A rapid direct assay of 3'-5' cyclic nucleotide phosphodiesterase activity using chromatography on immobilized acriflavin.

C Rochette-Egly, J M Egly
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Abstract

A chromatographic method using immobilized acriflavin has been developed for the separation of unreacted cyclic nucleotides from their corresponding 5'-nucleotides, in a direct assay of 3'-5' cyclic nucleotide phosphodiesterase using [3H]-cyclic nucleotides as substrate. The method based on the so-called charge-transfer overlap recognition between flavin and indol rings, provides a rapid (15-20 min) and sensitive elution of [3H]-5'nucleotides with high recovery (up to 98%) and low blanks, while [3H]-cyclic nucleotides are retarded on the column. By this method, the formation of some secondary products by purine metabolizing enzymes such as 5'-nucleotidases, nucleosidases and/or deaminases is taken into account, using [14C]-5'-AMP thus allowing an accurate determination of phosphodiesterase activity in any preparations.

固定化吖啶黄素上3′-5′环核苷酸磷酸二酯酶活性的快速直接测定。
以[3H]环核苷酸为底物,直接测定3'-5'环核苷酸磷酸二酯酶,采用固定化吖啶黄素色谱法分离未反应的环核苷酸和相应的5'-核苷酸。该方法基于黄素和吲哚环之间所谓的电荷转移重叠识别,提供了快速(15-20分钟)和灵敏的[3H]-5'核苷酸洗脱,回收率高(高达98%),低空白,而[3H]-环核苷酸在色谱柱上延迟。通过这种方法,考虑到嘌呤代谢酶如5′-核苷酸酶、核苷酶和/或脱氨酶形成的一些次级产物,使用[14C]-5′-AMP,从而可以准确测定任何制剂中的磷酸二酯酶活性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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