大肠杆菌的两个胞质外功能σ亚基,σ(E)和σ(FecI):启动子选择性和细胞内水平。
Two extracytoplasmic function sigma subunits, sigma(E) and sigma(FecI), of Escherichia coli: promoter selectivity and intracellular levels.
作者信息
Maeda H, Jishage M, Nomura T, Fujita N, Ishihama A
机构信息
National Institute of Genetics, Department of Molecular Genetics, Mishima, Shizuoka 411-5840, Japan.
出版信息
J Bacteriol. 2000 Feb;182(4):1181-4. doi: 10.1128/JB.182.4.1181-1184.2000.
Abstract
The promoter selectivity of two extracytoplasmic function (ECF) subfamily sigma subunits, sigma(E) (sigma(24)) and sigma(FecI) (sigma(18)), of Escherichia coli RNA polymerase was analyzed by using an in vitro transcription system and various promoters. The Esigma(E) holoenzyme recognized only the known cognate promoters, rpoEP2, rpoHP3, and degP, and the Esigma(FecI) recognized only one known cognate promoter, fecA. The strict promoter recognition properties of sigma(E) and sigma(FecI) are similar to those of other minor sigma subunits. Transcription by Esigma(E) and Esigma(FecI) was enhanced by high concentrations of glutamate, as in the case of other minor sigma subunits. The optimum temperature for transcription by Esigma(FecI) was low, around 25 degrees C, apparently in agreement with the high rate of iron sequestration by E. coli at low temperatures. By quantitative Western blot analysis, the intracellular levels of sigma(E) and sigma(FecI) in the uninduced steady-state culture of E. coli W3110 (type A) were determined to be 0.7 to 2.0 and 0.1 to 0.2 fmol per microg of total proteins (or 3 to 9 and 0.4 to 0.9 molecules per cell), respectively, and less than 1% of the level of the major sigma(70) subunit.
摘要
利用体外转录系统和各种启动子,分析了大肠杆菌RNA聚合酶的两个胞质外功能(ECF)亚家族的σ亚基σ(E)(σ(24))和σ(FecI)(σ(18))的启动子选择性。Esigma(E)全酶仅识别已知的同源启动子rpoEP2、rpoHP3和degP,而Esigma(FecI)仅识别一个已知的同源启动子fecA。σ(E)和σ(FecI)严格的启动子识别特性与其他次要σ亚基相似。与其他次要σ亚基一样,高浓度的谷氨酸可增强Esigma(E)和Esigma(FecI)的转录。Esigma(FecI)转录的最适温度较低,约为25℃,这显然与大肠杆菌在低温下的高铁螯合率一致。通过定量蛋白质免疫印迹分析,确定在未诱导的大肠杆菌W3110(A型)稳态培养物中,σ(E)和σ(FecI)的细胞内水平分别为每微克总蛋白0.7至2.0飞摩尔和0.
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