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Construction of tethered bilayer lipid membrane with oriented membrane proteins on surface modified mica substrate

机译:表面改性云母基质取向膜蛋白的旋翼双层脂质膜的构建

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Incorporating membrane proteins, which are major targets of drug discovery, into artificial planar lipid bilayer membranes is important. From the observation at the high spatiotemporal resolution in the microscopic region, the intermolecular interactions between lipids and membrane proteins can be revealed. It leads to elucidation of the reaction mechanisms occurring in biological membranes. However, when a lipid membrane supported on a solid substrate (SLB) is used, the following points are interfering with the research. The first point is the structural change due to the contact between the membrane protein and the underlying substrate. The other is disorder of the membrane protein orientation in the SLB. Research on the incorporation of membrane proteins has been done in the field of both physical and biological chemistry, but few reports have achieved detailed measurements with placing emphasis on the plasticity and diversity of membrane proteins. In this study, the tethered bilayer lipid membrane (tBLM) was formed on the atomically flat self-assembled monolayer modified surface which specifically binds to the membrane proteins in the membrane. The fluidity of artificial lipid bilayer and orientation of membrane proteins are observed by the epi-fluorescence microscopy and atomic force microscopy, respectively. The consequent decreased interaction between the substrate and lipid membrane and limited observation for the specific orientation of membrane proteins suggest that it was possible to reproduce the same environment as the biological membrane even in the artificial lipid bilayer membrane. The present tBLM system should be useful for the creation of basic technologies for structural, functional, and dynamical analysis of membrane proteins. It also leads to the understanding the molecular structure of biological membrane which include the various membrane proteins such as ion channels, transporters, pumps and enzymes with addition of more complex structural properties such as the underlying membrane scaffolds, asymmetric lipid composition and domains. (C) 2019 The Japan Society of Applied Physics
机译:掺入膜蛋白质,这些蛋白质是药物发现的主要目标,成为人造平面脂质双层膜很重要。从微观区域中的高时分辨率观察,可以揭示脂质和膜蛋白之间的分子间相互作用。它导致阐明生物膜中发生的反应机制。然而,当使用支撑在固体基质(SLB)上的脂质膜时,以下几点在干扰研究时。第一点是由于膜蛋白和下面基底之间的接触导致的结构变化。另一个是SLB中膜蛋白取向的紊乱。对膜蛋白掺入的研究已经在物理和生物学化学的领域中进行,但是少数报道已经达到了详细的测量,并强调膜蛋白的可塑性和多样性。在该研究中,在原子平自组装的单层改性表面上形成束缚双层脂质膜(TBLM),其特异性结合膜中的膜蛋白。通过外荧光显微镜和原子力显微镜观察人工脂双层和膜蛋白的取向的流动性。因此,基材和脂质膜之间的相互作用和对膜蛋白的比取向的有限观察表明,即使在人工脂质双层膜中也可以再现与生物膜的相同环境。目前的TBLM系统应该有助于创建膜蛋白的结构,功能和动态分析的基本技术。它还导致理解生物膜的分子结构,其包括各种膜蛋白,例如离子通道,转运蛋白,泵和酶,这些膜,包括更复杂的结构性质,例如下面的膜支架,不对称的脂质组合物和结构域。 (c)2019年日本应用物理学会

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  • 来源
    《Japanese journal of applied physics》 |2019年第2019期|SIIB12.1-SIIB12.5|共5页
  • 作者单位

    Gunma Univ Fac Sci & Technol Kiryu Gunma 3768515 Japan|Gunma Univ Ctr Food Sci & Wellness Maebashi Gunma 3718510 Japan;

    Gunma Univ Fac Sci & Technol Kiryu Gunma 3768515 Japan;

    Gunma Univ Ctr Instrumental Anal Kiryu Gunma 3768515 Japan;

    Gunma Univ Ctr Instrumental Anal Kiryu Gunma 3768515 Japan;

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