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通过 Gd³⁺-配合物在脂质双层中对 7TM 膜蛋白进行顺磁掺杂,用于固态 NMR 光谱学。

Paramagnetic doping of a 7TM membrane protein in lipid bilayers by Gd³⁺-complexes for solid-state NMR spectroscopy.

机构信息

Institute for Biophysical Chemistry, Centre for Biomolecular Magnetic Resonance, Goethe-University Frankfurt, Max von Laue Str. 9, 60438, Frankfurt am Main, Germany.

出版信息

J Biomol NMR. 2014 Jan;58(1):27-35. doi: 10.1007/s10858-013-9800-4. Epub 2013 Dec 4.

Abstract

A considerable limitation of NMR spectroscopy is its inherent low sensitivity. Approximately 90 % of the measuring time is used by the spin system to return to its Boltzmann equilibrium after excitation, which is determined by (1)H-T1 in cross-polarized solid-state NMR experiments. It has been shown that sample doping by paramagnetic relaxation agents such as Cu(2+)-EDTA accelerates this process considerably resulting in enhanced sensitivity. Here, we extend this concept to Gd(3+)-complexes. Their effect on (1)H-T1 has been assessed on the membrane protein proteorhodopsin, a 7TM light-driven proton pump. A comparison between Gd(3+)-DOTA, Gd(3+)-TTAHA, covalently attached Cu(2+)-EDTA-tags and Cu(2+)-EDTA reveals a 3.2-, 2.6-, 2.4- and 2-fold improved signal-to-noise ratio per unit time due to longitudinal paramagnetic relaxation enhancement. Furthermore, Gd(3+)-DOTA shows a remarkably high relaxivity, which is 77-times higher than that of Cu(2+)-EDTA. Therefore, an order of magnitude lower dopant concentration can be used. In addition, no line-broadening effects or peak shifts have been observed on proteorhodopsin in the presence of Gd(3+)-DOTA. These favourable properties make it very useful for solid-state NMR experiments on membrane proteins.

摘要

NMR 光谱学的一个相当大的局限性是其固有的低灵敏度。在激发后,自旋系统大约需要 90%的测量时间才能回到其玻尔兹曼平衡,这由(1)H-T1 在交叉极化固态 NMR 实验中决定。已经表明,通过顺磁弛豫剂(例如 Cu(2+)-EDTA)对样品进行掺杂可以大大加速该过程,从而提高灵敏度。在这里,我们将这一概念扩展到 Gd(3+)-配合物。已经评估了它们对膜蛋白蛋白酶蛋白的(1)H-T1 的影响,蛋白酶蛋白是一种 7TM 光驱动质子泵。Gd(3+)-DOTA、Gd(3+)-TTAHA、共价连接的 Cu(2+)-EDTA 标签和 Cu(2+)-EDTA 之间的比较表明,由于纵向顺磁弛豫增强,单位时间的信号与噪声比提高了 3.2、2.6、2.4 和 2 倍。此外,Gd(3+)-DOTA 的弛豫率非常高,是 Cu(2+)-EDTA 的 77 倍。因此,可以使用低得多的掺杂剂浓度。此外,在存在 Gd(3+)-DOTA 的情况下,未观察到蛋白酶蛋白的谱线展宽或峰位移。这些有利的性质使其非常适用于膜蛋白的固态 NMR 实验。

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