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糖纳米材料与凝集素结合亲和力的定量分析。

Quantification of binding affinity of glyconanomaterials with lectins.

机构信息

Department of Chemistry, University of Massachusetts Lowell, 1 University Ave., Lowell, Massachusetts 01854, USA.

出版信息

Chem Commun (Camb). 2020 Nov 14;56(88):13491-13505. doi: 10.1039/d0cc05899h. Epub 2020 Oct 15.

Abstract

Carbohydrate-mediated interactions are involved in many cellular activities including immune responses and infections. These interactions are relatively weak, and as such, cells employ multivalency, i.e., the presentation of multiple monovalent carbohydrate ligands within a close proximity, for cooperative binding thus drastically enhanced binding affinity. In the past two decades, the field of glyconanomaterials has emerged where nanomaterials are used as multivalent scaffolds to present multiple copies of carbohydrate ligands on the nanomaterial surface. At the core of glyconanomaterial research is the ability to control and modulate multivalency through ligand display. For the quantitative evaluation of multivalency, the binding affinity must be determined. Quantification of the binding parameters provides insights for not only the fundamental glyconanomaterial-lectin interactions, but also the rational design of effective diagnostics and therapeutics. Several methods have been developed to determine the binding affinity of glyconanomaterials with lectins, including fluorescence competitive assays in solution or on microarrays, Förster resonance energy transfer, fluorescence quenching, isothermal titration calorimetry, surface plasmon resonance spectroscopy, quartz crystal microbalance and dynamic light scattering. This Feature Article discusses each of these techniques, as well as how each technique is applied to determine the binding affinity of glyconanomaterials with lectins, and the data analysis. Although the results differed depending on the specific method used, collectively, they showed that nanomaterials as multivalent scaffolds could amplify the binding affinity of carbohydrate-lectin interactions by several orders of magnitude, the extent of which depending on the structure of the carbohydrate ligand, the ligand density, the linker length and the particle size.

摘要

碳水化合物介导的相互作用参与许多细胞活动,包括免疫反应和感染。这些相互作用相对较弱,因此,细胞采用多价性,即在近距离内呈现多个单价碳水化合物配体,以进行协同结合,从而大大增强结合亲和力。在过去的二十年中,糖纳米材料领域已经出现,其中纳米材料被用作多价支架,在纳米材料表面呈现多个碳水化合物配体的副本。糖纳米材料研究的核心是通过配体展示来控制和调节多价性的能力。为了定量评估多价性,必须确定结合亲和力。结合参数的量化不仅为基础的糖纳米材料-凝集素相互作用提供了深入了解,而且为有效诊断和治疗的合理设计提供了依据。已经开发了几种方法来确定糖纳米材料与凝集素的结合亲和力,包括溶液或微阵列中的荧光竞争测定、Förster 共振能量转移、荧光猝灭、等温滴定量热法、表面等离子体共振光谱法、石英晶体微天平法和动态光散射法。这篇专题文章讨论了这些技术中的每一种,以及每种技术如何应用于确定糖纳米材料与凝集素的结合亲和力以及数据分析。尽管结果因所用特定方法而异,但总体而言,它们表明纳米材料作为多价支架可以将碳水化合物-凝集素相互作用的结合亲和力放大几个数量级,其程度取决于碳水化合物配体的结构、配体密度、连接体长度和粒径。

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