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长春花色氨酸脱羧酶基因的核苷酸序列及tdc - gusA基因融合体在烟草中的表达

Nucleotide sequence of the tryptophan decarboxylase gene of Catharanthus roseus and expression of tdc-gusA gene fusions in Nicotiana tabacum.

作者信息

Goddijn O J, Lohman F P, de Kam R J, Schilperoort R A, Hoge J H

机构信息

Institute of Molecular Plant Sciences, Leiden University, Clusius Laboratory, The Netherlands.

出版信息

Mol Gen Genet. 1994 Jan;242(2):217-25. doi: 10.1007/BF00391016.

DOI:10.1007/BF00391016
PMID:8159173
Abstract

The enzyme tryptophan decarboxylase (TDC; EC 4.1.1.28) converts tryptophan into tryptamine. In Catharanthus roseus and other plants capable of producing terpenoid indole alkaloids (TIAs) TDC links primary metabolism to the secondary metabolic pathway involved in the biosynthesis of these compounds. The accumulation of tdc mRNA in C. roseus cells is developmentally regulated and transcriptionally influenced by elicitors (induction) and auxins (repression). Here we report that TDC is encoded by a single copy gene in the C. roseus genome. No introns were observed upon isolation and sequencing of this gene. To study gene expression controlled by the tdc promoter, a 2 kb promoter fragment and a number of 5' deleted promoter derivatives were joined in translational fusion to a beta-D-glucuronidase reporter gene (gusA). Expression of the chimaeric constructs was monitored in stably transformed tobacco plants and in transiently transfected tobacco protoplasts. Histochemical and fluorimetric analysis of transgenic plants revealed that 1938 bp of the tdc promoter (with respect to the translational start codon) give rise to GUS activity in roots, stems and leaves. No tissue or cell type specificity was noted. Promoter deletions up to nucleotide -398 directed lower levels of gusA expression but conferred the same pattern of staining for GUS activity as the -1938 construct. Further deletion of the tdc promoter up to nucleotide -232 resulted in drastically reduced GUS activity levels and loss of GUS staining in all parts of the transgenic plants. In contrast to stable transformation, the -232 tdc-gusA construct gave rise to GUS activity levels comparable to those of the -398 construct in an assay system for transient expression in protoplasts.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

色氨酸脱羧酶(TDC;EC 4.1.1.28)可将色氨酸转化为色胺。在长春花和其他能够产生萜类吲哚生物碱(TIA)的植物中,TDC将初级代谢与参与这些化合物生物合成的次级代谢途径联系起来。长春花细胞中tdc mRNA的积累受到发育调控,并受到激发子(诱导)和生长素(抑制)的转录影响。在此,我们报道TDC由长春花基因组中的一个单拷贝基因编码。分离并测序该基因后未观察到内含子。为了研究由tdc启动子控制的基因表达,将一个2 kb的启动子片段和多个5'端缺失的启动子衍生物与β-D-葡萄糖醛酸酶报告基因(gusA)进行翻译融合。在稳定转化的烟草植株和瞬时转染的烟草原生质体中监测嵌合构建体的表达。对转基因植株的组织化学和荧光分析表明,tdc启动子的1938 bp(相对于翻译起始密码子)在根、茎和叶中产生GUS活性。未观察到组织或细胞类型特异性。直至核苷酸-398的启动子缺失导致gusA表达水平降低,但赋予与-1938构建体相同的GUS活性染色模式。tdc启动子进一步缺失至核苷酸-232导致转基因植株所有部位的GUS活性水平大幅降低且GUS染色消失。与稳定转化相反,在原生质体瞬时表达检测系统中,-232 tdc-gusA构建体产生的GUS活性水平与-398构建体相当。(摘要截短至250字)

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