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Single-Molecule Observation of Ligand Binding and Conformational Changes in FeuA

机译:Feua的配体结合和构象变化的单分子观察

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摘要

The specific binding of ligands by proteins and the coupling of this process to conformational changes is fundamental to protein function. We designed a fluorescence-based single-molecule assay and data analysis procedure that allows the simultaneous real-time observation of ligand binding and conformational changes in FeuA. The substrate-binding protein FeuA binds the ligand ferri-bacillibactin and delivers it to the ATP-binding cassette importer FeuBC, which is involved in bacterial iron uptake. The conformational dynamics of FeuA was assessed via Förster resonance energy transfer, whereas the presence of the ligand was probed by fluorophore quenching. We reveal that ligand binding shifts the conformational equilibrium of FeuA from an open to a closed conformation. Ligand binding occurs via an induced-fit mechanism, i.e., the ligand binds to the open state and subsequently triggers a rapid closing of the protein. However, FeuA also rarely samples the closed conformation without the involvement of the ligand. This shows that ligand interactions are not required for conformational changes in FeuA. However, ligand interactions accelerate the conformational change 10,000-fold and temporally stabilize the formed conformation 250-fold.
机译:配体通过蛋白质的特异性结合和该方法的偶联以构象变化是对蛋白质功能的基础。我们设计了一种基于荧光的单分子测定和数据分析程序,允许同时实时观察Feua的配体结合和构象变化。底物结合蛋白Feua结合配体Ferri-bacillibactin,并将其递送至ATP结合盒进口剂Feufubc,其参与细菌熨斗吸收。通过Förster共振能量转移评估Feua的构象动态,而通过荧光团猝灭探测配体的存在。我们揭示了配体结合使Feua的构象平衡从开放到闭合构象移动。通过诱导配合机制发生配体结合,即配体与开口状态结合,随后触发蛋白质的快速关闭。然而,Feua也很少在没有配体的累及的情况下对闭合构象进行采样。这表明FEUA的构象变化不需要配体相互作用。然而,配体相互作用加速了10,000倍的构象变化,并在时间稳定形成的构象250倍。

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