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Advancements and Application of Microsecond Synchrotron X-ray Footprinting at the Advanced Light Source

机译:微秒同步加速器X射线足迹在先进光源上的研究进展与应用

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摘要

The method of synchrotron X-ray protein footprinting (XF-MS) is used to determine protein conformational changes, folding, proteinprotein and protein-ligand interactions, providing information which is often difficult to obtain using X-ray crystallography and other common structural biology methods [1–3]. The technique uses comparative in situ labeling of solvent-accessible side chains by highly reactive hydroxyl radicals (?OH) in buffered aqueous solution under different assay conditions. In regions where a protein is folded or binds a partner, these ?OH susceptible sites are inaccessible to solvent, and therefore protected from labeling. The ?OH are generated by the ionization of water using high-flux-density X-rays. High-flux density is a key factor for XF-MS labeling because obtaining an adequate steady-state concentration of hydroxyl radical within a short irradiation time is necessary to minimize radiation-induced secondary damage and also to overcome various scavenging reactions that reduce the yield of labeled side chains.
机译:同步加速器X射线蛋白质足迹法(XF-MS)用于确定蛋白质构象变化,折叠,蛋白质蛋白质和蛋白质配体相互作用,提供了通常难以使​​用X射线晶体学和其他常见结构生物学方法获得的信息[1-3]。该技术在不同的测定条件下,通过在缓冲水溶液中的高反应性羟基自由基(?OH)对溶剂可及的侧链进行了比较原位标记。在蛋白质折叠或结合伴侣的区域中,这些对?OH敏感的位点是溶剂无法接近的,因此可以防止标记。通过使用高通量密度的X射线使水离子化,可以生成αOH。高通量密度是XF-MS标记的关键因素,因为必须在短的照射时间内获得足够的稳态羟基自由基浓度,以最大程度地减少辐射引起的二次破坏,并克服各种降低其收率的清除反应。标记的侧链。

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