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Cell Type–Specific Localization of Transcripts Encoding Nine Consecutive Enzymes Involved in Protoberberine Alkaloid Biosynthesis

机译:细胞类型特异性转录原的编码小ber碱生物碱生物合成的九个连续酶的转录本。

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摘要

Molecular clones encoding nine consecutive biosynthetic enzymes that catalyze the conversion of l-dopa to the protoberberine alkaloid (S)-canadine were isolated from meadow rue (Thalictrum flavum ssp glaucum). The predicted proteins showed extensive sequence identity with corresponding enzymes involved in the biosynthesis of related benzylisoquinoline alkaloids in other species, such as opium poppy (Papaver somniferum). RNA gel blot hybridization analysis showed that gene transcripts for each enzyme were most abundant in rhizomes but were also detected at lower levels in roots and other organs. In situ RNA hybridization analysis revealed the cell type–specific expression of protoberberine alkaloid biosynthetic genes in roots and rhizomes. In roots, gene transcripts for all nine enzymes were localized to immature endodermis, pericycle, and, in some cases, adjacent cortical cells. In rhizomes, gene transcripts encoding all nine enzymes were restricted to the protoderm of leaf primordia. The localization of biosynthetic gene transcripts was in contrast with the tissue-specific accumulation of protoberberine alkaloids. In roots, protoberberine alkaloids were restricted to mature endodermal cells upon the initiation of secondary growth and were distributed throughout the pith and cortex in rhizomes. Thus, the cell type–specific localization of protoberberine alkaloid biosynthesis and accumulation are temporally and spatially separated in T. flavum roots and rhizomes, respectively. Despite the close phylogeny between corresponding biosynthetic enzymes, distinct and different cell types are involved in the biosynthesis and accumulation of benzylisoquinoline alkaloids in T. flavum and P. somniferum. Our results suggest that the evolution of alkaloid metabolism involves not only the recruitment of new biosynthetic enzymes, but also the migration of established pathways between cell types.
机译:从草地上分离出编码九种连续的生物合成酶的分子克隆,所述酶催化1-多巴转化为原小ber碱生物碱(S)-卡纳丁(Sad-canadine)(thalictrum flavum ssp glaucum)。预测的蛋白质与其他物种如罂粟(罂粟)的相关苄基异喹啉生物碱的生物合成中涉及的相应酶具有广泛的序列同一性。 RNA凝胶印迹杂交分析表明,每种酶的基因转录本在根茎中含量最高,但在根和其他器官中也检测到较低的水平。原位RNA杂交分析揭示了根部和根茎中小ber碱生物碱生物合成基因的细胞类型特异性表达。在根中,所有九种酶的基因转录本均定位于未成熟的内胚层,周周以及在某些情况下邻近的皮质细胞。在根茎中,编码所有九种酶的基因转录本仅限于叶原基的原皮。生物合成基因转录本的定位与原小ber碱生物碱的组织特异性积累相反。在根部,原小ber碱生物碱在次生生长开始时仅限于成熟的内胚层细胞,并分布在根茎的整个髓和皮质中。因此,黄柏生物碱生物合成和积累的细胞类型特异性定位在时间和空间上分别在黄萎病根和根茎中分开。尽管相应的生物合成酶之间的亲缘关系很近,但是不同的细胞类型也参与了黄T和大豆假单胞菌中苄基异喹啉生物碱的生物合成和积累。我们的结果表明,生物碱代谢的进化不仅涉及新生物合成酶的募集,而且还涉及细胞类型之间已建立途径的迁移。

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