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通过质子浴的平衡再平衡实现反复交叉极化接触:用于在磁定向双胶束中重组的膜蛋白的 NMR 灵敏度增强。

Repetitive cross-polarization contacts via equilibration-re-equilibration of the proton bath: Sensitivity enhancement for NMR of membrane proteins reconstituted in magnetically aligned bicelles.

机构信息

Department of Chemistry, North Carolina State University, 2620 Yarbrough Drive, Raleigh, NC 27695-8204, United States.

出版信息

J Magn Reson. 2011 Sep;212(1):245-8. doi: 10.1016/j.jmr.2011.06.028. Epub 2011 Jul 2.

DOI:10.1016/j.jmr.2011.06.028
PMID:21784682
Abstract

Thermodynamic limit of magnetization corresponding to the intact proton bath usually cannot be transferred in a single cross-polarization contact. This is mainly due to the finite ratio between the number densities of the high- and low-gamma nuclei, quantum-mechanical bounds on spin dynamics, and Hartmann-Hahn mismatches due to rf field inhomogeneity. Moreover, for fully hydrated membrane proteins refolded in magnetically oriented bicelles, short spin-lock relaxation times (T1ρ) and rf heating can further decrease cross polarization efficiency. Here we show that multiple equilibrations-re-equilibrations of the high- and low-spin reservoirs during the preparation period yield an over twofold gain in the magnetization transfer as compared to a single-contact cross polarization (CP), and up to 45% enhancement as compared to the mismatch-optimized CP-MOIST scheme for bicelle-reconstituted membrane proteins. This enhancement is achieved by employing the differences between the spin-lattice relaxation times for the high- and low-gamma spins. The new technique is applicable to systems with short T1ρ's, and speeds up acquisition of the multidimensional solid-state NMR spectra of oriented membrane proteins for their subsequent structural and dynamic studies.

摘要

与完整的质子浴对应的磁化强度热力学极限通常无法在单个交叉极化接触中传递。这主要是由于高低γ核的数密度比、自旋动力学的量子力学限制以及由于射频场不均匀性导致的哈特曼-哈恩失配。此外,对于在磁定向双型脂质体中重新折叠的完全水合膜蛋白,短自旋锁定弛豫时间 (T1ρ) 和射频加热会进一步降低交叉极化效率。在这里,我们表明在制备期间对高低自旋库进行多次平衡-再平衡可使磁化转移比单次接触交叉极化 (CP) 增加两倍以上,并且与双型脂质体重建膜蛋白的最佳失配 CP-MOIST 方案相比,增强高达 45%。这种增强是通过利用高低γ自旋的晶格弛豫时间之间的差异来实现的。该新技术适用于 T1ρ 较短的系统,并加快了定向膜蛋白的多维固态 NMR 谱的采集,以进行后续的结构和动力学研究。

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