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The LipB protein is a negative regulator of dam gene expression in Escherichia coli

机译:LipB蛋白是大肠杆菌中dam基因表达的负调控因子

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Transcription initiation of the major promoter (P2) of the Escherichia coli dam gene increases with growth rate. The presence of three partially palindromic motifs, (TTCAGT(N_(20))TGAG), designated G (growth)-boxes, within the -52 to +31 region of the promoter, may be related to growth rate control. Deletion of two of these repeats, downstream of the transcription initiation point, result in constitutive high activity of the promoter. The unlinked cde-4∷miniTn10 insertion also results in severalfold higher activity of the dam P2 promoter, suggesting that this mutation resulted in the loss of a putative dam P2 repressor. The cde-4 mutation was mapped to the lipB (lipoic acid) gene, which we show encodes a 24 kDa protein initiating at a TTG codon. LipB is a highly conserved protein in animal and plant species. other bacteria Archaea, and yeast. Plasmid expressing the native or hexahistidine-tagged LipB complement the phenotype of the cde-4 mutant strain. The level of LipB in vivo was higher in exponentially growing cells than those in the stationary phase. Three G-box motifs were also found in the lipB region. Models for the regulation of expression of the two genes are discussed.
机译:大肠杆菌dam基因的主要启动子(P2)的转录起始随生长速率增加。在启动子的-52至+31区域内存在三个部分回文基序(TTCAGT(N_(20))TGAG),称为G(生长)盒,可能与生长速率控制有关。在转录起始点的下游,缺失两个这样的重复序列可导致启动子的组成型高活性。未连接的cde-4∷miniTn10插入也导致dam P2启动子的活性提高了几倍,表明该突变导致推定的dam P2阻遏物丢失。将cde-4突变定位到lipB(硫辛酸)基因,我们显示该基因编码从TTG密码子起始的24 kDa蛋白。 LipB是动植物物种中高度保守的蛋白质。其他细菌古细菌和酵母。表达天然或带有六组氨酸标签的LipB的质粒与cde-4突变株的表型互补。指数生长的细胞中体内LipB的水平高于固定相中的水平。在lipB区域还发现了三个G-box基序。讨论了调节两个基因表达的模型。

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