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Conformation of spin-labeled melittin at membrane surfaces investigated by pulse saturation recovery and continuous wave power saturation electron paramagnetic resonance.

机译:通过脉冲饱和度恢复和连续波功率饱和电子顺磁共振研究膜表面自旋标记的蜂毒肽的构象。

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摘要

Melittin spin-labeled specifically with a nitroxide at positions 7, 21, 23, or the amino terminus was bound to phospholipid membranes, and the exposure of the spin label to the aqueous phase was investigated by measurement of Heisenberg exchange with chromium oxalate in the solution. The exchange frequency was determined by saturation recovery electron paramagnetic resonance (EPR) using a loop-gap resonator. This method allows use of very low concentrations (less than 1 mM) of chromium oxalate compared with conventional measurements of EPR line broadening (typically 50 mM), thus avoiding problems associated with high metal ion concentration. Differences in exchange frequency between the various positions were also estimated by continuous wave power saturation methods. In either approach, the spin label at lysine 7 was found to be the most exposed to chromium oxalate whereas that at lysine 23 was found to be the least exposed. This is consistent with a model for the membrane bound peptide in which an amphiphilic helix lies with its axis parallel to the bilayer surface and the hydrophobic moment points toward the bilayer interior.
机译:分别在7、21、23或氨基末端用一氧化氮自旋标记的Melittin结合到磷脂膜上,通过测量溶液中与草酸铬的Heisenberg交换来研究自旋标记物在水相中的暴露。交换频率通过使用环隙谐振器的饱和恢复电子顺磁共振(EPR)确定。与传统的EPR谱线加宽(通常为50 mM)测量相比,该方法允许使用非常低的草酸铬浓度(小于1 mM),从而避免了与高金属离子浓度相关的问题。还通过连续波功率饱和方法估算了各个位置之间交换频率的差异。在这两种方法中,发现赖氨酸7处的自旋标记暴露于草酸铬最多,而赖氨酸23处的自旋标记暴露最少。这与膜结合的肽的模型一致,在该模型中,两亲性螺旋的轴平行于双层表面,而疏水力矩指向双层内部。

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