首页> 外文会议>Annual Northeast Bioengineering Conference >Incorporation and Characterization of Alpha-Helical Peptide-Based Anchors into Bead-Supported Lipid Bilayer Membranes
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Incorporation and Characterization of Alpha-Helical Peptide-Based Anchors into Bead-Supported Lipid Bilayer Membranes

机译:将α-螺旋肽基锚的掺入和表征到珠子负载的脂质双层膜中

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Our aim is to design alpha-helical peptide complexes to enhance their stability and biological feasibility for the study of membrane proteins and their interactions. In on-going work, we employ (K3A4L2A7L2A3K3) as anchoring molecules, where conjugation of the peptide with fluoresceine isothiocyanate (FITC) allows one to access a variety of chemistries (such as introducing fluorescent dye, etc.) for orthogonal modification [1]. These peptides partition within NHS-PEG3000-NHS which function as in vitro models for interactions with the membrane, will be incorporated into mimic lipid bilayer membranes (such as DOPC) supported by microbeads. We could control the receptor site densities on lipobeads by varying the mole fraction of different lipids and ligands. Moreover, the secondary structure of peptide within these micelles is characterized with circular dichroism. Lateral fluidity of the fluorescently tagged peptide is analyzed via fluorescence imaging microscopy (Confocal Microscopy) and quantified using fluorescence recovery after photobleaching (FRAP) techniques. Variations in the peptide sequence allow us to rationally investigate the influence of sequence on peptide anchor stability.
机译:我们的目的是设计α-螺旋肽复合物,以提高膜蛋白及其相互作用研究的稳定性和生物可行性。在进行工作中,我们使用(K3A4L2A7L2A3K3)作为锚定分子,其中肽与荧光素异硫氰酸酯(FITC)的缀合物允许人们访问各种化学物质(例如引入荧光染料等)进行正交改性[1] 。这些肽分配在NHS-PEG3000-NH中的分配,其用作与膜相互作用的体外模型,将掺入Microbead的模拟脂质双层膜(如DOPC)中。通过改变不同脂质和配体的摩尔分数,我们可以控制Lipobeads上的受体位点密度。此外,这些胶束内的肽的二级结构具有圆形二色性的特征。通过荧光成像显微镜(共聚焦显微镜)分析荧光标记肽的侧向流动性,并在光漂白(FRAP)技术之后使用荧光回收定量。肽序列的变化使我们能够理由地研究序列对肽锚定稳定性的影响。

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