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Enhanced artemisinin yield by expression of rol genes in artemisia annua

机译:通过青蒿中rol基因的表达提高青蒿素产量

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摘要

Background: Despite of many advances in the treatment of malaria, it is still the fifth most prevalent disease worldwide and is one of the major causes of death in the developing countries which accounted for 584,000 deaths in 2013, as estimated by World Health Organization. Artemisinin from Artemisia annua is still one of the most effective treatments for malaria. Increasing the artemisinin content of A. annua plants by genetic engineering would improve the availability of this much-needed drug. Methods: In this regard, a high artemisinin-yielding hybrid of A. annua produced by the centre for novel agricultural products of the University of York, UK, was selected (artemisinin maximally 1.4 %). As rol genes are potential candidates of biochemical engineering, genetic transformation of A. annua with Agrobacterium tumefaciens GV3101 harbouring vectors with rol B and rol C genes was carried out with the objective of enhancement of artemisinin content. Transgenic lines produced were analysed by the LC-MS for quantitative analysis of artemisinin and analogues. These high artemisinin yielding transgenics were also analysed by real time quantitative PCR to find the molecular dynamics of artemisinin enhancement. Genes of artemisinin biosynthetic pathway were studied including amorphadiene synthase (ADS), cytochrome P450, (CYP71AV1) and aldehyde dehydrogenase 1 (ALDH1). Trichome-specific fatty acyl-CoA reductase 1(TAFR1) is an enzyme involved in both trichome development and sesquiterpenoid biosynthesis and both processes are important for artemisinin biosynthesis. Thus, real time qPCR analysis of the TAFR1 gene was carried out, and trichome density was determined. Results: Transgenics of rol B gene showed two- to ninefold (the decimal adds nothing in the abstract, please simplify to two- to ninefold) increase in artemisinin, 4-12-fold increase in artesunate and 1.2-3-fold increase in dihydroartemisinin. Whereas in the case of rol C gene transformants, a fourfold increase in artemisinin, four to ninefold increase in artesunate and one- to twofold increase in dihydroartemisinin concentration was observed. Transformants with the rol B gene had higher expression of these genes than rol C transformants. TAFR1 was also found to be more expressed in rol gene transgenics than wild type A. annua, which was also in accordance with the trichome density of the respective plant. Conclusion: Thus it was proved that rol B and rol C genes are effective in the enhancement of artemisinin content of A. annua, rol B gene being more active to play part in this enhancement than rol C gene.
机译:背景:尽管在疟疾治疗方面取得了许多进步,但它仍然是全世界第五大流行疾病,并且是发展中国家的主要死因之一,据世界卫生组织估计,2013年该疾病导致584,000人死亡。来自青蒿的青蒿素仍然是治疗疟疾的最有效方法之一。通过基因工程增加青蒿植物中青蒿素的含量,将提高这种急需药物的利用率。方法:在这方面,选择了由英国约克大学新型农产品中心生产的高产青蒿素杂交种青蒿(青蒿素最大含量为1.4%)。由于rol基因是生化工程的潜在候选者,目的是通过具有根癌农杆菌GV3101的农杆菌的遗传转化来携带青蒿素含量,所述根癌农杆菌GV3101包含具有rol B和rol C基因的载体。通过LC-MS分析产生的转基因品系,以对青蒿素及其类似物进行定量分析。还通过实时定量PCR分析了这些高产青蒿素的转基因,以发现青蒿素增强的分子动力学。研究了青蒿素生物合成途径的基因,包括吗啡二烯合酶(ADS),细胞色素P450(CYP71AV1)和醛脱氢酶1(ALDH1)。 Trichome特异性脂肪酰基辅酶A还原酶1(TAFR1)是一种酶,参与毛状体发育和倍半萜生物合成,这两个过程对于青蒿素的生物合成都很重要。因此,对TAFR1基因进行了实时qPCR分析,并测定了毛线密度。结果:rol B基因转基因显示青蒿素增加了2到9倍(十进制中没有添加任何东西,请简化为2到9倍),青蒿琥酯增加了4-12倍,双氢青蒿素增加了1.2-3倍。而在rol C基因转化子中,青蒿素增加了四倍,青蒿琥酯增加了四到九倍,二氢青蒿素浓度增加了一到两倍。具有rol B基因的转化体比rol C转化体具有更高的表达水平。还发现TAFR1在rol基因转基因中比野生型A.annua更表达,这也与相应植物的毛线密度一致。结论:由此证明,rol B和rol C基因在增强青蒿中青蒿素含量方面是有效的,而rol B基因比rol C基因更活跃。

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