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本文引用的文献

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Surface plasmon resonance study of protein-carbohydrate interactions using biotinylated sialosides.使用生物素化唾液酸苷对蛋白质-碳水化合物相互作用进行表面等离子体共振研究。
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Unnatural amino acid incorporation into virus-like particles.非天然氨基酸掺入病毒样颗粒。
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Free-solution, label-free molecular interactions studied by back-scattering interferometry.通过背散射干涉测量法研究的无标记分子在自由溶液中的相互作用。
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Anti-carbohydrate antibodies elicited by polyvalent display on a viral scaffold.多价展示在病毒支架上诱导的抗碳水化合物抗体。
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Nonlabeled quartz crystal microbalance biosensor for bacterial detection using carbohydrate and lectin recognitions.用于细菌检测的非标记石英晶体微天平生物传感器,采用碳水化合物和凝集素识别技术。
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7
SPR studies of carbohydrate-lectin interactions as useful tool for screening on lectin sources.表面等离子体共振(SPR)技术用于研究碳水化合物与凝集素的相互作用,是筛选凝集素来源的有效工具。
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8
Lectins: carbohydrate-specific reagents and biological recognition molecules.凝集素:碳水化合物特异性试剂及生物识别分子。
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Carbohydrate-functionalized dendrimers to investigate the predictable tunability of multivalent interactions.用于研究多价相互作用可预测可调性的碳水化合物功能化树枝状大分子。
Bioconjug Chem. 2006 Jul-Aug;17(4):958-66. doi: 10.1021/bc060107x.
10
Carbohydrate-protein interactions by "clicked" carbohydrate self-assembled monolayers.通过“点击”碳水化合物自组装单分子层实现的碳水化合物-蛋白质相互作用
Anal Chem. 2006 Mar 15;78(6):2001-8. doi: 10.1021/ac051919+.

通过背散射干涉测量法测定单价和多价碳水化合物-凝集素结合。

Measurement of monovalent and polyvalent carbohydrate-lectin binding by back-scattering interferometry.

作者信息

Kussrow Amanda, Kaltgrad Eiton, Wolfenden Mark L, Cloninger Mary J, Finn M G, Bornhop Darryl J

机构信息

Department of Chemistry and Vanderbilt Institute of Chemical Biology, Vanderbilt University, 4226 Stevenson Center, Nashville, Tennessee 37235, USA.

出版信息

Anal Chem. 2009 Jun 15;81(12):4889-97. doi: 10.1021/ac900569c.

DOI:10.1021/ac900569c
PMID:19462965
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2713007/
Abstract

Carbohydrate-protein binding is important to many areas of biochemistry. Here, backscattering interferometry (BSI) has been shown to be a convenient and sensitive method for obtaining quantitative information about the strengths and selectivities of such interactions. The surfaces of glass microfluidic channels were covalently modified with extravidin, to which biotinylated lectins were subsequently attached by incubation and washing. The binding of unmodified carbohydrates to the resulting avidin-immobilized lectins was monitored by BSI. Dose-response curves that were generated within several minutes and were highly reproducible in multiple wash/measure cycles provided adsorption coefficients that showed mannose to bind to concanavalin A (conA) with 3.7 times greater affinity than glucose consistent with literature values. Galactose was observed to bind selectively and with similar affinity to the lectin BS-1. The avidities of polyvalent sugar-coated virus particles for immobilized conA were much higher than monovalent glycans, with increases of 60-200 fold per glycan when arrayed on the exterior surface of cowpea mosaic virus or bacteriophage Qbeta. Sugar-functionalized PAMAM dendrimers showed size-dependent adsorption, which was consistent with the expected density of lectins on the surface. The sensitivity of BSI matches or exceeds that of surface plasmon resonance and quartz crystal microbalance techniques, and is sensitive to the number of binding events, rather than changes in mass. The operational simplicity and generality of BSI, along with the near-native conditions under which the target binding proteins are immobilized, make BSI an attractive method for the quantitative characterization of the binding functions of lectins and other proteins.

摘要

碳水化合物 - 蛋白质结合在生物化学的许多领域都很重要。在此,背散射干涉测量法(BSI)已被证明是一种便捷且灵敏的方法,可用于获取有关此类相互作用的强度和选择性的定量信息。玻璃微流控通道表面用抗生物素蛋白进行共价修饰,随后通过孵育和洗涤将生物素化的凝集素附着其上。通过BSI监测未修饰的碳水化合物与所得固定化抗生物素蛋白的凝集素的结合。在几分钟内生成且在多个洗涤/测量循环中具有高度可重复性的剂量 - 反应曲线提供了吸附系数,结果表明甘露糖与伴刀豆球蛋白A(conA)结合的亲和力比葡萄糖高3.7倍,这与文献值一致。观察到半乳糖与凝集素BS - 1有选择性结合且亲和力相似。多价糖包被的病毒颗粒对固定化conA的亲和力远高于单价聚糖,当排列在豇豆花叶病毒或噬菌体Qβ的外表面时,每个聚糖的亲和力增加60 - 200倍。糖功能化的聚酰胺 - 胺(PAMAM)树枝状大分子表现出尺寸依赖性吸附,这与表面凝集素的预期密度一致。BSI的灵敏度与表面等离子体共振和石英晶体微天平技术相当或更高,并且对结合事件的数量敏感,而非质量变化。BSI操作简单且具有通用性,以及目标结合蛋白固定化时接近天然的条件,使得BSI成为定量表征凝集素和其他蛋白质结合功能的有吸引力的方法。