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Lipid bilayer preparations of membrane proteins for oriented and magic-angle spinning solid-state NMR samples

机译:用于定向和魔角旋转固态NMR样品的膜蛋白脂质双层制备

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摘要

Solid-state NMR spectroscopy has been used successfully for characterizing the structure and dynamics of membrane proteins as well as their interactions with other proteins in lipid bilayers. Such an environment is often necessary for achieving native-like structures. Sample preparation is the key to this success. Here we present a detailed description of a robust protocol that results in high-quality membrane protein samples for both magic-angle spinning and oriented-sample solid-state NMR. The procedure is demonstrated using two proteins: CrgA (two transmembrane helices) and Rv1861 (three transmembrane helices), both from Mycobacterium tuberculosis. The success of this procedure relies on two points. First, for samples for both types of NMR experiment, the reconstitution of the protein from a detergent environment to an environment in which it is incorporated into liposomes results in 'complete' removal of detergent. Second, for the oriented samples, proper dehydration followed by rehydration of the proteoliposomes is essential. By using this protocol, proteoliposome samples for magic-angle spinning NMR and uniformly aligned samples (orientational mosaicity of <1) for oriented-sample NMR can be obtained within 10 d.
机译:固态NMR光谱已成功用于表征膜蛋白的结构和动力学以及它们与脂质双层中其他蛋白的相互作用。这样的环境通常对于实现类似本地的结构是必需的。样品制备是成功的关键。在这里,我们介绍了一个健壮的协议的详细说明,该协议可为魔角旋转和定向样本固态NMR生成高质量的膜蛋白样本。使用来自结核分枝杆菌的两种蛋白质:CrgA(两个跨膜螺旋)和Rv1861(三个跨膜螺旋)证明了该程序。此过程的成功取决于两点。首先,对于两种类型的NMR实验样品,蛋白质从去污剂环境到将其掺入脂质体的环境的重构都会导致去污剂的“完全”去除。其次,对于定向样品,适当的脱水以及随后的蛋白脂质体的再水化是必不可少的。通过使用该协议,可以在10 d内获得用于魔角旋转NMR的蛋白脂质体样品和用于取向样品NMR的均匀排列的样品(原始镶嵌度<1)。

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