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首页> 外文期刊>Plant Biotechnology >Molecular cloning of flavonoid biosynthetic genes and biochemical characterization of anthocyanin O-methyltransferase of NemophiLa menziesii Hook, and Arn.
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Molecular cloning of flavonoid biosynthetic genes and biochemical characterization of anthocyanin O-methyltransferase of NemophiLa menziesii Hook, and Arn.

机译:黄酮类生物合成基因的分子克隆和Nemophira menziesii钩的花青素O-甲基转移酶的生化特征,ARN。

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摘要

Blue flower color of Nemophila menziesii Hook, and Arn. is derived from a metalloanthocyanin, nemophilin, which comprises petunidin-3-0-[6-0-(trans-p-coumaroyl)-β-glucoside]-5-O-[6-O-(malonyl)-β-glucoside], apigenin-7-O- β-glucoside-4′-O-(6-O-malonyl)-β-glucoside, and Mg~(2+) and Fe~(3+) ions. The flavonoid biosynthetic pathway of nemophilin has not yet been characterized. RNA-Seq analysis of the petals yielded 61,491 contigs. These were searched using BLAST against petunia or torenia flavonoid biosynthetic proteins, which identified 11 putative full-length protein sequences belonging to the flavonoid biosynthetic pathway. RT-PCR using primers designed on the basis of these sequences yielded 14 sequences. Spatio-temporal transcriptome analysis indicated that genes involved in the early part of the pathway are strongly expressed during early-petal development and that those in the late part at late-flower opening stages, but they are rarely expressed in leaves. Flavanone 3-hydroxylase and flavonoid 3′,5′-hydroxylase cDNAs were successfully expressed in yeast to confirm their activities. Recombinant anthocyanin O-methyltransferase cDNA (NmAMT6) produced using Escherichia coli was subjected to biochemical characterization. Km of NmAMT6 toward delphinidin 3-O-glucoside was 22μM,which is comparable with Km values of anthocyanin O-methyltransferases from other plants. With delphinidin 3-O-glucoside as substrate, NmAMT6 almost exclusively yielded petunidin 3-O-glucoside rather than malvidin 3-O-glucoside. This specificity is consistent with the anthocyanin composition of Nemophila petals.
机译:Nemophila menziesii hook的蓝色花颜色和Arn。衍生自甲苯钴素,内美蛋白,其包含彼营蛋白-3-0- [6-0-(Trans-p-coumaroyl)-β-葡糖苷] -5-O- [6-O-(Malonyl)-β-葡糖苷] ],Apigenin-7-O-β-葡糖苷-4'-O-(6-O-丙二酰基)-β-葡糖苷,和Mg〜(2+)和Fe〜(3+)离子。 Nemophilin的类黄酮化生物合成途径尚未表征。花瓣的RNA-SEQ分析产生61,491个Contigs。这些搜索这些对抗矮牵牛或托雷尼亚黄酮类生物合成蛋白的爆炸,该蛋白质鉴定了属于类黄酮生物合成途径的11个推定的全长蛋白质序列。 RT-PCR使用基于这些序列设计的引物产生14个序列。时空转录组分析表明,涉及途径早期部分的基因在早期的发展中强烈表达,并且在晚开阶段后期的那些,但它们很少在叶子中表达。黄万酮3-羟化酶和黄酮类化合物3',5'-羟化酶CDNA在酵母中成功地表达以确认其活性。使用大肠杆菌生产的重组花青素型o-甲基转移酶cDNA(NMAMT6)进行生化表征。 NMAMT6朝向林肽3-O-葡糖苷的km为22μm,与来自其他植物的花青素O-甲基转移酶的KM值相当。用蛋白苷3-O-葡糖苷作为底物,NMAMT6几乎完全产生了喇叭蛋白3-O-葡糖苷而不是麦类3-O-葡糖苷。这种特异性与Nemophila花瓣的花青素组成一致。

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