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Purification and Reconstitution of TRPV1 for Spectroscopic Analysis

机译:用于光谱分析的TRPV1的纯化和重组

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摘要

Polymodal ion channels transduce multiple stimuli of different natures into allosteric changes; these dynamic conformations are challenging to determine and remain largely unknown. With recent advances in single-particle cryo-electron microscopy (cryo-EM) shedding light on the structural features of agonist binding sites and the activation mechanism of several ion channels, the stage is set for an in-depth dynamic analysis of their gating mechanisms using spectroscopic approaches. Spectroscopic techniques such as electron paramagnetic resonance (EPR) and double electron-electron resonance (DEER) have been mainly restricted to the study of prokaryotic ion channels that can be purified in large quantities. The requirement for large amounts of functional and stable membrane proteins has hampered the study of mammalian ion channels using these approaches. EPR and DEER offer many advantages, including determination of the structure and dynamic changes of mobile protein regions, albeit at low resolution, that might be difficult to obtain by X-ray crystallography or cryo-EM, and monitoring reversible gating transition (i.e., closed, open, sensitized, and desensitized). Here, we provide protocols for obtaining milligrams of functional detergent-solubilized transient receptor potential cation channel subfamily V member 1 (TRPV1) that can be labeled for EPR and DEER spectroscopy.
机译:多峰离子通道将不同性质的多种刺激转化为变构变化;这些动态构象很难确定,并且很大程度上仍然未知。随着单粒子冷冻电子显微镜(cryo-EM)的最新进展使激动剂结合位点的结构特征和几个离子通道的激活机制得以释放,为进一步动态分析其门控机制奠定了基础使用光谱方法。诸如电子顺磁共振(EPR)和双电子电子共振(DEER)之类的光谱技术主要限于可大量纯化的原核离子通道的研究。对大量功能性和稳定的膜蛋白的需求已阻碍了使用这些方法对哺乳动物离子通道的研究。 EPR和DEER具有许多优点,包括确定流动蛋白区域的结构和动态变化(尽管分辨率很低),这可能很难通过X射线晶体学或冷冻EM来获得,并且可以监测可逆的门控转变(即封闭,开放,敏感和不敏感)。在这里,我们提供了协议,以获取可标记为EPR和DEER光谱学的毫克功能性洗涤剂溶解的瞬态受体电位阳离子通道亚家族V成员1(TRPV1)。

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