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Site-Specific Incorporation of a Cu2+ Spin-Label into Proteins for Measuring Distances by Pulsed Dipolar ESR Spectroscopy

机译:特定位置将Cu2 +自旋标签掺入蛋白质中以通过脉冲双极ESR光谱法测量距离

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摘要

Pulsed dipolar ESR spectroscopy (PDS) is a powerful tool for measuring distances in solution-state macromolecules. Paramagnetic metal ions, such as Cu2+, are useful spin probes because they can report on metalloproteins features and can be spectroscopically distinguished from traditional ni-troxide (NO)-based labels. Here we demonstrate site-specific incorporation of Cu2+ into non-metalloproteins through use of a genetically encodable non-natural amino acid, 3-pyrazolyltyrosine (PyTyr). We first incorporate PyTyr in cyan-fluorescent protein (CFP) to measure Cu2+-to-NO distances and examine the effects of solvent conditions on Cu2+ binding and protein aggregation. We then apply the method to characterize the complex formed by the histidine kinase CheA and its target response reg-ulator CheY. The x-ray structure of CheY-PyTyr confirms Cu labeling at PyTyr but also reveals a secondary Cu site. Cu2+-to-NO and Cu2+-to-Cu2+ PDS measurements of CheY-PyTyr with nitroxide-labeled CheA provide new insight into the conformational landscape of the phosphotransfer complex and have implications for kinase regulation.
机译:脉冲偶极ESR光谱仪(PDS)是用于测量溶液态大分子中距离的强大工具。顺磁性金属离子(例如Cu 2 + )是有用的自旋探针,因为它们可以报告金属蛋白的特征,并且可以在光谱上与传统的基于一氧化氮(NO)的标记区分开。在这里,我们展示了通过使用可遗传编码的非天然氨基酸3-吡唑基酪氨酸(PyTyr),将Cu 2 + 特异性结合到非金属蛋白中。我们首先将PyTyr掺入青色荧光蛋白(CFP)中以测量Cu 2 + -NO的距离,并研究溶剂条件对Cu 2 + 结合和蛋白质的影响聚合。然后,我们应用该方法来表征由组氨酸激酶CheA及其靶标反应调节剂CheY形成的复合物。 CheY-PyTyr的X射线结构证实了PyTyr处的Cu标记,但还揭示了一个次级Cu位。使用亚硝酸盐标记的CheA对CheY-PyTyr进行Cu 2 + -to-NO和Cu 2 + -to-Cu 2 + PDS测量可提供磷酸转移复合物的构象格局的新见解,对激酶调节具有重要意义。

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