Département de Sciences Biologique, Université de Montréal, Saskatoon, Saskatchewan Canada S7N 0W9.
Plant Physiol. 1990 Nov;94(3):1323-9. doi: 10.1104/pp.94.3.1323.
Young leaves from Catharanthus roseus plants contain the enzymes which convert the monoterpenoid indole alkaloid, tabersonine by three hydroxylations, two methylations, and one acetylation step to vindoline. A novel direct enzyme assay has been developed for a hydroxylase involved in vindoline biosynthesis, which catalyzes the C4-hydroxylation of 2,3-dihydro-3-hydroxy-N(1)-methyltabersonine to the 3,4-dihydroxy derivative. The enzyme showed an absolute requirement for 2-oxoglutarate and enzymatic activity was enhanced by ascorbate, establishing it as a 2-oxoglutarate-dependent dioxygenase (EC 1.14.11.-). The hydroxylase exhibited specificity for position 4 of various alkaloid substrates. The enzyme exhibited a pH optima between 7 and 8 and an apparent molecular weight of 45,000. The appearance of 4-hydroxylase activity was developmentally regulated and was shown to be inducible by light treatment of seedlings. Substrate specificity studies of this enzyme for indole alkaloid substrate suggested that hydroxylation at position 3 and N-methylation occur prior to hydroxylation at position 4. This is in agreement with previous studies which suggest that C4-hydroxylation is the second to last step in vindoline biosynthesis in Catharanthus roseus.
长春花幼叶中含有将单萜吲哚生物碱——塔巴林通过三步羟化、两步甲基化和一步乙酰化转化为长春碱的酶。我们开发了一种新型的直接酶测定法,用于研究参与长春碱生物合成的羟化酶,该酶能催化 2,3-二氢-3-羟基-N(1)-甲基塔巴林的 C4-羟化,生成 3,4-二羟基衍生物。该酶表现出对 2-氧戊二酸的绝对需求,且抗坏血酸能增强酶活性,这表明它是一种 2-氧戊二酸依赖性双加氧酶(EC 1.14.11.-)。羟化酶对各种生物碱底物的 4 位具有特异性。该酶在 pH7-8 之间表现出最佳活性,表观分子量为 45000。4-羟化酶活性的出现受到发育调控,并且可以通过幼苗的光照处理诱导。对该酶的吲哚生物碱底物的特异性研究表明,3 位羟化和 N-甲基化发生在 4 位羟化之前。这与先前的研究结果一致,即 C4-羟化是长春花中长春碱生物合成的倒数第二步。
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