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烟草咖啡酸 O-甲基转移酶(COMT)II 基因的结构:参与多种刺激诱导基因表达的启动子序列的鉴定。

Structure of the tobacco caffeic acid O-methyltransferase (COMT) II gene: identification of promoter sequences involved in gene inducibility by various stimuli.

作者信息

Toquin Valérie, Grausem Bernard, Geoffroy Pierrette, Legrand Michel

机构信息

Institut de Biologie Moléculaire des Plantes du CNRS, UPR 2357, Université Louis Pasteur, 12, rue du Général Zimmer, 67000 Strasbourg, France.

出版信息

Plant Mol Biol. 2003 Jun;52(3):495-509. doi: 10.1023/a:1024810916909.

Abstract

The tobacco gene encoding caffeic acid-O-methyltransferase of class II (COMT II) was isolated, including a 1.7 kb 5'-flanking region. Sequence motifs were identified in COMT II gene promoter which are present in many genes of the phenylpropanoid pathway or in stress-inducible pathogenesis-related (PR) genes. A 1215 bp COMT II promoter fragment was transcriptionally fused to the GUS coding region and its activity pattern studied by stable expression of the fusion gene in tobacco. Transgenic lines were analysed for GUS and OMT activities upon infection, UV irradiation, wounding and treatment by various signalling compounds. The promoter proved responsive to various biotic and abiotic elicitors and to infection by avirulent and virulent pathogens. During the course of the hypersensitive reaction of tobacco to TMV two peaks were detected, an early one induced by the inoculation process and a second one at the onset of lesion formation. Parallel changes were observed between GUS activity that reflected the activity of the COMT II promoter fragment and COMT II activity that mirrored expression of the endogenous COMT II gene, indicating that COMT II pattern of expression is established at the transcriptional level. Various promoter fragments were fused to the GUS gene and revealed that gene induction by MeJA or UV and by TMV or wounding requires different sequences included in a 74 bp fragment. When the 74 bp sequence was multimerized and inserted ahead of the CaMV 35S RNA minimal promoter, one construct was shown to be capable of driving expression of the reporter gene around the TMV-infected sites in transgenic tobacco plants.

摘要

分离出了编码II类咖啡酸-O-甲基转移酶(COMT II)的烟草基因,包括一个1.7 kb的5'侧翼区域。在COMT II基因启动子中鉴定出了序列基序,这些基序存在于许多苯丙烷类途径的基因或应激诱导的病程相关(PR)基因中。将一个1215 bp的COMT II启动子片段与GUS编码区进行转录融合,并通过融合基因在烟草中的稳定表达来研究其活性模式。分析了转基因株系在感染、紫外线照射、创伤以及用各种信号化合物处理后的GUS和OMT活性。结果表明,该启动子对各种生物和非生物激发子以及无毒和有毒病原体的感染均有响应。在烟草对烟草花叶病毒(TMV)的过敏反应过程中检测到两个峰值,一个是由接种过程诱导的早期峰值,另一个是在病斑形成开始时出现的峰值。反映COMT II启动子片段活性的GUS活性与反映内源性COMT II基因表达的COMT II活性之间观察到平行变化,表明COMT II的表达模式是在转录水平上建立的。将各种启动子片段与GUS基因融合,结果显示茉莉酸甲酯(MeJA)或紫外线以及TMV或创伤诱导的基因表达需要一个74 bp片段中包含的不同序列。当将74 bp序列多聚化并插入到花椰菜花叶病毒(CaMV)35S RNA最小启动子之前时,其中一个构建体能够驱动转基因烟草植株中报告基因在TMV感染部位周围的表达。

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