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拟南芥多聚半乳糖醛酸甲酯酶参与对丁香假单胞菌的免疫反应。

Arabidopsis PECTIN METHYLESTERASEs contribute to immunity against Pseudomonas syringae.

机构信息

Department of Plant Biology and Microbial and Plant Genomics Institute , University of Minnesota, Saint Paul, Minnesota 55108.

出版信息

Plant Physiol. 2014 Feb;164(2):1093-107. doi: 10.1104/pp.113.227637. Epub 2013 Dec 23.

Abstract

Pectins, major components of dicot cell walls, are synthesized in a heavily methylesterified form in the Golgi and are partially deesterified by pectin methylesterases (PMEs) upon export to the cell wall. PME activity is important for the virulence of the necrotrophic fungal pathogen Botrytis cinerea. Here, the roles of Arabidopsis PMEs in pattern-triggered immunity and immune responses to the necrotrophic fungus Alternaria brassicicola and the bacterial hemibiotroph Pseudomonas syringae pv maculicola ES4326 (Pma ES4326) were studied. Plant PME activity increased during pattern-triggered immunity and after inoculation with either pathogen. The increase of PME activity in response to pathogen treatment was concomitant with a decrease in pectin methylesterification. The pathogen-induced PME activity did not require salicylic acid or ethylene signaling, but was dependent on jasmonic acid signaling. In the case of induction by A. brassicicola, the ethylene response factor, but not the MYC2 branch of jasmonic acid signaling, contributed to induction of PME activity, whereas in the case of induction by Pma ES4326, both branches contributed. There are 66 PME genes in Arabidopsis, suggesting extensive genetic redundancy. Nevertheless, selected pme single, double, triple and quadruple mutants allowed significantly more growth of Pma ES4326 than wild-type plants, indicating a role of PMEs in resistance to this pathogen. No decreases in total PME activity were detected in these pme mutants, suggesting that the determinant of immunity is not total PME activity; rather, it is some specific effect of PMEs such as changes in the pattern of pectin methylesterification.

摘要

果胶是双子叶植物细胞壁的主要成分,在高尔基体中以高度甲酯化的形式合成,并在出口到细胞壁时部分被果胶甲酯酶(PMEs)去甲酯化。PME 活性对坏死型真菌病原菌 Botrytis cinerea 的毒力很重要。在这里,研究了拟南芥 PME 在模式触发免疫以及对坏死型真菌Alternaria brassicicola 和细菌半生物营养型 Pseudomonas syringae pv maculicola ES4326(Pma ES4326)的免疫反应中的作用。植物 PME 活性在模式触发免疫期间以及接种任何病原体后都会增加。对病原体处理的 PME 活性增加伴随着果胶甲酯化程度的降低。病原体诱导的 PME 活性不依赖于水杨酸或乙烯信号,但依赖于茉莉酸信号。就 A. brassicicola 的诱导而言,乙烯反应因子,但不是茉莉酸信号的 MYC2 分支,有助于诱导 PME 活性,而在 Pma ES4326 的诱导中,两个分支都有贡献。拟南芥中有 66 个 PME 基因,表明存在广泛的遗传冗余。尽管如此,选择的 pme 单突变体、双突变体、三突变体和四突变体允许 Pma ES4326 比野生型植物生长得更多,表明 PME 在抵抗这种病原体方面发挥了作用。在这些 pme 突变体中没有检测到总 PME 活性的降低,这表明免疫的决定因素不是总 PME 活性;而是 PME 的某些特定作用,例如果胶甲酯化模式的变化。

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