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Solid-state 19F-NMR analysis of 19F-labeled tryptophan in gramicidin A in oriented membranes.

机译:定向膜中短杆菌肽A中19F标记色氨酸的固态19F-NMR分析。

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摘要

The response of membrane-associated peptides toward the lipid environment or other binding partners can be monitored by solid-state NMR of suitably labeled side chains. Tryptophan is a prominent amino acid in transmembrane helices, and its (19)F-labeled analogues are generally biocompatible and cause little structural perturbation. Hence, we use 5F-Trp as a highly sensitive NMR probe to monitor the conformation and dynamics of the indole ring. To establish this (19)F-NMR strategy, gramicidin A was labeled with 5F-Trp in position 13 or 15, whose chi(1)/chi(2) torsion angles are known from previous (2)H-NMR studies. First, the alignment of the (19)F chemical shift anisotropy tensor within the membrane was deduced by lineshape analysis of oriented samples. Next, the three principal axes of the (19)F chemical shift anisotropy tensor were assigned within the molecular frame of the indole ring. Finally, determination of chi(1)/chi(2) for 5F-Trp in the lipid gel phase showed that the side chain alignment differs by up to 20 degrees from its known conformation in the liquid crystalline state. The sensitivity gain of (19)F-NMR and the reduction in the amount of material was at least 10-fold compared with previous (2)H-NMR studies on the same system and 100-fold compared with (15)N-NMR.
机译:膜相关肽对脂质环境或其他结合伴侣的反应可以通过适当标记的侧链的固态NMR进行监测。色氨酸是跨膜螺旋中的重要氨基酸,其(19)F标记的类似物通常具有生物相容性,几乎不会引起结构扰动。因此,我们使用5F-Trp作为高灵敏度NMR探针来监测吲哚环的构象和动力学。为了建立此(19)F-NMR策略,将麦地西丁A在位置13或15中标记为5F-Trp,从先前的(2)H-NMR研究可知其chi(1)/ chi(2)扭转角。首先,通过定向样品的线形分析推导了膜内(19)F化学位移各向异性张量的排列。接下来,在吲哚环的分子框架内分配(19)F化学位移各向异性张量的三个主轴。最后,在脂质凝胶相中测定5F-Trp的chi(1)/ chi(2)表明,侧链排列与其在液晶态下的已知构象相差最多20度。与以前在相同系统上进行的(2)H-NMR研究相比,(19)F-NMR的灵敏度提高和材料数量的减少至少10倍,而与(15)N-NMR相比则为100倍。

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