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Essential Role of the Iron-Regulated Outer Membrane Receptor FauA in Alcaligin Siderophore-Mediated Iron Uptake in Bordetella Species

机译:铁型外膜受体FAUA在嗜血杆菌介导的博德菌介导的铁摄取的基本作用

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摘要

Phenotypic analysis using heterologous host systems localized putative Bordetella pertussis ferric alcaligin transport genes and Fur-binding sequences to a 3.8-kb genetic region downstream from the alcR regulator gene. Nucleotide sequencing identified a TonB-dependent receptor family homolog gene, fauA, predicted to encode a polypeptide with high amino acid sequence similarity with known bacterial ferric siderophore receptors. In Escherichia coli, the fauA genes of both B. pertussis and Bordetella bronchiseptica directed the production of a 79-kDa polypeptide, approximating the predicted size of the mature FauA protein. B. bronchiseptica fauA insertion mutant BRM17 was unable to utilize ferric alcaligin, and in complementation analyses ferric alcaligin utilization was restored to this mutant by supplying the wild-type fauA gene in trans. Mutant BRM18, carrying a nonpolar in-frame fauA deletion mutation, was defective in ferric alcaligin utilization and 55Fe-ferric alcaligin uptake and no longer produced a 79-kDa iron-regulated outer membrane protein. In complementation analyses, BRM18 merodiploids bearing the wild-type fauA gene in trans regained ferric alcaligin siderophore transport and utilization functions and produced the 79-kDa protein. Analysis of a plasmid-borne fauA-lacZ operon fusion confirmed that fauA is subject to iron regulation at the transcriptional level and that cis-acting transcriptional control elements mediating fauA iron repressibility reside within the 3.8-kb PstI fauA DNA region. Moreover, expression of the fauA-lacZ fusion gene under iron starvation conditions was shown to be alcR dependent. FauA is a 79-kDa iron-regulated outer membrane receptor protein required for transport and utilization of ferric alcaligin siderophore complexes by Bordetella species. Originally published Journal of Bacteriology, Vol. 181, No. 19, Oct 1999
机译:使用异源宿主系统的表型分析局部推定的Bordetella Pertroseissis Ferric Alcaligin运输基因和毛皮结合序列到Alcr调节剂基因下游的3.8kb遗传区域。核苷酸测序确定了的TonB依赖性受体家族同系物基因,fauA,预测其编码的多肽具有高氨基与已知的细菌三价铁载体受体酸序列相似性。在大肠杆菌中,B.Pertussis和Bordetella Bronchiseptica的Faua基因指导了79kDa多肽的产生,近似于成熟的假蛋白的预测尺寸。 B. Bronchiseptica Faua插入突变体BRM17不能利用氟丙氨酸,并且在互补分析中,通过在反式中供应野生型假型基因来恢复到该突变体中的丙碳素利用。突变体BRM18,携带非框架内毛毛缺失突变,在氟碳植物利用和55次氟葡萄酒摄取,不再产生79 kDa铁调节的外膜蛋白。在互补分析中,BRM18携带野生型FAUA基因的BRM18 Metodipss在反式中恢复过氟苯葡萄酒铁素铁孔运输和利用函数,并产生了79-KDA蛋白。分析质粒传播的FAUA-LACZ操纵子融合证实,假影在转录水平上受到铁调节的影响,并且CIS作用转录对照元素介导人工失用率的转铁抑制性在3.8-Kb Psti Faua DNA区域内。此外,证明了铁饥饿条件下的FAUA-LacZ融合基因的表达被依赖于ALCR。 FAUA是由Bordetella物种运输和利用Ferric alcaligin Siderophores络合物所需的79kDa铁管制外膜受体蛋白。最初公布的细菌学杂志,Vol。 1999年10月19日181日

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