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首页> 外文期刊>Microbiology >The molecular basis for the differential regulation of the hlyE-encoded haemolysin of Escherichia coli by FNR and HlyX lies in the improved Activating Region 1 contact of HlyX
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The molecular basis for the differential regulation of the hlyE-encoded haemolysin of Escherichia coli by FNR and HlyX lies in the improved Activating Region 1 contact of HlyX

机译:FNR和Hlyx的HALEE-COMODIA COLI的HLYE编码的HALE-编码的HAEMOLISIN的差异调节的分子基于HLYX的改进的活化区域1接触

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The regulator of fumarate and nitrate reduction (FNR) protein of Escherichia coli is an oxygen-responsive transcription regulator that acts mainly to activate the transcription of genes associated with anaerobic energy generation during periods of oxygen starvation. The hlyX gene of the swine pathogen Actinobacillus pleuropneumoniae encodes an FNR homologue, HlyX, which can complement the anaerobic respiratory deficiencies of an fnr mutant. However, FNR and HlyX have distinct but overlapping regulons because during anaerobic incubation, hlyX-expressing E. coli K-12 strains produce an otherwise latent haemolysin. The gene encoding the ‘latent’ haemolysin has been designated hlyE and analysis of the promoter region by DNase I footprinting reveals the presence of an FNR- (HlyX-) binding site. Anaerobic expression of an hlyE::lacZ reporter was 6.5-fold higher in hlyX compared to fnr-expressing cells. Both FNR and HlyX recruited RNA polymerase to the hlyE promoter but formed different ternary complexes. One major transcript (tsp1) initiating at 78.5 bp downstream of the FMR-binding site and four minor transcripts initiating at 73.5 (tsp2), 71.5 (tsp3), 63.5 (tsp4) and 62.5 (tsp5) bp from the FNR site were detected. From the position of the FNR box relative to the transcript starts, hlyE is expressed from a Class I FNR-regulated promoter. Substitution of selected FNR amino acids with the residues found in the equivalent positions in HlyX indicated that Activating Region 1 (AR1) of FNR forms a surface encompassing β9 to β11 and that the AR1 contact at Class I promoters is different to that at Class II promoters, although the same surface is involved. The FNR variant, FNR-A225T, combined the properties of FNR (good activation from Class II promoters) and HlyX (good activation of Class I promoters) and conferred the haemolytic phenotype.
机译:大肠杆菌的富马酸盐和硝酸盐还原(FNR)蛋白的调节剂是氧响应转录调节剂,其主要用于激活氧饥饿期间与厌氧能量产生相关的基因的转录。猪病原体Actinobacillus的Hlyx基因Pleuropneumoniae编码了Hlyx的FNR同源物,可以补充FNR突变体的厌氧呼吸缺陷。然而,FNR和Hlyx具有不同但重叠的调节件,因为在厌氧孵育期间,表达E. Coli K-12菌株产生另外潜水蛋白。编码“潜伏”氧血清素的基因已被指定为HLYE,并通过DNA酶I脚印分析启动子区域揭示了FNR-(HLYX-)结合位点的存在。与FNR表达的细胞相比,Hlye :: Lacz报告者的厌氧表达在Hlyx中较高6.5倍。 FNR和Hlyx均赋予Hlye启动子的RNA聚合酶,但形成了不同的三元络合物。检测到在FMR结合位点下游的78.5bp的一个主要转录物(Tsp1)和在73.5(Tsp2),71.5(Tsp3),63.5(Tsp4)和来自FNR位点的71.5(Tsp3)和62.5(Tsp5)Bp的4个次要转录物。从FNR盒的位置相对于转录物开始,Hlye由I类FNR调节启动子表达。选择的FNR氨基酸与在Hlyx的等效位置中发现的残基表明,FnR的活化区域1(AR1)形成包围β9至β11的表面,并且在I类启动子的AR1接触在II类启动子中不同,虽然涉及相同的表面。 FNR变体,FNR-A225T,组合FNR的性质(良好的II类启动子激活)和Hlyx(良好的I类启动子激活)并赋予溶血表型。

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