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作为亲和色谱基质的琼脂糖4B。使用氮氧化物作为模型配体的自旋标记研究。

Sepharose 4B as a matrix for affinity chromatography. A spin-labelling investigation using nitroxides as model ligands.

作者信息

Aplin J D, Hall L D

出版信息

Eur J Biochem. 1980 Sep;110(1):295-309. doi: 10.1111/j.1432-1033.1980.tb04868.x.

Abstract

Nitroxide spin labels were attached to CNBr-activated Sepharose 4B directly and through oligoglycines and oo-amino-carboxylic acids of varying length. The homogeneity of the carbohydrate environments of directly attached labels was investigated by measuring dipolar interactions between nitroxides as a function of solvation and of spin dilution with a diamagnetic analogue, as well as by electron exchange between the nitroxides and paramagnetic metal ions in solution. Only the exchange experiment revealed any inhomogeneity, suggesting that a small proportion of sites may be less accessible than the majority. The distances between sites were sufficiently small to allow, in principle, multiple-site interactions between quite small proteins in solution and immobilized ligands. Reorientation of the label at the matrix, characterized by the correlation time t, became more rapid with increasing spacer length n. For n > 12, the decrease in t was less pronounced. The two types of spacer behaved similarly. Thus an ideal spacer length for affinity separations is 12 atoms; this is in good agreement with data from a variety of affinity separations. The results of electron spin resonance studies of the effect of non-aqueous solvent on directly and indirectly labelled Sepharose 4B were used to suggest reasons why enzymes immobilized on Sepharose may be stabilized to denaturing solvents.

摘要

氮氧化物自旋标记物直接以及通过不同长度的寡甘氨酸和α-氨基羧酸连接到溴化氰活化的琼脂糖4B上。通过测量氮氧化物之间的偶极相互作用(作为溶剂化作用和用抗磁性类似物进行自旋稀释的函数)以及通过氮氧化物与溶液中顺磁性金属离子之间的电子交换,研究了直接连接的标记物的碳水化合物环境的均匀性。只有交换实验揭示了任何不均匀性,这表明一小部分位点可能比大多数位点更难接近。位点之间的距离足够小,原则上允许溶液中相当小的蛋白质与固定化配体之间发生多位点相互作用。标记物在基质上的重排,以相关时间t为特征,随着间隔长度n的增加而变得更快。对于n>12,t的降低不太明显。两种类型的间隔物表现相似。因此,亲和分离的理想间隔长度是12个原子;这与各种亲和分离的数据非常一致。关于非水溶剂对直接和间接标记的琼脂糖4B影响的电子自旋共振研究结果被用来推测固定在琼脂糖上的酶可能对变性溶剂稳定的原因。

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