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烟草过氧化物酶基因tpoxN1血管系统特异性表达的一种新型伤口响应顺式元件VWRE。

A novel wound-responsive cis-element, VWRE, of the vascular system-specific expression of a tobacco peroxidase gene, tpoxN1.

作者信息

Sasaki Katsutomo, Ito Hiroyuki, Mitsuhara Ichiro, Hiraga Susumu, Seo Shigemi, Matsui Hirokazu, Ohashi Yuko

机构信息

Division of Plant Sciences, Organization of National Institute of Agrobiological Sciences, Tsukuba, Ibaraki 305-8602, Japan.

出版信息

Plant Mol Biol. 2006 Nov;62(4-5):753-68. doi: 10.1007/s11103-006-9055-5. Epub 2006 Aug 29.

Abstract

The wound-induced expression of tpoxN1, encoding a tobacco peroxidase, is unique because of its vascular system-specific expression and insensitivity to known wound-signal compounds such as jasmonic acid, ethylene, and plant hormones [Sasaki et al. (2002) Plant Cell Physiol 43:108-117]. To study the mechanism of expression, the 2-kbp tpoxN1 promoter region and successive 5'-deletion of the promoter were introduced as GUS fusion genes into tobacco plants. Analysis of GUS activity in transgenic plants indicated that a vascular system-specific and wound-responsive cis-element (VWRE) is present at the -239/-200 region of the promoter. Gel mobility shift assays suggested that a nuclear factor(s) prepared from wounded tobacco stems binds a 14-bp sequence (-229/-215) in the -239/-200 region in a sequence-specific manner. A mutation in this 14-bp region of the -239 promoter fragment resulted in a considerable decrease in wound-responsive GUS activity in transgenic plants. An 11-bp sequence, which completely overlaps with the 14-bp sequence, was found in the 5' distal region (-420/-410) and is thought to contribute to the wound-induced expression together with the 14-bp. The -114-bp core promoter of the tpoxN1 gene was indispensable for wound-induced expression, indicating that the 14-bp region is a novel wound-responsive cis-element VWRE, which may work cooperatively with other factors in the promoter.

摘要

编码烟草过氧化物酶的tpoxN1在伤口诱导下的表达具有独特性,这是因为它在维管系统中特异性表达,并且对茉莉酸、乙烯等已知的伤口信号化合物以及植物激素不敏感[Sasaki等人(2002年),《植物细胞生理学》43:108 - 117]。为了研究其表达机制,将2千碱基对的tpoxN1启动子区域以及启动子的连续5'端缺失片段作为GUS融合基因导入烟草植株。对转基因植株中GUS活性的分析表明,在启动子的 - 239 / - 200区域存在一个维管系统特异性且对伤口有响应的顺式作用元件(VWRE)。凝胶迁移率变动分析表明,从受伤烟草茎中制备的一种核因子以序列特异性方式结合在 - 239 / - 200区域中的一个14碱基序列( - 229 / - 215)上。 - 239启动子片段中这个14碱基区域的突变导致转基因植株中伤口响应性GUS活性大幅下降。在5'端远端区域( - 420 / - 410)发现了一个与该14碱基序列完全重叠的11碱基序列,并且认为它与14碱基序列一起对伤口诱导的表达有贡献。tpoxN1基因的 - 114碱基核心启动子对于伤口诱导的表达是必不可少的,这表明14碱基区域是一个新的伤口响应性顺式作用元件VWRE,它可能与启动子中的其他因子协同作用。

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