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Genetic engineering of shikonin biosynthesis hairy root cultures of Lithospermum erythrorhizon transformed with the bacterial ubiC gene

机译:细菌ubiC基因转化紫草紫草的紫草素生物合成毛状根培养物的遗传工程

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摘要

The biosynthetic pathway to 4-hydroxybenzoate (4HB), a precursor of the naphthoquinone pigment shikonin, was modified in Lithospermum erythrorhizon hairy root cultures by introduction of the bacterial gene ubiC. This gene of Escherichia coli encodes chorismate pyruvate-lyase (CPL), an enzyme that converts chorismate into 4HB and is not normally present in plants. The ubiC gene was fused to the sequence for a chloroplast transit peptide and placed under control of a constitutive plant promoter. This construct was introduced into L. erythrorhizon by Agrobacterium rhizogenes-mediated transformation. The resulting hairy root cultures showed high CPL activity. 4HB produced by the CPL reaction was utilized for shikonin biosynthesis, as shown by in vivo inhibition of the native pathway to 4HB with 2-aminoindan-2-phosphonic acid (AIP), an inhibitor of phenylalanine ammonia-lyase. A feeding experiment with [1,7- super(13)C sub(2)]shikimate showed that in the absence of AIP the artificially introduced CPL reaction contributed ca. 20% of the overall 4HB biosynthesis in the transgenic cultures. ubiC transformation did not lead to a statistically significant increase of shikonin formation, but to a 5-fold increase of the accumulation of menisdaurin, a nitrile glucoside which is presumably related to aromatic amino acid metabolism.
机译:通过引入细菌基因ubiC,在紫草红毛毛根培养物中修饰了萘醌色素紫草素前体4-羟基苯甲酸酯(4HB)的生物合成途径。大肠杆菌的该基因编码分支酸丙酮酸裂合酶(CPL),一种将分支酸转化为4HB的酶,通常在植物中不存在。 ubiC基因融合到叶绿体转运肽的序列上,并置于组成型植物启动子的控制下。通过发根农杆菌介导的转化将该构建体引入到紫杉菌中。所得的毛状根培养物显示出高的CPL活性。由CPL反应产生的4HB用于紫草素生物合成,如体内用苯丙氨酸解氨酶抑制剂2-氨基茚满-2-膦酸(AIP)抑制4HB的天然途径所示。用[1,7-super(13)C sub(2)] shikimate进行的补料实验表明,在没有AIP的情况下,人工引入的CPL反应可产生约5%的酸。转基因培养物中全部4HB生物合成的20%。 ubiC转化并没有导致统计学上紫草素形成的显着增加,但导致半月板苷(一种可能与芳香族氨基酸代谢有关的腈糖苷)的积聚增加了5倍。

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