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Affinity biosensors using recombinant native membrane proteins displayed on exosomes: application to botulinum neurotoxin B receptor

机译:使用在外泌体上展示的重组天然膜蛋白的亲和力生物传感器:应用于肉毒杆菌神经毒素B受体

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摘要

The development of simple molecular assays with membrane protein receptors in a native conformation still represents a challenging task. Exosomes are extracellular vesicles which, due to their stability and small size, are suited for analysis in various assay formats. Here, we describe a novel approach to sort recombinant fully native and functional membrane proteins to exosomes using a targeting peptide. Specific binding of high affinity ligands to the potassium channel Kv1.2, the G-protein coupled receptor CXCR4, and the botulinum neurotoxin type B (BoNT/B) receptor, indicated their correct assembly and outside out orientation in exosomes. We then developed, using a label-free optical biosensor, a new method to determine the kinetic constants of BoNT/B holotoxin binding to its receptor synaptotagmin2/GT1b ganglioside (kon = 2.3 ×105 M−1.s−1, koff = 1.3 10−4 s−1), yielding an affinity constant (KD = 0.6 nM) similar to values determined from native tissue. In addition, the recombinant binding domain of BoNT/B, a potential vector for neuronal delivery, bound quasi-irreversibly to synaptotagmin 2/GT1b exosomes. Engineered exosomes provide thus a novel means to study membrane proteins for biotechnology and clinical applications.
机译:用天然构象的膜蛋白受体进行简单的分子测定仍是一项艰巨的任务。外来体是细胞外囊泡,由于其稳定性和小尺寸,适合用于各种测定形式的分析。在这里,我们描述了一种新颖的方法,可以使用靶向肽将重组的完全天然和功能性膜蛋白分选到外来体。高亲和力配体与钾通道Kv1.2,G蛋白偶联受体CXCR4和肉毒杆菌B型神经毒素(BoNT / B)受体的特异性结合表明它们在外泌体中的正确组装和外向定向。然后,我们使用无标记的光学生物传感器开发了一种新方法,用于确定BoNT / B全毒素与其受体突触标签素2 / GT1b神经节苷脂结合的动力学常数(kon = 2.3×10 5 M −1 .s -1 ,koff = 1.3 10 −4 s -1 ),产生亲和常数(KD = 0.6 nM)类似于从天然组织确定的值。此外,BoNT / B的重组结合域,一种潜在的神经元传递载体,与突触标签蛋白2 / GT1b外泌体准不可逆地结合。因此,工程外泌体提供了一种新颖的方法来研究膜蛋白,以用于生物技术和临床应用。

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