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A Dioxygenase Catalyzes Steroid 16α-Hydroxylation in Steroidal Glycoalkaloid Biosynthesis

机译:双加氧酶催化甾体生物碱合成中的甾体16α-羟基化。

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摘要

Steroidal glycoalkaloids (s) are toxic specialized metabolites that are found in the Solanaceae. Potato (Solanum tuberosum) contains the s α-solanine and α-chaconine, while tomato (Solanum lycopersicum) contains α-tomatine, all of which are biosynthesized from cholesterol. However, although two cytochrome P450 monooxygenases that catalyze the 22- and 26-hydroxylation of cholesterol have been identified, the 16-hydroxylase remains unknown. Feeding with deuterium-labeled cholesterol indicated that the 16α- and 16β-hydrogen atoms of cholesterol were eliminated to form α-solanine and α-chaconine in potato, while only the 16α-hydrogen atom was eliminated in α-tomatine biosynthesis, suggesting that a single oxidation at C-16 takes place during tomato biosynthesis while a two-step oxidation occurs in potato. Here, we show that a 2-oxoglutarate-dependent dioxygenase, designated as 16DOX, is involved in biosynthesis. We found that the transcript of potato 16DOX (St16DOX) was expressed at high levels in the tuber sprouts, where large amounts of s are accumulated. Biochemical analysis of the recombinant St16DOX protein revealed that St16DOX catalyzes the 16α-hydroxylation of hydroxycholesterols and that (22S)-22,26-dihydroxycholesterol was the best substrate among the nine compounds tested. St16DOX-silenced potato plants contained significantly lower levels of s, and a detailed metabolite analysis revealed that they accumulated the glycosides of (22S)-22,26-dihydroxycholesterol. Analysis of the tomato 16DOX (Sl16DOX) gene gave essentially the same results. These findings clearly indicate that 16DOX is a steroid 16α-hydroxylase that functions in the biosynthetic pathway. Furthermore, St16DOX silencing did not affect potato tuber yield, indicating that 16DOX may be a suitable target for controlling toxic levels in potato.
机译:甾体类生物碱是茄科中发现的有毒专门代谢产物。马铃薯(Solanum tuberosum)含有α-茄碱和α-查茄碱,而番茄(Solanum lycopersicum)含有α-番茄碱,所有这些都是由胆固醇生物合成的。然而,尽管已经鉴定出两种催化胆固醇的22-和26-羟基化的细胞色素P450单加氧酶,但是16-羟化酶仍然未知。饲喂氘标记的胆固醇表明,胆固醇中的胆固醇的16α-和16β-氢原子被消除,从而形成马铃薯中的α-茄碱和α-查茄碱,而α-番茄碱的生物合成中仅消除了16α-氢原子。番茄生物合成过程中,C-16处发生单氧化,而马铃薯则发生两步氧化。在这里,我们显示了2-氧戊二酸酯依赖性双加氧酶,称为16DOX,参与生物合成。我们发现马铃薯16DOX(St16DOX)的转录本在块茎芽中高水平表达,其中大量s积累。重组St16DOX蛋白质的生化分析表明,St16DOX催化羟基胆固醇的16α-羟基化,并且(22S)-22,26-二羟基胆固醇是测试的9种化合物中最佳的底物。 St16DOX沉默的马铃薯植株中的s含量显着降低,详细的代谢产物分析表明它们积聚了(22S)-22,26-二羟基胆固醇的糖苷。番茄16DOX(S16DOX)基因的分析给出了基本相同的结果。这些发现清楚地表明16DOX是在生物合成途径中起作用的类固醇16α-羟化酶。此外,St16DOX沉默不会影响马铃薯块茎的产量,这表明16DOX可能是控制马铃薯中毒性水平的合适靶标。

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