Hutchens T W, Yip T T, Porath J
Institute of Biochemistry, University of Uppsala, Sweden.
Anal Biochem. 1988 Apr;170(1):168-82. doi: 10.1016/0003-2697(88)90105-4.
Quantitative or analytical affinity chromatography has been successful primarily for the analysis of biologically determined macromolecular affinity relationships. Quantitative approaches are also needed to better characterize simpler, chemically defined immobilized ligands with potential for selective interaction with specific, predetermined protein surface groups. Protein interaction with immobilized metal is a rather selective and versatile, high-affinity adsorption technique for which there is little quantitative information. Using model protein interactions with immobilized Cu2+ ions, we have compared analytical frontal affinity chromatographic methods to a simple, nonchromatographic protocol for the rapid determination of quantitative affinity relationships. Values obtained for the equilibrium dissociation constant (Kd) and binding capacity (Lt) characterizing the interaction of lysozyme with immobilized Cu2+ were quite similar by frontal analysis (Kd = 37-42 X 10(-6) M; Lt = 6.8-7.4 X 10(-6) mol protein/ml gel) and by equilibrium binding analyses (Kd = 33 +/- 4.7 X 10(-6) M; Lt = 5.8-6.1 X 10(-6) mol protein/ml gel; 14 determinations). The interaction of ovalbumin with immobilized Cu2+ was characterized by an affinity (Kd = 4.2-4.8 X 10(-6) M) and capacity (Lt = 1.5-2.1 X 10(-6) mol protein/ml gel) which were also the same regardless of the method for affinity analysis. These values indicate that the total protein bound at saturation corresponds to as much as 17% of the total immobilized Cu2+ ions (approximately 40 X 10(-6) mol/ml gel). Thus, depending on the fraction of total immobilized Cu2+ available for interaction with a given protein (e.g., lysozyme), the number of individual immobilized ligands actively participating as well as those rendered unavailable upon individual protein binding events may be greater than 1. Linear Scatchard plots obtained for both lysozyme and ovalbumin (purified) suggest the presence of only a single type of immobilized Cu2+-protein interaction operative under the experimental conditions employed. However, Scatchard analyses of data obtained by the nonchromatographic equilibrium binding method also demonstrated the ability to simultaneously resolve the contribution of two components whose presence was predicted by frontal chromatography. Our results support the validity and utility of equilibrium binding data analyzed according to the equations outlined by Scatchard and others as an alternative to analytical chromatographic methods.
定量或分析亲和色谱主要成功用于分析生物测定的大分子亲和关系。还需要定量方法来更好地表征更简单的、化学定义的固定化配体,这些配体有可能与特定的、预先确定的蛋白质表面基团发生选择性相互作用。蛋白质与固定化金属的相互作用是一种相当选择性和通用的高亲和力吸附技术,关于它的定量信息很少。利用模型蛋白与固定化Cu2+离子的相互作用,我们将分析前沿亲和色谱方法与一种简单的非色谱方法进行了比较,以快速确定定量亲和关系。通过前沿分析(Kd = 37 - 42×10(-6) M;Lt = 6.8 - 7.4×10(-6) mol蛋白/ml凝胶)和平衡结合分析(Kd = 33 ± 4.7×10(-6) M;Lt = 5.8 - 6.1×10(-6) mol蛋白/ml凝胶;14次测定)得到的表征溶菌酶与固定化Cu2+相互作用的平衡解离常数(Kd)和结合容量(Lt)值非常相似。卵清蛋白与固定化Cu2+的相互作用的特征在于亲和力(Kd = 4.2 - 4.8×10(-6) M)和容量(Lt = 1.5 - 2.1×10(-6) mol蛋白/ml凝胶),无论亲和分析方法如何,这些值也是相同的。这些值表明,饱和时结合的总蛋白相当于固定化Cu2+离子总量的17%(约40×10(-6) mol/ml凝胶)。因此,取决于可用于与给定蛋白质(如溶菌酶)相互作用的固定化Cu2+总量的比例,积极参与的单个固定化配体的数量以及在单个蛋白质结合事件后变得不可用的数量可能大于1。溶菌酶和卵清蛋白(纯化的)得到的线性Scatchard图表明,在所采用的实验条件下,仅存在一种类型的固定化Cu2+-蛋白质相互作用。然而,通过非色谱平衡结合方法获得的数据的Scatchard分析也证明了能够同时解析前沿色谱预测存在的两种成分的贡献。我们的结果支持根据Scatchard等人概述的方程分析的平衡结合数据作为分析色谱方法的替代方法的有效性和实用性。
