Kröger Carsten, Fuchs Thilo M
Zentralinstitut für Ernährungs- und Lebensmittelforschung, Abteilung Mikrobiologie, Technische Universität München, Weihenstephaner Berg 3, D-85354 Freising, Germany.
J Bacteriol. 2009 Jan;191(2):545-54. doi: 10.1128/JB.01253-08. Epub 2008 Nov 14.
Knockout mutation of STM4432 resulted in a growth-deficient phenotype of Salmonella enterica serovar Typhimurium in the presence of myo-inositol (MI) as the sole carbon source. STM4432 is part of a 22.6-kb genomic island which spans STM4417 to STM4436 (genomic island 4417/4436) and is responsible for MI degradation. Genome comparison revealed the presence of this island in only six Salmonella strains and a high variability of the iol gene organization in gram-negative bacteria. Upon nonpolar deletion of 11 island loci, the genes involved in six enzymatic steps of the MI pathway were identified. The generation time of S. enterica serovar Typhimurium in minimal medium with MI decreases with higher concentrations of this polyol. Reverse transcriptase PCR showed five separate transcriptional units encompassing the genes iolA-iolB, iolE-iolG1, iolC1-iolC2, iolD1-iolD2-iolG2, and iolI2-iolH. Luciferase reporter assays revealed a strong induction of their promoters in the presence of MI but not glucose. The main regulator, IolR, was identified due to a reduced lag phase of a strain mutated in STM4417 (iolR). Deletion of iolR resulted in stimulation of the iol operons, indicating its negative effect on the iol genes of S. enterica serovar Typhimurium in rich medium at a transcriptional level. Bandshift assays demonstrated the binding of this putative repressor to promoter sequences of iolA, iolC1, and iolD1. Binding of IolR to its own promoter and induced iolR expression in an IolR-negative background demonstrate that its transcription is autoregulated. This is the first characterization of MI degradation in a gram-negative bacterium, revealing a complex transcriptional organization and regulation of the S. enterica serovar Typhimurium iol genes.
在以肌醇(MI)作为唯一碳源的情况下,STM4432基因的敲除突变导致鼠伤寒沙门氏菌出现生长缺陷型表型。STM4432是一个22.6 kb基因组岛的一部分,该基因组岛跨越STM4417至STM4436(基因组岛4417/4436),负责MI的降解。基因组比较显示,仅在六种沙门氏菌菌株中存在该岛,并且革兰氏阴性菌中iol基因组织具有高度变异性。在对11个岛位点进行非极性缺失后,鉴定出了参与MI途径六个酶促步骤的基因。在含有MI的基本培养基中,鼠伤寒沙门氏菌的代时随着该多元醇浓度的升高而降低。逆转录酶PCR显示有五个独立的转录单元,包括iolA - iolB、iolE - iolG1、iolC1 - iolC2、iolD1 - iolD2 - iolG2和iolI2 - iolH基因。荧光素酶报告基因检测显示,在存在MI而非葡萄糖的情况下,其启动子受到强烈诱导。由于STM4417(iolR)突变菌株的延迟期缩短,鉴定出了主要调节因子IolR。iolR的缺失导致iol操纵子受到刺激,表明其在丰富培养基中对鼠伤寒沙门氏菌iol基因在转录水平上具有负效应。凝胶迁移实验证明了这种假定的阻遏物与iolA、iolC1和iolD1启动子序列的结合。IolR与其自身启动子的结合以及在IolR阴性背景下诱导的iolR表达表明其转录是自动调节的。这是对革兰氏阴性菌中MI降解的首次表征,揭示了鼠伤寒沙门氏菌iol基因复杂的转录组织和调控。