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拟南芥转录因子 WRKY8 与其互作伙伴 VQ9 拮抗作用,共同调控盐胁迫耐受性。

Arabidopsis transcription factor WRKY8 functions antagonistically with its interacting partner VQ9 to modulate salinity stress tolerance.

机构信息

Key Laboratory of Tropical Forest Ecology, Xishuangbanna Tropical Botanical Garden, Chinese Academy of Sciences, Kunming, Yunnan 650223, China.

出版信息

Plant J. 2013 Jun;74(5):730-45. doi: 10.1111/tpj.12159. Epub 2013 Apr 1.

DOI:10.1111/tpj.12159
PMID:23451802
Abstract

The WRKY transcription factors have been demonstrated to play crucial roles in regulating stress responses; however, the exact mechanisms underlying their involvement in stress responses are not fully understood. Arabidopsis WRKY8 was predominantly expressed in roots and was highly upregulated by salt treatment. Disruption of WRKY8 rendered plants hypersensitive to salt, showing delayed germination, inhibited post-germination development and accelerated chlorosis. Further investigation revealed that WRKY8 interacted with VQ9, and their interaction decreased the DNA-binding activity of WRKY8. The VQ9 protein was exclusively localized in the nucleus, and VQ9 expression was strongly responsive to NaCl treatment. Mutation of VQ9 enhanced tolerance to salt stress, indicating that VQ9 acts antagonistically with WRKY8 to mediate responses to salt stress. The antagonist functions of WRKY8 and VQ9 were consistent with an increased or reduced Na⁺/K⁺ concentration ratio, as well as contrasting expression patterns of downstream stress-responsive genes in salt-stressed wrky8 and vq9 mutants. Moreover, chromatin immunoprecipitation (ChIP) assays showed that WRKY8 directly bound the promoter of RD29A under salt conditions. These results provided strong evidence that the VQ9 protein acts as a repressor of the WRKY8 factor to maintain an appropriate balance of WRKY8-mediated signaling pathways to establish salinity stress tolerance.

摘要

WRKY 转录因子被证明在调节应激反应中起着至关重要的作用;然而,它们参与应激反应的确切机制尚不完全清楚。拟南芥 WRKY8 主要在根中表达,并被盐处理高度上调。WRKY8 的破坏使植物对盐敏感,表现出发芽延迟、萌发后发育受抑制和黄化加速。进一步的研究表明,WRKY8 与 VQ9 相互作用,它们的相互作用降低了 WRKY8 的 DNA 结合活性。VQ9 蛋白专门定位于细胞核中,并且 VQ9 的表达对 NaCl 处理强烈响应。VQ9 的突变增强了对盐胁迫的耐受性,表明 VQ9 与 WRKY8 拮抗作用以介导对盐胁迫的响应。WRKY8 和 VQ9 的拮抗作用与增加或减少 Na⁺/K⁺浓度比以及盐胁迫下 wrky8 和 vq9 突变体中下游应激响应基因的对比表达模式一致。此外,染色质免疫沉淀(ChIP)实验表明,WRKY8 在盐条件下直接结合 RD29A 的启动子。这些结果有力地证明了 VQ9 蛋白作为 WRKY8 因子的抑制剂,以维持 WRKY8 介导的信号通路的适当平衡,从而建立耐盐性。

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