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通过顺磁弛豫增强对胶束结合肽进行定位

Positioning of micelle-bound peptides by paramagnetic relaxation enhancements.

作者信息

Zangger Klaus, Respondek Michal, Göbl Christoph, Hohlweg Walter, Rasmussen Kenneth, Grampp Günter, Madl Tobias

机构信息

Institute of Chemistry/Organic and Bioorganic Chemistry, University of Graz, Austria.

出版信息

J Phys Chem B. 2009 Apr 2;113(13):4400-6. doi: 10.1021/jp808501x.

Abstract

Many peptides, proteins, and drugs interact with biological membranes, and knowing the mode of binding is essential to understanding their biological functions. To obtain the complete orientation and immersion depth of such a compound, the membrane-mimetic system (micelle) is placed in an aqueous buffer containing the soluble and inert paramagnetic contrast agent Gd(DTPA-BMA). Paramagnetic relaxation enhancements (PREs) of a specific nucleus then depend only on its distance from the surface. The positioning of a structurally characterized compound can be obtained by least-squares fitting of experimental PREs to the micelle center position. This liquid-state NMR approach, which does not rely on isotopic labeling or chemical modification, has been applied to determine the location of the presumed transmembrane region 7 of yeast V-ATPase (TM7) and the membrane-bound antimicrobial peptide CM15 in micelles. TM7 binds in a trans-micelle orientation with the N-terminus being slightly closer to the surface than the C-terminus. CM15 is immersed unexpectedly deep into the micelle with the more hydrophilic side of the helix being closer to the surface than the hydrophobic one.

摘要

许多肽、蛋白质和药物会与生物膜相互作用,了解其结合模式对于理解它们的生物功能至关重要。为了获得此类化合物的完整取向和浸入深度,将膜模拟系统(胶束)置于含有可溶性惰性顺磁性造影剂钆(DTPA - BMA)的水性缓冲液中。然后,特定原子核的顺磁弛豫增强(PREs)仅取决于其与表面的距离。通过将实验测得的PREs与胶束中心位置进行最小二乘法拟合,可获得结构特征明确的化合物的定位。这种不依赖同位素标记或化学修饰的液态核磁共振方法,已被用于确定酵母V - ATP酶假定的跨膜区域7(TM7)以及胶束中膜结合抗菌肽CM15的位置。TM7以跨胶束取向结合,其N端比C端略靠近表面。CM15意外地深入浸入胶束中,螺旋的亲水性一侧比疏水性一侧更靠近表面。

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