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首页> 外文期刊>Journal of chromatography, A: Including electrophoresis and other separation methods >Determination of binding constants between one protein and multiple carbohydrates by affinity chromatography on a microchip
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Determination of binding constants between one protein and multiple carbohydrates by affinity chromatography on a microchip

机译:通过微芯片上的亲和色谱法测定一种蛋白质与多种碳水化合物之间的结合常数

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摘要

Development of rapid, reliable and high throughput methods for evaluating the interactions between different carbohydrates and a same protein is critical to carbohydrate drug development. In this study, we develop a novel strategy based on an affinity chromatography for quickly determining the binding constants of different carbohydrates to a same protein. The core of our method is the inversely proportional relationship between the binding constant and a new termed parameter, critical elution concentration (CMC). CMC is defined as the lowest concentration of displacing reagent, a series of carbohydrates herein, at which the protein specifically bond to the affinity column can be eluted off as an intact peak by the carbohydrate solution in a certain time. The interactions between a series of sulfate polysaccharides and granulocyte colony-stimulating factor (G-CSF) are selected as model. Through a 200. μm long heparin affinity column microfabricated inside a channel of 50. μm width and 20. μm height, the binding constant of each G-CSF-polysaccharide binding pair can be obtained within 1. h, around one sixth of time needed by traditional capillary electrophoresis based method.
机译:开发快速,可靠和高通量的方法以评估不同碳水化合物与同一蛋白质之间的相互作用对碳水化合物药物的开发至关重要。在这项研究中,我们开发了一种基于亲和色谱的新策略,可快速确定不同碳水化合物与同一蛋白质的结合常数。我们方法的核心是结合常数与新的参数临界洗脱浓度(CMC)之间的反比例关系。 CMC定义为置换试剂的最低浓度,即本文中的一系列碳水化合物,在一定时间内,与亲和柱特异性结合的蛋白质可以作为一个完整的峰洗脱出来。选择一系列硫酸盐多糖与粒细胞集落刺激因子(G-CSF)之间的相互作用作为模型。通过在50.μm宽度和20.μm高度的通道内微型制造的200.μm长的肝素亲和柱,可以在1小时内(大约所需时间的六分之一)获得每个G-CSF-多糖结合对的结合常数。通过传统的基于毛细管电泳的方法。

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