K. Shimura, Takuma Waki, Masaki Okada, T. Toda, Izumi Kimoto, K. Kasai
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A dual buffer system, 60 mM borate-Na (pH 9.35) as an electrophoresis buffer and 60 mM 3-morpholinopropanesulfonic acid-Na (pH 7.35) containing 0.1% Tween 20 as a sample buffer, was employed to allow the interactions to occur at a physiological pH and also to maintain a high level of electroosmosis and reproducibility in the bare silica capillaries. The electrophoresis of the fluorophore-labeled proteins was carried out in the presence of affinophores, and changes in the mobility of the labeled proteins were analyzed in terms of the mobility moment, which represents the average mobility of the proteins, thus permitting the dissociation constants for the protein-affinophore interactions to be determined. The affinophoresis system was then used to evaluate the extent of binding of low molecular mass compounds based on the inhibition of the affinophoresis. In combination with the mobility moment analysis and the dual buffer system, the multi-capillary electrophoresis instruments proved to be useful for the analysis of biomolecular interactions by electrophoresis.","PeriodicalId":15059,"journal":{"name":"Journal of capillary electrophoresis","volume":"13 1","pages":"53-60"},"PeriodicalIF":0.0000,"publicationDate":"2005-06-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":"{\"title\":\"Mobility-moment analysis of protein-ligand interactions using a multi-capillary electrophoresis instrument : Competitive affinophoresis of concanavalin A and trypsin\",\"authors\":\"K. Shimura, Takuma Waki, Masaki Okada, T. Toda, Izumi Kimoto, K. 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引用次数: 0
摘要
以豆豆蛋白a和胰蛋白酶为模型,对配备激光诱导荧光检测器的全自动96毛细管电泳仪在亲和电泳分析中的实用性进行了评价。将亲和配体对氨基苯基甘露苷和对氨基苯并脒分别与可溶性琥珀基聚赖氨酸偶联,以1/5的羧基密度制备了刀豆蛋白A和胰蛋白酶的亲和载体。采用双缓冲系统,60 mM硼酸钠(pH 9.35)作为电泳缓冲液,60 mM 3- morpholinopropanesonic - na (pH 7.35)含0.1% Tween 20作为样品缓冲液,使相互作用在生理pH下发生,并保持高水平的电渗透和裸二氧化硅毛细血管的再现性。在亲和团存在的情况下对荧光团标记的蛋白质进行电泳,并根据代表蛋白质平均迁移率的迁移矩分析标记蛋白质迁移率的变化,从而确定蛋白质-亲和团相互作用的解离常数。然后使用亲和性电泳系统来评估基于亲和性电泳抑制的低分子质量化合物的结合程度。与迁移矩分析和双缓冲系统相结合,证明了多毛细管电泳仪在电泳分析生物分子相互作用方面的作用。
Mobility-moment analysis of protein-ligand interactions using a multi-capillary electrophoresis instrument : Competitive affinophoresis of concanavalin A and trypsin
The utility of an automated 96-capillary electrophoresis instrument equipped with a laser-induced fluorescence detector was evaluated in the analysis of affinophoresis using concanavalin A and trypsin as models. Affinophores for concanavalin A and trypsin were prepared by coupling the affinity ligands, p-aminophenylmannoside and p-aminobenzamidine to soluble succinylpolylysine, respectively at a density of about 1/5 of the carboxyl groups. A dual buffer system, 60 mM borate-Na (pH 9.35) as an electrophoresis buffer and 60 mM 3-morpholinopropanesulfonic acid-Na (pH 7.35) containing 0.1% Tween 20 as a sample buffer, was employed to allow the interactions to occur at a physiological pH and also to maintain a high level of electroosmosis and reproducibility in the bare silica capillaries. The electrophoresis of the fluorophore-labeled proteins was carried out in the presence of affinophores, and changes in the mobility of the labeled proteins were analyzed in terms of the mobility moment, which represents the average mobility of the proteins, thus permitting the dissociation constants for the protein-affinophore interactions to be determined. The affinophoresis system was then used to evaluate the extent of binding of low molecular mass compounds based on the inhibition of the affinophoresis. In combination with the mobility moment analysis and the dual buffer system, the multi-capillary electrophoresis instruments proved to be useful for the analysis of biomolecular interactions by electrophoresis.