首页> 外文期刊>Journal of the American Chemical Society >Asymmetric Insertion of Membrane Proteins in Lipid Bilayers by Solid-State NMR Paramagnetic Relaxation Enhancement: A Cell-Penetrating Peptide Example
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Asymmetric Insertion of Membrane Proteins in Lipid Bilayers by Solid-State NMR Paramagnetic Relaxation Enhancement: A Cell-Penetrating Peptide Example

机译:通过固态NMR顺磁弛豫增强膜蛋白在脂质双层中的不对称插入:细胞穿透肽的例子。

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摘要

A novel solid-state NMR technique for identifying the asymmetric insertion depths of membrane proteins in lipid bilayers is introduced. By applying Mn~(2+) ions on the outer but not the inner leaflet of lipid bilayers, the sidedness of protein residues in the lipid bilayer can be determined through paramagnetic relaxation enhancement (PRE) effects. Protein-free lipid membranes with one-side Mn~(2+)-bound surfaces exhibit significant residual~(31)P and lipid headgroup~(13)C intensities, in contrast to two-side Mn~(2+)-bound membranes, where lipid headgroup signals are mostly suppressed. Applying this method to a cell-penetrating peptide, penetratin, we found that at low peptide concentrations, penetratin is distributed in both leaflets of the bilayer, in contrast to the prediction of the electroporation model, which predicts that penetratin binds to only the outer lipid leaflet at low peptide concentrations to cause an electric field that drives subsequent peptide translocation. The invalidation of the electroporation model suggests an alternative mechanism for intracellular import of penetratin, which may involve guanidinium-phosphate complexation between the peptide and the lipids.
机译:介绍了一种新颖的固态NMR技术,用于识别脂质双层中膜蛋白的不对称插入深度。通过在脂质双层的外部而非内部小叶上施加Mn〜(2+)离子,可以通过顺磁弛豫增强(PRE)效应确定脂质双层中蛋白质残基的侧面。与两侧Mn〜(2+)结合相反,具有一侧Mn〜(2+)结合表面的无蛋白脂质膜表现出显着的残留〜(31)P和脂质头基〜(13)C强度。膜,其中脂质头基团信号大部分被抑制。将这种方法应用于穿透细胞的肽Penetratin,我们发现在低肽浓度下,Penetratin分布在双层的两个小叶中,这与电穿孔模型的预测相反,后者预测了Penetratin仅与外部脂质结合低肽浓度的小叶会引起电场,从而驱动随后的肽易位。电穿孔模型的无效提示了渗透剂渗透细胞内的另一种机制,这可能涉及肽和脂质之间的胍盐-磷酸络合。

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