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通过改变磷脂双分子脂质体的大小和电荷来调节液晶和取向凝胶介质中膜蛋白的取向。

Modulating alignment of membrane proteins in liquid-crystalline and oriented gel media by changing the size and charge of phospholipid bicelles.

机构信息

Laboratory of Chemical Physics, National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK), National Institutes of Health, Building 5, Room 126, 9000 Rockville Pike, Bethesda, MD 20892-0520, USA.

出版信息

J Biomol NMR. 2013 Apr;55(4):369-77. doi: 10.1007/s10858-013-9720-3. Epub 2013 Mar 19.

Abstract

We demonstrate that alignment of a structured peptide or small protein solubilized in mixed phospholipid:detergent micelles or bicelles, when embedded in a compressed gel or liquid crystalline medium, can be altered by either changing the phospholipid aggregate shape, charge, or both together. For the hemagglutinin fusion peptide solubilized in bicelles, we show that bicelle shape and charge do not change its helical hairpin structure but impact its alignment relative to the alignment medium, both in charged compressed acrylamide gel and in liquid crystalline d(GpG). The method can be used to generate sets of residual dipolar couplings that correspond to orthogonal alignment tensors, and holds promise for high-resolution structural refinement and dynamic mapping of membrane proteins.

摘要

我们证明了在压缩凝胶或液晶介质中,当溶解在混合磷脂:去污剂胶束或双胶束中的结构化肽或小蛋白被嵌入时,通过改变磷脂聚集体的形状、电荷或两者同时改变,可以改变其对齐方式。对于溶解在双胶束中的血凝素融合肽,我们表明双胶束的形状和电荷不会改变其螺旋发夹结构,但会影响其相对于对齐介质的排列方式,无论是在带电荷的压缩丙烯酰胺凝胶中还是在液晶 d(GpG)中。该方法可用于生成对应于正交排列张量的残差偶极耦合集,有望实现膜蛋白的高分辨率结构精修和动态映射。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e9aa/3636151/fd9f024d60fc/nihms449671f1.jpg

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