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用非甾体配体对类固醇转化酶进行“亲和”色谱分析。

"Affinity" chromatography of steroid-transforming enzymes with a non-steroidal ligand.

作者信息

Renwick A G, Chambers S M, Willcox P

出版信息

Biochem J. 1979 Feb 1;177(2):401-8. doi: 10.1042/bj1770401.

Abstract

The chromatographic behaviour of an avian oestradiol-17 beta dehydrogenase, the 3(17) beta-hydroxy steroid dehydrogenase from Pseudomonas testosteroni and cortisone reductase from Streptomyces dehydrogenans was studied on columns of p-(phenoxypropoxy)aniline attached to CNBr-activated Sepharose. The ligand was effective in adsorbing the oestradiol dehydrogenase from a partially purified extract of chicken liver, and the cortisone reductase was perferentially retained when mixtures of the three dehydrogenases were applied to columns in 10mM-buffer. Under these conditions the 3(17)beta-hydroxy steroid dehydrogenase was eluted in the front, but was adsorbed in the presence of 3 M-KCl. beta-N-Acetylglucosaminidase present in the liver preparation was not retained by the ligand, whereas lactate dehydrogenase from rabbit muscle was adsorbed in a manner similar to the retention pattern found on affinity chromatography with 2',5'-ADP--Sepharose. The mean overall purification of the oestradiol dehydrogenase was 13-fold, with a mean recovery of 53%. p-(Phenoxypropoxy)aniline offers promise for the purification of steroid-transforming enzymes where elution with substrate or cofactor is not wanted. It is also suggested that the ligand may be of service in the purification of receptors of hormonal steroids.

摘要

研究了禽类雌二醇-17β脱氢酶、睾丸酮假单胞菌的3(17)β-羟基类固醇脱氢酶和脱氢链霉菌的可的松还原酶在连接到溴化氰活化琼脂糖上的对-(苯氧基丙氧基)苯胺柱上的色谱行为。该配体可有效地从鸡肝部分纯化提取物中吸附雌二醇脱氢酶,当将三种脱氢酶的混合物应用于10mM缓冲液中的柱时,可的松还原酶被优先保留。在这些条件下,3(17)β-羟基类固醇脱氢酶在前沿被洗脱,但在3M-KCl存在下被吸附。肝制剂中存在的β-N-乙酰氨基葡萄糖苷酶不被该配体保留,而兔肌肉中的乳酸脱氢酶的吸附方式与用2',5'-ADP-琼脂糖进行亲和色谱时的保留模式相似。雌二醇脱氢酶的平均总纯化倍数为13倍,平均回收率为53%。对-(苯氧基丙氧基)苯胺为不需要用底物或辅因子洗脱的类固醇转化酶的纯化提供了希望。还表明该配体可能有助于纯化激素类固醇的受体。

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