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生氰糖苷的生物合成:糖基化步骤的体外分析

Biosynthesis of cyanogenic glucosides: in vitro analysis of the glucosylation step.

作者信息

Hösel W, Schiel O

出版信息

Arch Biochem Biophys. 1984 Feb 15;229(1):177-86. doi: 10.1016/0003-9861(84)90142-5.

Abstract

The last step in the biosynthesis of cyanogenic glucosides, the glucosylation of the cyanohydrin intermediate, has been investigated in detail using Triglochin maritima seedlings. The glucosyltransferase activity is not associated with membranes and appears to be a "soluble" enzyme. The cyanohydrin intermediate, which is formed by hydroxylation of 4-hydroxyphenylacetonitrile by a membrane-bound enzyme, is free to equilibrate in the presence of the glucosyltransferase and UDPG, because it can be trapped very efficiently. This indicates that this intermediate is not channeled (unlike some of the other intermediates), although it is probably the most labile of all of them. The glucosyltransferase of T. maritima responsible for the glucosylation of the cyanohydrin was separated from another glucosyltransferase, which used 4-hydroxybenzylalcohol as a substrate, and purified over 200-fold. It catalyzed the glucose transfer from UDPG to only 4-hydroxymandelonitrile and 3,4-dihydroxymandelonitrile, giving rise to the respective cyanogenic glucosides. Although the activities with these two substrates behaved differently in certain respects (e.g., extent of inactivation during purification and difference in activation by higher salt concentrations), most of the data acquired favor the view that only one enzyme in T. maritima is responsible for the glucosylation of both substrates.

摘要

利用海韭菜幼苗,对生氰糖苷生物合成的最后一步,即氰醇中间体的糖基化反应进行了详细研究。糖基转移酶活性与膜无关,似乎是一种“可溶性”酶。氰醇中间体由膜结合酶催化4-羟基苯乙腈羟基化形成,在糖基转移酶和UDPG存在的情况下可自由平衡,因为它能被非常有效地捕获。这表明该中间体不像其他一些中间体那样被通道化,尽管它可能是所有中间体中最不稳定的。负责氰醇糖基化的海韭菜糖基转移酶与另一种以4-羟基苄醇为底物的糖基转移酶分离,并纯化了200多倍。它催化UDPG中的葡萄糖仅转移到4-羟基苯乙腈和3,4-二羟基苯乙腈,生成相应的生氰糖苷。尽管这两种底物的活性在某些方面表现不同(例如,纯化过程中的失活程度和高盐浓度激活的差异),但获得的大多数数据支持这样一种观点,即海韭菜中只有一种酶负责这两种底物的糖基化。

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