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对经PGPR引发以抵御感染的番茄植株中组织特异性防御反应的代谢组学评估

Metabolomic Evaluation of Tissue-Specific Defense Responses in Tomato Plants Modulated by PGPR-Priming against Infection.

作者信息

Mhlongo Msizi I, Piater Lizelle A, Steenkamp Paul A, Labuschagne Nico, Dubery Ian A

机构信息

Research Centre for Plant Metabolomics, Department of Biochemistry, University of Johannesburg, P.O. Box 524, Auckland Park, Johannesburg 2006, South Africa.

Department of Plant and Soil Sciences, University of Pretoria, Private Bag X20, Hatfield, Pretoria 0028, South Africa.

出版信息

Plants (Basel). 2021 Jul 26;10(8):1530. doi: 10.3390/plants10081530.

Abstract

Plant growth-promoting rhizobacteria (PGPR) can stimulate disease suppression through the induction of an enhanced state of defense readiness. Here, untargeted ultra-high performance liquid chromatography-mass spectrometry (UHPLC-MS) and targeted ultra-high performance liquid chromatography coupled to triple-quadrupole mass spectrometry (UHPLC-QqQ-MS) were used to investigate metabolic reprogramming in tomato plant tissues in response to priming by N04 and T22 against . Roots were treated with the two PGPR strains prior to stem inoculation with Metabolites were methanol-extracted from roots, stems and leaves at two-eight days post-inoculation. Targeted analysis by UHPLC-QqQ-MS allowed quantification of aromatic amino acids and phytohormones. For untargeted analysis, UHPLC-MS data were chemometrically processed to determine signatory biomarkers related to priming against . The aromatic amino acid content was differentially reprogrammed in and primed plants responding to . Furthermore, abscisic acid and methyl salicylic acid were found to be major signaling molecules in the tripartite interaction. LC-MS metabolomics analysis showed time-dependent metabolic changes in the primed-unchallenged vs. primed-challenged tissues. The annotated metabolites included phenylpropanoids, benzoic acids, glycoalkaloids, flavonoids, amino acids, organic acids, as well as oxygenated fatty acids. Tissue-specific reprogramming across diverse metabolic networks in roots, stems and leaves was also observed, which demonstrated that PGPR priming resulted in modulation of the defense response to infection.

摘要

植物促生根际细菌(PGPR)可通过诱导增强的防御准备状态来刺激病害抑制。在此,采用非靶向超高效液相色谱 - 质谱联用(UHPLC - MS)和靶向超高效液相色谱 - 串联四极杆质谱联用(UHPLC - QqQ - MS)技术,研究番茄植株组织中响应N04和T22引发处理以抵御[病原体名称未给出]的代谢重编程。在茎接种[病原体名称未给出]之前,用这两种PGPR菌株处理根部。在接种后2 - 8天,从根、茎和叶中用甲醇提取代谢物。通过UHPLC - QqQ - MS进行靶向分析可对芳香族氨基酸和植物激素进行定量。对于非靶向分析,对UHPLC - MS数据进行化学计量学处理,以确定与抵御[病原体名称未给出]引发相关的标志性生物标志物。在响应[病原体名称未给出]时,经N04和T22引发处理的植物中芳香族氨基酸含量发生了差异重编程。此外,脱落酸和甲基水杨酸被发现是三方相互作用中的主要信号分子。LC - MS代谢组学分析表明,在未受挑战的引发组织与受挑战的引发组织中存在时间依赖性的代谢变化。注释的代谢物包括苯丙烷类、苯甲酸、糖苷生物碱、黄酮类、氨基酸、有机酸以及氧化脂肪酸。还观察到根、茎和叶中不同代谢网络的组织特异性重编程,这表明PGPR引发导致了对[病原体名称未给出]感染的防御反应的调节。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b666/8400099/ab2892639f25/plants-10-01530-g001.jpg

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