Molecular cloning and functional bacterial expression of a plant glucosidase specifically involved in alkaloid biosynthesis

生物合成 阿玛林 生物化学 葡萄糖苷酶 生物 生物碱 吲哚生物碱 夹竹桃科 立体化学 吲哚试验 大肠杆菌 化学 基因 植物 神经科学
作者
Heribert Warzecha,Irina Gerasimenko,Toni M. Kutchan,Joachim Stöckigt
出处
期刊:Phytochemistry [Elsevier BV]
卷期号:54 (7): 657-666 被引量:58
标识
DOI:10.1016/s0031-9422(00)00175-8
摘要

Monoterpenoid indole alkaloids are a vast and structurally complex group of plant secondary compounds. In contrast to other groups of plant products which produce many glycosides, indole alkaloids rarely occur as glucosides. Plants of Rauvolfia serpentina accumulate ajmaline as a major alkaloid, whereas cell suspension cultures of Rauvolfia mainly accumulate the glucoalkaloid raucaffricine at levels of 1.6 g/l. Cell cultures do contain a specific glucosidase. known as raucaffricine-O-beta-D-glucosidase (RG), which catalyzes the in vitro formation of vomilenine, a direct intermediate in ajmaline biosynthesis. Here, we describe the molecular cloning and functional expression of this enzyme in Escherichia coli. RG shows up to 60% amino acid identity with other glucosidases of plant origin and it shares several sequence motifs with family 1 glucosidases which have been characterized. The best substrate specificity for recombinant RG was raucaffricine (KM 1.3 mM, Vmax 0.5 nkat/microg protein) and only a few closely related structural derivatives were also hydrolyzed. Moreover, an early intermediate of ajmaline biosynthesis, strictosidine, is a substrate for recombinant RG (KM 1.8 mM, Vmax 2.6 pkat/microg protein) which was not observed for the low amounts of enzyme isolated from Rauvolfia cells.
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