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The Global Regulator Genes from Biocontrol Strain Serratia plymuthica IC1270: Cloning Sequencing and Functional Studies

机译:生物防治菌株沙雷氏菌IC1270的全球调节基因:克隆测序和功能研究。

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摘要

The biocontrol activity of various fluorescent pseudomonads towards plant-pathogenic fungi is dependent upon the GacA/GacS-type two-component system of global regulators and the RpoS transcription sigma factor. In particular, these components are required for the production of antifungal antibiotics and exoenzymes. To investigate the effects of these global regulators on the expression of biocontrol factors by plant-associated bacteria other than Pseudomonas spp., gacA/gacS and rpoS homologues were cloned from biocontrol strain IC1270 of Serratia plymuthica, which produces a set of antifungal compounds, including chitinolytic enzymes and the antibiotic pyrrolnitrin. The nucleotide and deduced protein sequence alignments of the cloned gacA/gacS-like genes—tentatively designated grrA (global response regulation activator) and grrS (global response regulation sensor) and of the cloned rpoS gene revealed 64 to 93% identity with matching genes and proteins of the enteric bacteria Escherichia coli, Pectobacterium carotovora subsp. carotovora, and Serratia marcescens. grrA, grrS, and rpoS gene replacement mutants of strain IC1270 were deficient in the production of pyrrolnitrin, an exoprotease, and N-acylhomoserine lactone quorum-sensing signal molecules. However, neither mutant appeared to differ from the parental strain in the production of siderophores, and only grrA and grrS mutants were deficient in the production of a 58-kDa endochitinase, representing the involvement of other sigma factors in the regulation of strain IC1270's chitinolytic activity. Compared to the parental strain, the grrA, grrS, and rpoS mutants were markedly less capable of suppressing Rhizoctonia solani and Pythium aphanidermatum under greenhouse conditions, indicating the dependence of strain IC1270's biocontrol property on the GrrA/GrrS and RpoS global regulators.
机译:各种荧光假单胞菌对植物致病真菌的生物防治活性取决于全局调节剂的GacA / GacS型两组分系统和RpoS转录sigma因子。特别地,这些成分是生产抗真菌抗生素和外切酶所必需的。为了研究这些全局调控因子对假单胞菌属以外的植物相关细菌生物控制因子表达的影响,从粘质沙雷氏菌的生物控制菌株IC1270中克隆了gacA / gacS和rpoS同源物,产生了一系列抗真菌化合物,包括几丁质酶和抗生素吡咯硝菌素。克隆的gacA / gacS样基因(暂定为grrA(全局应答调节激活剂)和grrS(全局应答调节传感器))与克隆的rpoS基因的核苷酸序列和推导的蛋白质序列比对结果显示,与匹配基因的同源性为64%至93%肠杆菌大肠杆状菌亚种的蛋白质。胡萝卜和粘质沙雷氏菌。菌株IC1270的grrA,grrS和rpoS基因替代突变体在吡咯硝菌素,一种外切蛋白酶和N-酰基高丝氨酸内酯群体感应信号分子的产生中不足。然而,在铁载体的生产中,这两个突变体似乎都与亲本菌株没有区别,只有 grrA grrS 突变体在生产58 kDa内切几丁质内切酶方面是有缺陷的。其他西格玛因素参与对IC1270菌株几丁质分解活性的调节。与亲本菌株相比, grrA grrS rpoS 突变体抑制 solhisthonia solani 的能力明显降低。和 Pythium aphanidermatum 在温室条件下,表明菌株IC1270的生物防治特性对GrrA / GrrS和RpoS全球调节剂的依赖性。

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