首页> 外文期刊>Journal of Molecular Biology >Thermodynamics of E. coli cytidine repressor interactions with DNA: distinct modes of binding to different operators suggests a role in differential gene regulation.
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Thermodynamics of E. coli cytidine repressor interactions with DNA: distinct modes of binding to different operators suggests a role in differential gene regulation.

机译:大肠杆菌胞苷阻遏物与DNA相互作用的热力学:结合不同操作员的不同模式表明在差异基因调控中起作用。

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Interactions between the Escherichia coli cytidine repressor protein (CytR) and its operator sites at the different promoters that comprise the CytR regulon, play an important role in the regulation of these promoters. The natural operators are palindromes separated by variable length central spacers (0-9 bp). We have suggested that this variability affects the flexibility of CytR-DNA contacts, thereby affecting the critical protein-protein interactions between CytR and the cAMP receptor protein (CRP) that underlie differential repression and activation of CytR-regulated genes. To assess this hypothesis, we investigated the thermodynamics of CytR binding to the natural operator sequences found in udpP and deoP2. To separate effects due to spacing from effects due to the differing sequences of the recognition half-sites of these two operators, we also investigated CytR binding to artificial hybrid operators, in which the half-site sequences of udpP and deoP2 were exchanged. Thermodynamic parameters, DeltaS(o), DeltaH(o) and DeltaC(o)(p), were determined by van't Hoff analysis of CytR binding, monitored by changes in the steady-state fluorescence anisotropy of dye-conjugated, operator-containing oligonucleotides. Large differences in thermodynamics were observed that depend primarily on the central spacer rather than the sequences of the recognition half-sites. Binding to operators with deoP2 spacing results in a very large, negative DeltaC(o)(p). Association is strongly favored enthalpically and strongly disfavored entropically at ambient temperature. By contrast, binding to operators with udpP spacing results in a small, negative DeltaC(o)(p). Association is weakly favored both enthalpically and entropically at ambient temperature. A difference of such magnitude in DeltaDeltaC(o)(p) has not been reported previously for specific binding of a transcription factor to different sites. The identical salt dependence of CytR binding to deoP2 and udpP operators indicates that ion-dependent processes do not contribute significantly to this difference. Thus, the different thermodynamic effects appear to reflect distinctly different modes of site-specific DNA binding. We discuss similarities to operator binding by CytR homologs among LacI family repressors, and we consider how different CytR binding modes might affect interactions with other components of the gene regulatory machinery that contribute to differential gene regulation.
机译:大肠杆菌胞苷阻遏蛋白(CytR)和其操纵子位点在组成CytR regulon的不同启动子之间的相互作用,在调节这些启动子中起重要作用。自然算子是由可变长度的中央间隔区(0-9 bp)分隔的回文。我们已经表明,这种可变性会影响CytR-DNA接触的灵活性,从而影响CytR和cAMP受体蛋白(CRP)之间的关键蛋白-蛋白相互作用,而这些相互作用是CytR调控基因的差异抑制和激活的基础。为了评估该假设,我们研究了CytR与udpP和deoP2中发现的天然操纵子序列结合的热力学。为了将这两个操纵基因的识别半位点序列不同所产生的间隔效应与间隔效应分开,我们还研究了CytR与人工杂交操纵子的结合,其中udpP和deoP2的半位点序列被交换。热力学参数DeltaS(o),DeltaH(o)和DeltaC(o)(p)通过CytR结合的van't Hoff分析来确定,并通过染料共轭,操作员-染料偶联的稳态荧光各向异性的变化进行监测含有寡核苷酸。观察到热力学的巨大差异,主要取决于中央间隔子,而不是识别半位点的序列。以deoP2间距绑定到运算符会导致非常大的负DeltaC(o)(p)。在环境温度下,缔合在焓上被强烈支持而在熵上被强烈反对。相反,以udpP间距绑定到运算符会导致较小的负DeltaC(o)(p)。在环境温度下,无论是在焓上还是在熵上,缔合都较弱。先前尚未报道过DeltaDeltaC(o)(p)的这种大小差异,该差异是转录因子与不同位点的特异性结合。 CytR与deoP2和udpP操纵子结合的盐依赖性相同,表明离子依赖性过程对这种差异没有明显贡献。因此,不同的热力学效应似乎反映了位点特异性DNA结合的明显不同模式。我们讨论了与LacI家族阻遏物之间CytR同源物与操纵子结合的相似性,并且我们考虑了不同的CytR结合方式可能如何影响与基因调控机制中其他有助于差异基因调控的成分之间的相互作用。

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