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在烟草中分离和鉴定苏氨酸脱氨酶启动子。

Isolation and characterization of the threonine deaminase promoter in Nicotiana attenuata.

机构信息

Department of Molecular Ecology, Max-Planck Institute of Chemical Ecology, Hans Knöll Str. 8, D-07745 Jena, Germany.

Department of Molecular Ecology, Max-Planck Institute of Chemical Ecology, Hans Knöll Str. 8, D-07745 Jena, Germany.

出版信息

Plant Sci. 2006 Oct;171(4):435-40. doi: 10.1016/j.plantsci.2006.05.005. Epub 2006 May 30.

Abstract

The enzyme encoded by the threonine deaminase (TD) gene catalyzes the conversion of threonine to α-keto butyrate in the biosynthesis of isoleucine (Ile). In Nicotiana attenuata, TD transcripts accumulate constitutively in cotyledons and flowers and are elicited in leaves by wounding, herbivore attack, and methyl jasmonic acid (MeJA) treatment. To understand TD's unique pattern of expression, we isolated a genomic clone of the TD gene from N. attenuata and characterized its promoter. T2 transgenic plants, each harboring single copies of fusions of different parts of the 5' non-coding region to the β-glucuronidase reporter gene, demonstrated that the promoter was constitutively expressed in seedlings and flowers, and elicited in leaves by wounding or by MeJA treatment. Promoter deletion analysis defined the promoter regions capable of directing minimal expression in cotyledons and anthers as -142 to -31bp, and in stigmas as -289 to -231bp. Regions from -142 to -31bp were found to be important for basal elicitation in leaves by both wounding and MeJA treatment. These promoter elements may prove valuable in biotechnological applications.

摘要

苏氨酸脱氨酶(TD)基因编码的酶在异亮氨酸(Ile)的生物合成中催化苏氨酸向α-酮丁酸的转化。在黄花烟草中,TD 转录本在子叶和花朵中持续积累,并在叶片中受到创伤、草食动物攻击和茉莉酸甲酯(MeJA)处理的诱导。为了了解 TD 独特的表达模式,我们从黄花烟草中分离出 TD 基因的基因组克隆,并对其启动子进行了特征分析。T2 转基因植物,每个都携带有不同 5'非编码区部分与β-葡萄糖醛酸酶报告基因的融合,证明启动子在幼苗和花朵中持续表达,并在叶片中受到创伤或 MeJA 处理的诱导。启动子缺失分析定义了能够在子叶和花药中指导最小表达的启动子区域为-142 至-31bp,在柱头中为-289 至-231bp。发现-142 至-31bp 区域对于叶片中创伤和 MeJA 处理的基础诱导非常重要。这些启动子元件在生物技术应用中可能具有重要价值。

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