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丁香假单胞菌avr基因在大肠杆菌中的表型表达与hrp编码的分泌系统的活性相关。

Phenotypic expression of Pseudomonas syringae avr genes in E. coli is linked to the activities of the hrp-encoded secretion system.

作者信息

Pirhonen M U, Lidell M C, Rowley D L, Lee S W, Jin S, Liang Y, Silverstone S, Keen N T, Hutcheson S W

机构信息

Department of Plant Biology, University of Maryland at College Park 20742, USA.

出版信息

Mol Plant Microbe Interact. 1996 May;9(4):252-60. doi: 10.1094/mpmi-9-0252.

Abstract

The specific recognition of elicitors produced by plant pathogenic bacteria carrying avirulence (avr) genes is postulated to initiate cellular defense responses in plants expressing corresponding resistance genes. The biochemical functions of most avr genes, however, are not known. A heterologous system was developed to phenotypically express Pseudomonas syringae avr genes in Escherichia coli cells that required the P. syringae hrp cluster. E. coli MC4100 transformants carrying the plasmic-borne P. syringae pv. syringae Pss61 hrp cluster and p. syringae pv. glycinea avrB expressed from a triple lacUV5 promoter gained the ability to elicit the hypersensitive response in soybean cultivars expressing Rpg1 and in an Arabidopsis thaliana accession expressing RPM1. Inactivation of energy transducing or outer membrane components of the hrp-encoded secretion system blocked phenotypic expression expression of avrB in E. coli, but deletions abolishing harpinPSS production had little effect on the production of the AvrB phenotype by the E. coli transformants. Phenotypic expression of avrA, AvrPto, avrRpm1, avrRpt2, and avrPph3 in E. coli was also shown to require the hrp cluster. The results indicate that generation of the Avr phenotype in P. syringae strains is specifically dependent on the secretion activities of the hrp cluster.

摘要

推测携带无毒(avr)基因的植物病原菌产生的激发子的特异性识别可启动表达相应抗性基因的植物中的细胞防御反应。然而,大多数avr基因的生化功能尚不清楚。开发了一种异源系统,以在需要丁香假单胞菌hrp簇的大肠杆菌细胞中表型表达丁香假单胞菌的avr基因。携带质粒携带的丁香假单胞菌丁香假单胞菌Pss61 hrp簇和从三重lacUV5启动子表达的大豆丁香假单胞菌avrB的大肠杆菌MC4100转化体获得了在表达Rpg1的大豆品种和表达RPM1的拟南芥种质中引发过敏反应的能力。hrp编码的分泌系统的能量转导或外膜成分的失活阻断了avrB在大肠杆菌中的表型表达,但消除harpinPSS产生的缺失对大肠杆菌转化体产生AvrB表型的影响很小。还显示avrA、AvrPto、avrRpm1、avrRpt2和avrPph3在大肠杆菌中的表型表达需要hrp簇。结果表明,丁香假单胞菌菌株中Avr表型的产生特别依赖于hrp簇的分泌活性。

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