Moorthy Sudha, Mahadevan S
Department of Molecular Reproduction, Development, and Genetics, Indian Institute of Science, Bangalore 560012, India.
J Bacteriol. 2002 Jul;184(14):4033-8. doi: 10.1128/JB.184.14.4033-4038.2002.
The bgl promoter is silent in wild-type Escherichia coli under standard laboratory conditions, and as a result, cells exhibit a beta-glucoside-negative (Bgl-) phenotype. Silencing is brought about by negative elements that flank the promoter and include DNA structural elements and sequences that interact with the nucleoid-associated protein H-NS. Mutations that confer a Bgl+ phenotype arise spontaneously at a detectable frequency. Transposition of DNA insertion elements within the regulatory locus, bglR, constitutes the major class of activating mutations identified in laboratory cultures. The rpoS-encoded sigmaS, the stationary-phase sigma factor, is involved in both physiological as well as genetic changes that occur in the cell under stationary-state conditions. In an attempt to see if the rpoS status of the cell influences the nature of the mutations that activate the bgl promoter, we analyzed spontaneously arising Bgl+ mutants in rpoS+ and rpoS genetic backgrounds. We show that the spectrum of activating mutations in rpoS cells is different from that in rpoS+ cells. Unlike rpoS+ cells, where insertions in bglR are the predominant activating mutations, mutations in hns make up the majority in rpoS cells. The physiological significance of these differences is discussed in the context of survival of natural populations of E. coli.
在标准实验室条件下,bgl启动子在野生型大肠杆菌中是沉默的,因此细胞呈现β-葡萄糖苷阴性(Bgl-)表型。沉默是由启动子侧翼的负调控元件引起的,这些元件包括DNA结构元件以及与类核相关蛋白H-NS相互作用的序列。赋予Bgl+表型的突变会以可检测到的频率自发产生。DNA插入元件在调控位点bglR内的转座构成了在实验室培养物中鉴定出的主要激活突变类型。由rpoS编码的σS,即稳定期σ因子,参与了细胞在稳定状态条件下发生的生理和遗传变化。为了探究细胞的rpoS状态是否会影响激活bgl启动子的突变性质,我们分析了rpoS+和rpoS基因背景下自发产生的Bgl+突变体。我们发现rpoS细胞中的激活突变谱与rpoS+细胞中的不同。与rpoS+细胞不同,在rpoS+细胞中bglR中的插入是主要的激活突变,而在rpoS细胞中,hns中的突变占大多数。这些差异的生理意义将在大肠杆菌自然种群生存的背景下进行讨论。