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Generating a metal-responsive transcriptional regulator to test what confers metal-sensing in cells.

机译:产生金属反应性转录调节剂,以测试赋予细胞金属感测的物质。

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摘要

FrmR from Salmonella enterica serovar typhimurium (a CsoR/RcnR-like transcriptional de-repressor) is shown to repress the frmRA operator-promoter, and repression is alleviated by formaldehyde but not manganese, iron, cobalt, nickel, copper, or Zn(II) within cells. In contrast, repression by a mutant FrmRE64H (which gains an RcnR metal ligand) is alleviated by cobalt and Zn(II). Unexpectedly, FrmR was found to already bind Co(II), Zn(II), and Cu(I), and moreover metals, as well as formaldehyde, trigger an allosteric response that weakens DNA affinity. However, the sensory metal sites of the cells' endogenous metal sensors (RcnR, ZntR, Zur, and CueR) are all tighter than FrmR for their cognate metals. Furthermore, the endogenous metal sensors are shown to out-compete FrmR. The metal-sensing FrmRE64H mutant has tighter metal affinities than FrmR by approximately 1 order of magnitude. Gain of cobalt sensing by FrmRE64H remains enigmatic because the cobalt affinity of FrmRE64H is substantially weaker than that of the endogenous cobalt sensor. Cobalt sensing requires glutathione, which may assist cobalt access, conferring a kinetic advantage. For Zn(II), the metal affinity of FrmRE64H approaches the metal affinities of cognate Zn(II) sensors. Counter-intuitively, the allosteric coupling free energy for Zn(II) is smaller in metal-sensing FrmRE64H compared with nonsensing FrmR. By determining the copies of FrmR and FrmRE64H tetramers per cell, then estimating promoter occupancy as a function of intracellular Zn(II) concentration, we show how a modest tightening of Zn(II) affinity, plus weakened DNA affinity of the apoprotein, conspires to make the relative properties of FrmRE64H (compared with ZntR and Zur) sufficient to sense Zn(II) inside cells.
机译:沙门氏菌沙门氏菌血清型鼠伤寒沙门氏菌(CsoR / RcnR样转录去阻遏物)的FrmR被显示可抑制frmRA操纵子启动子,而甲醛,锰,铁,钴,镍,铜或锌(II )。相反,钴和Zn(II)减轻了突变型FrmRE64H(获得RcnR金属配体)的抑制作用。出乎意料的是,发现FrmR已结合Co(II),Zn(II)和Cu(I),而且金属以及甲醛会触发变构反应,从而削弱DNA亲和力。但是,细胞内源性金属传感器(RcnR,ZntR,Zur和CueR)的感觉金属位点对于同源金属均比FrmR紧。此外,内源金属传感器的性能优于FrmR。金属感测的FrmRE64H突变体比FrmR具有更紧密的金属亲和力,约为1个数量级。由于FrmRE64H的钴亲和力远弱于内源钴传感器的钴亲和力,因此FrmRE64H对钴的感测增益仍然难以捉摸。钴感测需要谷胱甘肽,这可能有助于钴的进入,从而赋予了动力学优势。对于Zn(II),FrmRE64H的金属亲和力接近同源Zn(II)传感器的金属亲和力。与直觉相反,与无感FrmR相比,金属感测FrmRE64H中Zn(II)的变构偶联自由能较小。通过确定每个细胞的FrmR和FrmRE64H四聚体的拷贝,然后估计启动子的占有率作为细胞内Zn(II)浓度的函数,我们表明Zn(II)亲和力的适度收紧加上载脂蛋白的弱DNA亲和力如何共谋使FrmRE64H(与ZntR和Zur相比)的相对特性足以感测细胞内的Zn(II)。

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