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DNA binding of the transcription activator protein meIR from Escherichia coli and its C-terminal domain

机译:大肠杆菌转录激活蛋白meIR及其C端结构域的DNA结合

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摘要

MeIR is an Escherichia coli transcription factor belonging to the AraC family. It activates expression of the meIAB operon in response to melibiose. Full-length MeIR (MeIR303) binds to two pairs of sites upstream of the meIAB transcription start site, denoted sites 1' and 1 and sites 2 and 2', and to a fifth site, R, which overlaps the divergent meIR promoter. The C-terminal domain of MeIR (MeIR173) does not activate transcription. Here we show that, like MeIR3103, when MeIR173 binds to sites 1 and 2 it recruits CRP to bind between these sites. Hence, the C-terminal domain is involved in heterologous interactions. MeIR173 binds to the R site, which has 11 of 18 bp identical to sites 1 and 2 but, surprisingly, does not bind to site 1', which has 12 of 18 bp identical, nor to site 2'. Using electrophoretic mobility shift assays, we show that the binding of MeIR303 to sites 1' and 2' is due to cooperative binding with the adjacent site. This homologous cooparativity requires the N-terminal domain of the protein. Activation of the meIAB promoter requires MeIR to occupy site 2', which overlaps the -35 hexamer. Hence, both domains of MeIR are required for transcription activation.
机译:MeIR是属于AraC家族的大肠杆菌转录因子。它响应于蜜二糖而激活meIAB操纵子的表达。全长MeIR(MeIR303)结合到meIAB转录起始位点上游的两对位点(表示为位点1'和1以及位点2和2'),并结合到第五位点R,该位点与发散的meIR启动子重叠。 MeIR的C末端结构域(MeIR173)不激活转录。在这里,我们表明,就像MeIR3103一样,当MeIR173结合到位点1和2时,它募集CRP来结合这些位点之间。因此,C-末端结构域参与异源相互作用。 MeIR173结合R位点,R位点具有与位点1和2相同的18bp的11个碱基,但是令人惊讶地,它不结合位点1',其具有18bp的12个相同的碱基,也没有位点2'。使用电泳迁移率变动分析,我们显示MeIR303与位点1'和2'的结合是由于与相邻位点的协同结合。这种同源的共亲和性需要蛋白质的N-末端结构域。 meIAB启动子的激活需要MeIR占据位点2',该位点与-35六聚体重叠。因此,MeIR的两个域都是转录激活所必需的。

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