Subcellular localization requirements and specificities for plant immune receptor Toll‐interleukin‐1 receptor signaling

生物 拟南芥 亚细胞定位 细胞生物学 免疫受体 信号转导 烟草 受体 核定位序列 拟南芥 突变体 遗传学 细胞质 基因
作者
Maud Bernoux,Jian Chen,Xiaoxiao Zhang,Kim Newell,Jian Hu,Laurent Deslandes,Peter N. Dodds
出处
期刊:Plant Journal [Wiley]
卷期号:114 (6): 1319-1337 被引量:5
标识
DOI:10.1111/tpj.16195
摘要

SUMMARY Recent work shed light on how plant intracellular immune receptors of the nucleotide‐binding leucine‐rich repeat (NLR) family are activated upon pathogen effector recognition to trigger immune responses. Activation of Toll‐interleukin‐1 receptor (TIR) domain‐containing NLRs (TNLs) induces receptor oligomerization and close proximity of the TIR domain, which is required for TIR enzymatic activity. TIR‐catalyzed small signaling molecules bind to EDS1 family heterodimers and subsequently activate downstream helper NLRs, which function as Ca 2+ permeable channel to activate immune responses eventually leading to cell death. Subcellular localization requirements of TNLs and signaling partners are not well understood, although they are required to understand fully the mechanisms underlying NLR early signaling. TNLs show diverse subcellular localization while EDS1 shows nucleocytosolic localization. Here, we studied the impact of TIR and EDS1 mislocalization on the signaling activation of different TNLs. In Nicotiana benthamiana , our results suggest that close proximity of TIR domains isolated from flax L6 and Arabidopsis RPS4 and SNC1 TNLs drives signaling activation from different cell compartments. Nevertheless, both Golgi‐membrane anchored L6 and nucleocytosolic RPS4 have the same requirements for EDS1 subcellular localization in Arabidopsis thaliana . By using mislocalized variants of EDS1, we found that autoimmune L6 and RPS4 TIR domain can induce seedling cell death when EDS1 is present in the cytosol. However, when EDS1 is restricted to the nucleus, both induce a stunting phenotype but no cell death. Our data point out the importance of thoroughly investigating the dynamics of TNLs and signaling partners subcellular localization to understand TNL signaling fully.
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