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The molecular cloning of artemisinic aldehyde Δ11(13) reductase and its role in glandular trichome-dependent biosynthesis of artemisinin in Artemisia annua

机译:青蒿醛Δ11(13)还原酶的分子克隆及其在青蒿中青蒿素依赖的青蒿素生物合成中的作用

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摘要

At some point during biosynthesis of the antimalarial artemisinin in glandular trichomes of Artemisia annua, the Delta 11(13) double bond originating in amorpha-4,11-diene is reduced. This is thought to occur in artemisinic aldehyde, but other intermediates have been suggested. In an effort to understand double bond reduction in artemisinin biosynthesis, extracts of A. annua flower buds were investigated and found to contain artemisinic aldehyde Delta 11(13) double bond reductase activity. Through a combination of partial protein purification, mass spectrometry, and expressed sequence tag analysis, a cDNA clone corresponding to the enzyme was isolated. The corresponding gene Dbr2, encoding a member of the enoate reductase family with similarity to plant 12-oxophytodienoate reductases, was found to be highly expressed in glandular trichomes. Recombinant Dbr2 was subsequently characterized and shown to be relatively specific for artemisinic aldehyde and to have some activity on small alpha,beta-unsaturated carbonyl compounds. Expression in yeast of Dbr2 and genes encoding four other enzymes in the artemisinin pathway resulted in the accumulation of dihydroartemsinic acid. The relevance of Dbr2 to trichome-specific artemisinin biosynthesis is discussed.
机译:在青蒿的腺毛中抗疟药青蒿素的生物合成过程中,源自无定形4,11-二烯的Delta 11(13)双键被还原。认为这是在青蒿素醛中发生的,但是已经提出了其他中间体。为了理解青蒿素生物合成中的双键还原,调查了A. annua花芽的提取物,发现其含有青蒿醛Delta 11(13)双键还原酶活性。通过部分蛋白质纯化,质谱和表达序列标签分析的组合,分离了与该酶相对应的cDNA克隆。发现相应的基因Dbr2,其编码与植物12-氧代二乙二酸还原酶相似的烯酸还原酶家族的成员,在腺毛状体中高表达。重组Dbr2随后进行了表征,并显示出对青蒿素醛具有相对特异性,并且对小的α,β-不饱和羰基化合物具有一定的活性。 Dbr2在酵母中的表达以及青蒿素途径中编码其他四种酶的基因导致了二氢青蒿素酸的积累。讨论了Dbr2与毛状体特异青蒿素生物合成的相关性。

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