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自组装 tethered 双分子脂质膜

Self-assembled tethered bimolecular lipid membranes.

作者信息

Sinner Eva-Kathrin, Ritz Sandra, Naumann Renate, Schiller Stefan, Knoll Wolfgang

机构信息

Max Planck Institute for Polymer Research, Mainz, Germany.

出版信息

Adv Clin Chem. 2009;49:159-79. doi: 10.1016/s0065-2423(09)49007-3.

Abstract

This chapter describes some of the strategies developed in our group for designing, constructing and structurally and functionally characterizing tethered bimolecular lipid membranes (tBLM). We introduce this platform as a novel model membrane system that complements the existing ones, for example, Langmuir monolayers, vesicular liposomal dispersions and bimolecular ("black") lipid membranes. Moreover, it offers the additional advantage of allowing for studies of the influence of membrane structure and order on the function of integral proteins, for example, on how the composition and organization of lipids in a mixed membrane influence the ion translocation activity of integral channel proteins. The first strategy that we introduce concerns the preparation of tethered monolayers by the self-assembly of telechelics. Their molecular architecture with a headgroup, a spacer unit (the "tether") and the amphiphile that mimics the lipid molecule allows them to bind specifically to the solid support thus forming the proximal layer of the final architecture. After fusion of vesicles that could contain reconstituted proteins from a liposomal dispersion in contact to this monolayer the tethered bimolecular lipid membrane is obtained. This can then be characterized by a broad range of surface analytical techniques, including surface plasmon spectroscopies, the quartz crystal microbalance, fluorescence and IR spectroscopies, and electrochemical techniques, to mention a few. It is shown that this concept allows for the construction of tethered lipid bilayers with outstanding electrical properties including resistivities in excess of 10 MOmega cm2. A modified strategy uses the assembly of peptides as spacers that couple covalently via their engineered sulfhydryl or lipoic acid groups at the N-terminus to the employed gold substrate, while their C-terminus is being activated afterward for the coupling of, for example, dimyristoylphosphatidylethanol amine (DMPE) lipid molecules via the NH2 moiety of their headgroups. It is demonstrated that these membranes are well suited for the in situ synthesis of membrane protein by a cell-free expression approach. The vectorial integration of an in vitro synthesized odorant receptor, OR5 from the rat, is demonstrated by means of antibodies that specifically bind to a tag at the N-terminus of the receptor and is read out by surface plasmon fluorescence spectroscopy. A completely different strategy employs his-tagged membrane proteins in their solubilized form binding to a surface-attached Ni(+)-NTA monolayer generating a well-oriented protein layer the density of which can be easily controlled by online monitoring the binding (assembly) step by surface plasmon spectroscopy. Moreover, the attachment of the his-tag to either the C- or the N-terminus allows for the complete control of the protein orientation. After the exchange of the detergent micelle by a lipid bilayer via a surface dialysis procedure an electrically very well isolating protein-tethered membrane is formed. We show that this "wiring" of the functional units allows for the (external) manipulation of the oxidation state of the redox-protein cytochrome c Oxidase by the control of the potential applied to the gold substrate which is used as the working electrode in an electrochemical attachment.

摘要

本章介绍了我们团队开发的一些用于设计、构建以及对拴系双分子脂质膜(tBLM)进行结构和功能表征的策略。我们将这个平台作为一种新型的模型膜系统来介绍,它可以补充现有的膜系统,例如朗缪尔单层膜、囊泡脂质体分散体系和双分子(“黑色”)脂质膜。此外,它还具有额外的优势,即能够研究膜结构和有序性对整合蛋白功能的影响,例如混合膜中脂质的组成和组织方式如何影响整合通道蛋白的离子转运活性。我们介绍的第一个策略涉及通过远螯聚合物的自组装制备拴系单层膜。它们具有头基、间隔单元(“拴系”)和模拟脂质分子的两亲分子的分子结构,这使得它们能够特异性地结合到固体支持物上,从而形成最终结构的近端层。在与该单层膜接触的脂质体分散体系中含有重组蛋白的囊泡融合后,即可获得拴系双分子脂质膜。然后,可以通过多种表面分析技术对其进行表征,包括表面等离子体光谱、石英晶体微天平、荧光和红外光谱以及电化学技术等等。结果表明,这个概念能够构建出具有出色电学性质的拴系脂质双层膜,其电阻率超过10 MΩ·cm²。一种改进的策略是使用肽作为间隔物进行组装,这些肽通过其在N端工程化的巯基或硫辛酸基团与所用的金基底共价偶联,随后其C端被激活,以便通过其头基的NH₂部分偶联例如二肉豆蔻酰磷脂酰乙醇胺(DMPE)脂质分子。结果表明,这些膜非常适合通过无细胞表达方法原位合成膜蛋白。通过特异性结合受体N端标签的抗体证明了体外合成的大鼠气味受体OR5的矢量整合,并通过表面等离子体荧光光谱进行读出。一种完全不同的策略是使用以可溶形式存在的带有组氨酸标签的膜蛋白,使其与表面附着的Ni(⁺)-NTA单层结合,从而生成一个取向良好的蛋白层,其密度可以通过表面等离子体光谱在线监测结合(组装)步骤轻松控制。此外,将组氨酸标签连接到C端或N端可以完全控制蛋白的取向。通过表面透析程序用脂质双层替换去污剂胶束后,形成了电学上非常绝缘的蛋白拴系膜。我们表明,这种功能单元的“连接”允许通过控制施加到用作电化学附着工作电极的金基底上的电位来(外部)操纵氧化还原蛋白细胞色素c氧化酶的氧化态。

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