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多层囊泡融合快速形成低缺陷密度束缚双层。

Fast formation of low-defect-density tethered bilayers by fusion of multilamellar vesicles.

机构信息

Institute of Biochemistry, Vilnius University, Sauletekio 7, Vilnius LT-10257 , Lithuania.

Institute for Bioscience and Biotechnology Research, Rockville, MD 20850, USA.

出版信息

Biochim Biophys Acta Biomembr. 2017 May;1859(5):669-678. doi: 10.1016/j.bbamem.2017.01.015. Epub 2017 Jan 12.

DOI:10.1016/j.bbamem.2017.01.015
PMID:28088448
Abstract

A facile and reproducible preparation of surface-supported lipid bilayers is essential for fundamental membrane research and biotechnological applications. We demonstrate that multilamellar vesicles fuse to molecular-anchor-grafted surfaces yielding low-defect-density, tethered bilayer membranes. Continuous bilayers are formed within 10min, while the electrically insulating bilayers with <0.1μm defect density can be accomplished within 60min. Surface plasmon resonance spectroscopy indicates that an amount of lipid material transferred from vesicles to a surface is inversely proportional to the density of an anchor, while the total amount of lipid that includes tethered and transferred lipid remains constant within 5% standard error. This attests for the formation of intact bilayers independent of the tethering agent density. Neutron reflectometry (NR) revealed the atomic level structural details of the tethered bilayer showing, among other things, that the total thickness of the hydrophobic slab of the construct was 3.2nm and that the molar fraction of cholesterol in lipid content is essentially the same as the molar fraction of cholesterol in the multilamellar liposomes. NR also indicated the formation of an overlayer with an effective thickness of 1.9nm. These overlayers may be easily removed by a single rinse of the tethered construct with 30% ethanol solution. Fast assembly and low residual defect density achievable within an hour of fusion makes our tethered bilayer methodology an attractive platform for biosensing of membrane damaging agents, such as pore forming toxins.

摘要

一种简单且可重现的制备表面支撑脂质双层的方法对于基础膜研究和生物技术应用至关重要。我们证明多分子层囊泡融合到分子锚定接枝表面上,得到低缺陷密度的固定双层膜。在 10 分钟内形成连续双层,而缺陷密度<0.1μm 的电绝缘双层可以在 60 分钟内完成。表面等离子体共振光谱表明,从囊泡转移到表面的脂质材料量与锚定密度成反比,而包括固定和转移脂质在内的总脂质量在 5%标准误差内保持不变。这证明了完整双层的形成独立于固定剂密度。中子反射测量(NR)揭示了固定双层的原子级结构细节,除其他外,表明构建体的疏水区块的总厚度为 3.2nm,并且脂质中胆固醇的摩尔分数与多层脂质体中胆固醇的摩尔分数基本相同。NR 还表明形成了具有 1.9nm 有效厚度的覆盖层。这些覆盖层可以通过用 30%乙醇溶液对固定构造物进行单次冲洗轻易去除。融合后一小时内可实现快速组装和低残余缺陷密度,使得我们的固定双层方法成为用于检测膜损伤剂(如孔形成毒素)的有吸引力的生物传感器平台。

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