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CpR18是一种新型的含SAP结构域的植物转录因子,它与来自复苏植物粉花苣苔(Craterostigma plantagineum Hochst.)的CDeT27 - 45基因的ABA介导表达所必需的启动子区域结合。

CpR18, a novel SAP-domain plant transcription factor, binds to a promoter region necessary for ABA mediated expression of the CDeT27-45 gene from the resurrection plant Craterostigma plantagineum Hochst.

作者信息

Hilbricht Tobias, Salamini Francesco, Bartels Dorothea

机构信息

Max-Planck-Institut für Züchtungsforschung, Carl-von-Linné-Weg 10, D-50829 Köln, Germany.

出版信息

Plant J. 2002 Aug;31(3):293-303. doi: 10.1046/j.1365-313x.2002.01357.x.

Abstract

CDeT27-45 is a lea-like gene from the resurrection plant Craterostigma plantagineum (Scrophulariaceae) which is strongly expressed in vegetative tissues in response to dehydration or treatment with abscisic acid (ABA). Expression of the gene is correlated with the acquisition of desiccation tolerance. Nuclear proteins bind to a 29-bp cis-regulatory region of the promoter which is essential for transcriptional activation of the CDeT27-45 gene by ABA. Using a yeast one-hybrid screen, the cDNA clone CpR18 was isolated, which encodes a protein with specific binding activity for the cis-regulatory element in the CDeT27-45 promoter. The protein contains an acidic region, a SAP-domain, a zinc finger of the C3H-type, and two motifs which are conserved in proteins from several plant species. One of the conserved regions is rich in basic residues and is predicted to form a helix-loop-helix structure. The R18 gene shows high similarities to genomic sequences and ESTs from other plant species. The tissue-specific expression pattern of the rare R18 mRNA and the distribution of nuclear protein binding activity for the CDeT27-45 promoter fragment are compared. The R18 protein is indeed localized in the nucleus, and activates transcription of CDeT27-45 promoter-GUS fusion constructs in tobacco protoplasts. DNA blot analysis and isolation of genomic clones reveal that two copies of R18 are present in the C. plantagineum genome.

摘要

CDeT27 - 45是来自复苏植物车前叶蓝蓟(玄参科)的一个类lea基因,在营养组织中,它会因脱水或脱落酸(ABA)处理而强烈表达。该基因的表达与获得耐干燥性相关。核蛋白与启动子的一个29 bp顺式调控区域结合,该区域对于ABA对CDeT27 - 45基因的转录激活至关重要。通过酵母单杂交筛选,分离出了cDNA克隆CpR18,它编码一种对CDeT27 - 45启动子中的顺式调控元件具有特异性结合活性的蛋白质。该蛋白质包含一个酸性区域、一个SAP结构域、一个C3H型锌指以及在几种植物物种的蛋白质中保守的两个基序。其中一个保守区域富含碱性残基,预计会形成螺旋 - 环 - 螺旋结构。R18基因与其他植物物种的基因组序列和EST具有高度相似性。比较了稀有R18 mRNA的组织特异性表达模式以及CDeT27 - 45启动子片段的核蛋白结合活性分布。R18蛋白确实定位于细胞核中,并在烟草原生质体中激活CDeT27 - 45启动子 - GUS融合构建体的转录。DNA印迹分析和基因组克隆的分离表明,车前叶蓝蓟基因组中存在两个R18拷贝。

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