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Molecular cloning and overexpression of the tyrosine aminotransferase (TAT) gene leads to increased rosmarinic acid yield in Perilla frutescens

机译:酪氨酸氨基转移酶(TAT)基因的分子克隆和过度表达导致紫苏中迷迭香酸产量的增加

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摘要

Perilla frutescens is a medicinal plant that produces various bioactive compounds, including unsaturated fatty acids and phenolic compounds such as rosmarinic acid (α-O-caffeoyl-3, 4 -dihydroxyphenylacetic acid, RA). Tyrosine aminotransferase (TAT) catalyzes the first step in the tyrosine-derived branch of RA biosynthesis, and TAT is presumed to have a role in RA accumulation. Here, we report the isolation of full-length TAT cDNA (designated PfTAT) from P. frutescens. Sequence analysis revealed that PfTAT contained 1,535 bp long and an open reading frame of 1,233 bp encoding 411 amino acid residues. Analysis of PfTAT genomic DNA revealed 7 exons and 5 introns. The 5′ flanking sequence of PfTAT was also cloned, and a group of putative cis-acting elements such TATA box, CAAT box, TC-rich repeats and G box were identified. Quantitative real-time PCR analysis indicated that constitutive expression of PfTAT in leaves was much higher than in roots and stems. A vector was constructed containing the PfTAT gene derived by the cauliflower mosaic virus 35S promoter. Transgenic P. frutescens overexpressing PfTAT was obtained with an Agrobacterium tumefaciens-mediated transformation system and overexpression was confirmed by PCR and Southern blot. PfTAT mRNA expression in transgenic plant lines measured by real-time quantitative PCR was 2–3 times greater than PfTAT expression in the untransformed plant line. Also, enhanced gene expression corresponded to significantly increased RA in PfTAT-transgenic lines, as quantified by HPLC. Our data emphasize the importance of PfTAT in the production of RA in P. frutescens.
机译:紫苏是一种药用植物,会产生各种生物活性化合物,包括不饱和脂肪酸和酚类化合物,例如迷迭香酸(α-O-咖啡酰-3、4-二羟基苯基乙酸,RA)。酪氨酸氨基转移酶(TAT)催化酪氨酸衍生的RA生物合成分支的第一步,并且推测TAT在RA积累中具有作用。在这里,我们报告从疫霉中分离出全长TAT cDNA(称为PfTAT)。序列分析显示,PfTAT包含1,535 bp长,一个1,233 bp的开放阅读框,编码411个氨基酸残基。对PfTAT基因组DNA的分析显示有7个外显子和5个内含子。还克隆了PfTAT的5'侧翼序列,并鉴定了一组推定的顺式作用元件,例如TATA盒,CAAT盒,富含TC的重复序列和G盒。实时定量PCR分析表明,PfTAT在叶中的组成型表达远高于根和茎。构建了包含花椰菜花叶病毒35S启动子衍生的PfTAT基因的载体。用根癌农杆菌介导的转化系统获得了过表达PfTAT的转基因弗氏疟原虫,并通过PCR和Southern印迹证实了过表达。通过实时定量PCR测定的转基因植物品系中的PfTAT mRNA表达是未转化植物品系中PfTAT表达的2-3倍。而且,如通过HPLC定量的,增强的基因表达对应于PfTAT转基因系中的RA显着增加。我们的数据强调了PfTAT在弗氏假单胞菌RA生产中的重要性。

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    Laboratory of Food Additives and Nutrition College of Food Engineering and Biological Technology Tianjin University of Science and Technology">(1);

    Laboratory of Food Additives and Nutrition College of Food Engineering and Biological Technology Tianjin University of Science and Technology">(1);

    Laboratory of Food Additives and Nutrition College of Food Engineering and Biological Technology Tianjin University of Science and Technology">(1);

    Laboratory of Food Additives and Nutrition College of Food Engineering and Biological Technology Tianjin University of Science and Technology">(1);

    Tianjin Entry-Exit Inspection and Quarantine Bureau">(2);

    Laboratory of Food Additives and Nutrition College of Food Engineering and Biological Technology Tianjin University of Science and Technology">(1);

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  • 原文格式 PDF
  • 正文语种 eng
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  • 关键词

    Perilla frutescens; PfTAT; cDNA cloning; Overexpression; Rosmarinic acid;

    机译:紫苏;PfTAT;cDNA克隆;过度表达;迷迭香酸;

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