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Secondary structure and DNA binding by the C-terminal domain of the transcriptional activator NifA from Klebsiella pneumoniae

机译:肺炎克雷伯氏菌转录激活因子NifA的C末端结构域的二级结构和DNA结合

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摘要

The NifA protein of Klebsiella pneumoniae is required for transcriptional activation of all nitrogen fixation (nif) operons except the regulatory nifLA genes. At these operons, NifA binds to an upstream activator sequence (UAS), with the consensus TGT-N10-ACA, via a C-terminal DNA-binding domain (CTD). Binding of the activator to this upstream enhancer-like sequence allows NifA to interact with RNA polymerase containing the alternative sigma factor, σ54. The isolated NifA CTD is monomeric and binds specifically to DNA in vitro as shown by DNase I footprinting. Heteronuclear 3D NMR experiments have been used to assign the signals from the protein backbone. Three α-helices have been identified, based on secondary chemical shifts and medium range Hαi-NHi + 1, and NHi-NHi + 1 NOEs. On addition of DNA containing a half-site UAS, several changes are observed in the NMR spectra, allowing the identification of residues that are most likely to interact with DNA. These occur in the final two helices of the protein, directly confirming that DNA binding is mediated by a helix–turn–helix motif.
机译:除调节性nifLA基因外,所有氮固定(nif)操纵子的转录激活都需要肺炎克雷伯菌的NifA蛋白。在这些操纵子处,NifA通过共有的TGT-N10-ACA经由C端DNA结合域(CTD)与上游激活子序列(UAS)结合。激活剂与该上游增强子样序列的结合使NifA与包含替代σ因子σ54的RNA聚合酶相互作用。分离的NifA CTD是单体的,在体外特异性结合DNA,如DNase I足迹所示。异核3D NMR实验已用于分配蛋白质骨架的信号。基于次级化学位移和中等范围的Hαi-NHi+1和NHi-NHi +1 NOE,已经鉴定出三个α螺旋。添加含有半位点UAS的DNA时,在NMR光谱中观察到一些变化,从而可以鉴定最可能与DNA相互作用的残基。这些发生在蛋白质的最后两个螺旋中,直接证实DNA结合是由螺旋-转-螺旋基序介导的。

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