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基于新型琼脂糖的阴离子交换剂上蛋白质的梯度和等度高效液相色谱法

Gradient and isocratic high-performance liquid chromatography of proteins on a new agarose-based anion exchanger.

作者信息

Yao K, Hjertén S

出版信息

J Chromatogr. 1987 Jan 9;385:87-98. doi: 10.1016/s0021-9673(01)94624-2.

DOI:10.1016/s0021-9673(01)94624-2
PMID:3104376
Abstract

We describe a new, simple, and mild method for the preparation of anion-exchangers, based on the coupling of alkylamines to epoxy-activated agarose (prepared by the reaction of agarose with butanediol diglycidyl ether). Since a polar OH-group is formed when an epoxide reacts with an OH or NH2 group, the ion-exchanger did not show any hydrophobic interaction. This is important, since it may be impossible to desorb a protein from an ion exchanger having a hydrophobic character, because increasing the salt concentration of the eluent to decrease the electrostatic binding inevitably strengthens the hydrophobic interaction. By the method described, 3-diethylamino-2-hydroxy-propyl agarose (DEAHP-agarose) was prepared. High resolution of proteins was obtained by gradient elution at both high and low degrees of substitution. However, isocratic separations required a low degree of substitution, in accordance with a hypothesis previously put forward in connection with a theoretical and experimental study of the conditions for isocratic elution of macromolecules on amphiphilic gels. A study of the retention times of several proteins at different pH levels and buffer compositions indicated that different pH levels should be tested for maximal resolution and that, in many cases, the best resolution can be obtained if the DEAHP-agarose is operated in a buffer containing sodium acetate instead of sodium chloride. A quaternary amine agarose, 3-methyldiethylamino-2-hydroxy-propyl agarose (QAE-agarose), can be synthesized easily from DEAHP-agarose by alkylation with methyl iodide. The titration curves of DEAHP-agarose and QAE-agarose showed pK values around 9.5 and 11.3, respectively.

摘要

我们描述了一种制备阴离子交换剂的新方法,该方法简单且温和,基于烷基胺与环氧活化琼脂糖(由琼脂糖与丁二醇二缩水甘油醚反应制备)的偶联。由于环氧化物与OH或NH2基团反应时会形成极性OH基团,因此该离子交换剂未表现出任何疏水相互作用。这一点很重要,因为从具有疏水特性的离子交换剂上解吸蛋白质可能是不可能的,因为增加洗脱液的盐浓度以减少静电结合不可避免地会增强疏水相互作用。通过所述方法制备了3 - 二乙氨基 - 2 - 羟丙基琼脂糖(DEAHP - 琼脂糖)。在高取代度和低取代度下通过梯度洗脱均获得了蛋白质的高分辨率。然而,等度分离需要低取代度,这与先前针对两亲性凝胶上大分子等度洗脱条件的理论和实验研究提出的假设一致。对几种蛋白质在不同pH值和缓冲液组成下的保留时间的研究表明,为了获得最大分辨率,应测试不同的pH值,并且在许多情况下,如果DEAHP - 琼脂糖在含有乙酸钠而非氯化钠的缓冲液中操作,可以获得最佳分辨率。季胺琼脂糖,即3 - 甲基二乙氨基 - 2 - 羟丙基琼脂糖(QAE - 琼脂糖),可以通过用碘甲烷烷基化从DEAHP - 琼脂糖轻松合成。DEAHP - 琼脂糖和QAE - 琼脂糖的滴定曲线分别显示pK值约为9.5和11.3。

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