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首页> 外文期刊>Plant Cell, Tissue and Organ Culture: An International Journal on in Vitro Culture of Higher Plants >Glandular trichome-specific expression of alcohol dehydrogenase 1 (ADH1) using a promoter-GUS fusion in Artemisia annua L.
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Glandular trichome-specific expression of alcohol dehydrogenase 1 (ADH1) using a promoter-GUS fusion in Artemisia annua L.

机译:在Artemisia Annua L中使用启动子 - GUS融合的醇脱氢酶1(ADH1)的腺体滴毛瘤特异性表达。

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摘要

Artemisinin, isolated from Artemisia annua L., is widely known as a functional anti-malaria drug. Due to the low content of artemisinin in A. annua plants, great efforts have been made to determine the artemisinin biosynthetic pathway by genetic engineering. ADH1, encoding an alcohol dehydrogenase, was cloned from the glandular secretory trichomes (GSTs) in A. annua. The gene expression analysis showed that ADH1 was predominately expressed in buds and young leaves, and the expression of ADH1 was the highest in the youngest leaves. To further investigate the expression pattern of ADH1 in A. annua, a 1070-bp promoter region of ADH1 was cloned. We found 14 putative cis-elements were presented in the ADH1 promoter sequence, indicating that ADH1 is complexly regulated. The ADH1 promoter sequence was fused to the beta-glucuronidase reporter gene (GUS) and introduced into A. annua plants. GUS signals were only found in the glandular secretory trichomes of young tissues in transgenic A. annua plants. Besides, the treatment of A. annua seedlings with 100 mu M methyl jasmonate (MeJA) and 100 mu M abscisic acid (ABA), respectively, increased the ADH1 transcript levels. The dual luciferase (dual-LUC) assay demonstrated that the reported transcription factors, MYC2 and ERF1, activated the expression of ADH1 in vivo. Our study shows that ADH1 gene is exclusively expressed in the glandular secretory trichomes of young tissues of A. annua, it implies that the promoter of ADH1 gene could be used in engineering of A. annua for increasing artemisinin content.
机译:来自Artemisia Annua L.的氨甲酸,被广泛称为功能性抗疟疾药物。由于ANNUA植物中的青蒿素含量较低,已经进行了巨大的努力来确定通过基因工程来确定蒿蛋白生物合成途径。编码醇脱氢酶的ADH1从A annua的腺体分泌毛滴(GST)中克隆。基因表达分析表明,ADH1主要用芽和幼叶表达,并且ADH1的表达是最年轻的叶子中最高的。为了进一步研究A.Anua中ADH1的表达模式,克隆了ADH1的1070bp启动子区。我们发现14个推定的顺式元素在ADH1启动子序列中呈现,表明ADH1是复杂的调节。将ADH1启动子序列融合给β-葡糖醛酸酶报告基因(GUS)并引入A.Anua植物。 GUS信号仅在转基因A. annua植物中的年轻组织的腺体分泌毛状体中发现。此外,分别治疗100 mu m甲酸亚甲酸(Meja)和100μm脱落酸(aba)的Anua幼苗增加了ADH1转录水平。双荧光素酶(Dual-Luc)测定表明,报告的转录因子,MyC2和ERF1,活化了体内ADH1的表达。我们的研究表明,ADH1基因仅在A. Annua的年轻组织的腺体分泌毛子中表达。它意味着ADH1基因的启动子可用于A. Annua的工程,用于增加青蒿素含量。

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  • 作者单位

    Shanghai Jiao Tong Univ Key Lab Urban Agr South SJTU Fudan Nottingham Plant Biotechnol R&

    D Ctr Minist Agr Plant Biotechnol Res Ctr Sch Agr &

    Bio Shanghai 200240 Peoples R China;

    Shanghai Jiao Tong Univ Key Lab Urban Agr South SJTU Fudan Nottingham Plant Biotechnol R&

    D Ctr Minist Agr Plant Biotechnol Res Ctr Sch Agr &

    Bio Shanghai 200240 Peoples R China;

    Shanghai Jiao Tong Univ Key Lab Urban Agr South SJTU Fudan Nottingham Plant Biotechnol R&

    D Ctr Minist Agr Plant Biotechnol Res Ctr Sch Agr &

    Bio Shanghai 200240 Peoples R China;

    Shanghai Jiao Tong Univ Key Lab Urban Agr South SJTU Fudan Nottingham Plant Biotechnol R&

    D Ctr Minist Agr Plant Biotechnol Res Ctr Sch Agr &

    Bio Shanghai 200240 Peoples R China;

    Shanghai Jiao Tong Univ Key Lab Urban Agr South SJTU Fudan Nottingham Plant Biotechnol R&

    D Ctr Minist Agr Plant Biotechnol Res Ctr Sch Agr &

    Bio Shanghai 200240 Peoples R China;

    Shanghai Jiao Tong Univ Key Lab Urban Agr South SJTU Fudan Nottingham Plant Biotechnol R&

    D Ctr Minist Agr Plant Biotechnol Res Ctr Sch Agr &

    Bio Shanghai 200240 Peoples R China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 植物细胞学;
  • 关键词

    Abscisic acid; Artemisinin; Glandular secretory trichomes; beta-Glucuronidase; Methyl jasmonate;

    机译:脱落酸;青蒿素;腺体分泌毛状体;β-葡糖醛酸酶;茉莉酸甲酯;

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