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根际细菌诱导拟南芥产生的系统抗性需要在施用部位依赖乙烯的信号传导。

Systemic resistance in Arabidopsis induced by rhizobacteria requires ethylene-dependent signaling at the site of application.

作者信息

Knoester M, Pieterse C M, Bol J F, Van Loon L C

机构信息

Institute of Biology, Utrecht University, The Netherlands.

出版信息

Mol Plant Microbe Interact. 1999 Aug;12(8):720-7. doi: 10.1094/MPMI.1999.12.8.720.

Abstract

Root colonization of Arabidopsis thaliana by the nonpathogenic, rhizosphere-colonizing, biocontrol bacterium Pseudomonas fluorescens WCS417r has been shown to elicit induced systemic resistance (ISR) against Pseudomonas syringae pv. tomato (Pst). The ISR response differs from the pathogen-inducible systemic acquired resistance (SAR) response in that ISR is independent of salicylic acid and not associated with pathogenesis-related proteins. Several ethylene-response mutants were tested and showed essentially normal symptoms of Pst infection. ISR was abolished in the ethylene-insensitive mutant etr1-1, whereas SAR was unaffected. Similar results were obtained with the ethylene-insensitive mutants ein2 through ein7, indicating that the expression of ISR requires the complete signal-transduction pathway of ethylene known so far. The induction of ISR by WCS417r was not accompanied by increased ethylene production in roots or leaves, nor by increases in the expression of the genes encoding the ethylene biosynthetic enzymes 1-aminocyclopropane-1-carboxylic (ACC) synthase and ACC oxidase. The eir1 mutant, displaying ethylene insensitivity in the roots only, did not express ISR upon application of WCS417r to the roots, but did exhibit ISR when the inducing bacteria were infiltrated into the leaves. These results demonstrate that, for the induction of ISR, ethylene responsiveness is required at the site of application of inducing rhizobacteria.

摘要

已证明,非致病性、定殖于根际的生防细菌荧光假单胞菌WCS417r在拟南芥根部定殖可诱导对丁香假单胞菌番茄致病变种(Pst)的系统抗性(ISR)。ISR反应与病原体诱导的系统获得性抗性(SAR)反应不同,因为ISR不依赖水杨酸,也与病程相关蛋白无关。对几个乙烯反应突变体进行了测试,结果显示它们感染Pst后的症状基本正常。乙烯不敏感突变体etr1-1中ISR被消除,而SAR未受影响。乙烯不敏感突变体ein2至ein7也得到了类似结果,这表明ISR的表达需要目前已知的完整乙烯信号转导途径。WCS417r诱导ISR并不伴随着根或叶中乙烯产量的增加,也不伴随着编码乙烯生物合成酶1-氨基环丙烷-1-羧酸(ACC)合酶和ACC氧化酶的基因表达增加。eir1突变体仅在根部表现出乙烯不敏感性,在根部施用WCS417r后不表达ISR,但当诱导细菌渗入叶片时则表现出ISR。这些结果表明,对于ISR的诱导,在诱导根际细菌施用部位需要乙烯反应性。

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