in the ABA-independent osmotic stress response pathway. The disulfide exchange between GPX1 and bZIP68 induces homo-tetramerization of bZIP68 and thus positively regulates osmotic stress response by regulating osmotic-responsive gene expression. Furthermore, we discovered that the nuclear translocation of GPX1 is regulated by its acetylation under osmotic stress. Taken together, our findings not only uncover the redox regulation of the GPX1-bZIP68 module during osmotic stress but also highlight the coordination of protein acetylation and redox signaling in plant osmotic stress responses.

摘要

干旱和高盐度引起的渗透胁迫是限制植物生长和农业产量的重要环境威胁。氧化还原调控在植物胁迫响应中起着重要作用,但植物感知和转导氧化还原信号的机制仍未得到充分探索。在这里,我们报道了谷胱甘肽过氧化物酶 GPX1 在水稻渗透胁迫响应中的关键功能,它作为一种氧化还原传感器和转导器。GPX1 在暴露于渗透胁迫时迅速被氧化,并形成一个分子内二硫键,这对于 VRE 样碱性亮氨酸拉链(bZIP)转录因子 bZIP68 的激活是必需的,bZIP68 参与 ABA 非依赖性渗透胁迫响应途径。GPX1 和 bZIP68 之间的二硫键交换诱导 bZIP68 的同源四聚化,从而通过调节渗透响应基因的表达来正向调节渗透胁迫响应。此外,我们发现渗透胁迫下 GPX1 的核转位受其乙酰化的调控。总之,我们的研究结果不仅揭示了 GPX1-bZIP68 模块在渗透胁迫下的氧化还原调控,还强调了蛋白质乙酰化和氧化还原信号在植物渗透胁迫响应中的协调作用。

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