首页> 美国卫生研究院文献>Journal of Bacteriology >Functional Characterization of Seven γ-Glutamylpolyamine Synthetase Genes and the bauRABCD Locus for Polyamine and β-Alanine Utilization in Pseudomonas aeruginosa PAO1
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Functional Characterization of Seven γ-Glutamylpolyamine Synthetase Genes and the bauRABCD Locus for Polyamine and β-Alanine Utilization in Pseudomonas aeruginosa PAO1

机译:铜绿假单胞菌PAO1中7个γ-谷氨酰胺多胺合成酶基因的功能表征以及bauRABCD位点用于多胺和β-丙氨酸的利用

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摘要

Pseudomonas aeruginosa and many other bacteria can utilize biogenic polyamines, including diaminopropane (DAP), putrescine (Put), cadaverine (Cad), and spermidine (Spd), as carbon and/or nitrogen sources. Transcriptome analysis in response to exogenous Put and Spd led to the identification of a list of genes encoding putative enzymes for the catabolism of polyamines. Among them, pauA1 to pauA6, pauB1 to pauB4, pauC, and pauD1 and pauD2 (polyamine utilization) encode enzymes homologous to Escherichia coli PuuABCD of the γ-glutamylation pathway in converting Put into GABA. A series of unmarked pauA mutants was constructed for growth phenotype analysis. The results revealed that it requires specific combinations of pauA knockouts to abolish utilization of different polyamines and support the importance of γ-glutamylation for polyamine catabolism in P. aeruginosa. Another finding was that the list of Spd-inducible genes overlaps almost completely with that of Put-inducible ones except the pauA3B2 operon and the bauABCD operon (β-alanine utilization). Mutation analysis led to the conclusion that pauA3B2 participate in catabolism of DAP, which is related to the aminopropyl moiety of Spd, and that bauABCD are essential for growth on β-alanine derived from DAP (or Spd) catabolism via the γ-glutamylation pathway. Measurements of the pauA3-lacZ and bauA-lacZ expression indicated that these two promoters were differentially induced by Spd, DAP, and β-alanine but showed no apparent response to Put, Cad, and GABA. Induction of the pauA3 and bauA promoters was abolished in the bauR mutant. The recombinant BauR protein was purified to demonstrate its interactions with the pauA3 and bauA regulatory regions in vitro. In summary, the present study support that the γ-glutamylation pathway for polyamine utilization is evolutionarily conserved in E. coli and Pseudomonas spp. and is further expanded in Pseudomonas to accommodate a more diverse metabolic capacity in this group of microorganisms.
机译:铜绿假单胞菌和许多其他细菌可以利用生物多胺,包括二氨基丙烷(DAP),腐胺(Put),尸胺(Cad)和亚精胺(Spd)作为碳和/或氮源。响应外源Put和Spd的转录组分析导致鉴定了编码假定的多胺分解代谢酶的基因清单。其中,pauA1至pauA6,pauB1至pauB4,pauC以及pauD1和pauD2(多胺利用)编码与转化Put到GABA中的γ-谷氨酰化途径的大肠杆菌PuuABCD同源的酶。构建了一系列未标记的pauA突变体,用于生长表型分析。结果表明,它需要pauA基因敲除的特定组合,才能消除对不同多胺的利用,并支持γ-谷氨酰化对于铜绿假单胞菌中多胺分解代谢的重要性。另一个发现是,除了pauA3B2操纵子和 bauABCD 操纵子(β- a)外,Spd诱导基因的清单与Put诱导基因的清单几乎完全重叠。 lanine u tilization)。突变分析得出的结论是, pauA3B2 参与了DAP的分解代谢,这与Spd的氨丙基部分有关,并且 bauABCD 对于β-丙氨酸衍生的生长是必不可少的通过γ-谷氨酰化途径从DAP(或Spd)分解代谢。对 pauA3-lacZ bauA-lacZ 表达的测量表明,这两个启动子被Spd,DAP和β-丙氨酸差异诱导,但对Put没有明显的反应, Cad和GABA。 bauR 突变体中取消了 pauA3 bauA 启动子的诱导。纯化了重组BauR蛋白,以证明其与 pauA3 bauA 调控区 的相互作用。总而言之,本研究支持γ-谷氨酰化途径用于多胺的利用在 E中在进化上是保守的。大肠杆菌假单胞菌 spp。并在 Pseudomonas 中进一步扩展,以适应这组微生物的新陈代谢能力。

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