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Single Gold Nanoparticle Localized Surface Plasmon Resonance Spectral Imaging for Quantifying Binding Constant of Carbohydrate-Protein Interaction

机译:单金纳米粒子局部表面等离子共振光谱成像定量的碳水化合物-蛋白质相互作用的结合常数。

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Quantifying carbohydrate-protein (ligand-receptor) interactions is important to understand diverse biological processes and to develop new diagnostic and therapeutic methods. We develop an approach to quantitatively study carbohydrate-protein interactions by Au nanoparticle localized surface plasmon resonance (LSPR) peak position shift at the single particles level. Unlike the previous techniques for single particle LSPR spectral imaging, only the first-order streak of an individual nanoparticle is needed to extract a LSPR spectrum, which has great potential to increase throughput to 500 single particle spectra in each frame. LSPR peak shift of protein modified single Au nanoparticles is found to be a function of its ligand concentration, which can be used to fit the binding constants of the interactions. The moderate interactions of Antithrombin III (AT III) and heparins including low molecular weight heparin (LMWH) are determined as well as the strong interaction of transferrin and antitransferrin and the weak interaction of bovine serum album (BSA) and heparin. The measured binding constants of transferrin to antitransferrin, heparin and LMWH to AT III, and BSA to heparin are (3.0 ± 0.6) × 10~9 M~(-1), (3.1 ± 0.3) × 10~6 M~(-1), (8.0 ± 0.5) × 10~5 M~(-1), and (5.1 ± 0.1) × 10~3 M~(-1), respectively, which are in good agreement with the reported values.
机译:量化碳水化合物-蛋白质(配体-受体)的相互作用对于理解多种生物过程以及开发新的诊断和治疗方法非常重要。我们开发一种方法来定量研究金-纳米粒子局部表面等离振子共振(LSPR)峰值位置位移在单个粒子水平上的碳水化合物-蛋白质相互作用。与以前的单粒子LSPR光谱成像技术不同,只需要单个纳米粒子的一阶条纹即可提取LSPR光谱,这具有极大的潜力将每帧中的通量提高到500个单粒子光谱。发现蛋白修饰的单个Au纳米粒子的LSPR峰位移是其配体浓度的函数,可用于拟合相互作用的结合常数。确定了抗凝血酶III(AT III)和肝素(包括低分子量肝素(LMWH))的适度相互作用,以及运铁蛋白和抗运铁蛋白的强相互作用以及牛血清蛋白(BSA)和肝素的弱相互作用。测得的运铁蛋白与抗运铁蛋白,肝素和LMWH与AT III的结合常数以及BSA与肝素的结合常数为(3.0±0.6)×10〜9 M〜(-1),(3.1±0.3)×10〜6 M〜(- 1),(8.0±0.5)×10〜5 M〜(-1)和(5.1±0.1)×10〜3 M〜(-1),与报告值非常吻合。

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