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玉米丙酮酸、正磷酸二激酶基因中的顺式作用元件。

Cis-acting elements in the pyruvate, orthophosphate dikinase gene from maize.

作者信息

Matsuoka M, Numazawa T

机构信息

Department of Plant Physiology, National Institute of Agrobiological Resources, Ibaraki, Japan.

出版信息

Mol Gen Genet. 1991 Aug;228(1-2):143-52. doi: 10.1007/BF00282459.

DOI:10.1007/BF00282459
PMID:1653403
Abstract

To investigate the mechanisms that control expression of the gene for pyruvate, orthophosphate dikinase (PPDK) in maize, the 5' flanking region of the gene was analyzed for interactions with nuclear extracts. Gel retardation assays showed that there are several sites in the promoter region which bind to protein factors. In this report we describe further study of one of these sites, designated the PPD-1 binding site. The nuclear binding factor, PPD-1, is restricted to nuclear extracts from green leaves where the PPDK gene is expressed. No binding of PPD-1 was detected in tissues such as roots or etiolated leaves where the gene is not expressed in vivo. Gel retardation assays using deletion fragments from the promoter region and synthetic oligonucleotides, as well as exonuclease III protection assays, revealed that the site of PPD-1 binding lies between positions -301 and -296. To identify the functional role of the interaction between PPD-1 and its binding site, a deletion series of the promoter region was joined to a reporter gene, beta-glucuronidase. These constructs were introduced into green leaves of maize by microprojectile bombardment. Expression of the reporter gene occurred if the PPD-1 binding site remained in the promoter region of the chimeric genes but deletion of the binding site caused a drastic reduction in expression levels. These data indicate that interaction between PPD-1 and its binding site is essential for active transcription of the PPDK gene.

摘要

为了研究调控玉米中丙酮酸磷酸双激酶(PPDK)基因表达的机制,对该基因的5'侧翼区域进行了分析,以确定其与核提取物的相互作用。凝胶阻滞分析表明,启动子区域有多个位点与蛋白质因子结合。在本报告中,我们进一步研究了其中一个位点,即PPD - 1结合位点。核结合因子PPD - 1仅存在于PPDK基因表达的绿叶核提取物中。在根或黄化叶等该基因在体内不表达的组织中未检测到PPD - 1的结合。使用启动子区域的缺失片段和合成寡核苷酸进行凝胶阻滞分析,以及核酸外切酶III保护分析,结果表明PPD - 1的结合位点位于 - 301至 - 296位之间。为了确定PPD - 1与其结合位点之间相互作用的功能作用,将一系列启动子区域缺失片段与报告基因β - 葡萄糖醛酸酶连接。通过微粒轰击将这些构建体导入玉米绿叶中。如果PPD - 1结合位点保留在嵌合基因的启动子区域,则报告基因会表达,但结合位点的缺失会导致表达水平急剧下降。这些数据表明,PPD - 1与其结合位点之间的相互作用对于PPDK基因的活性转录至关重要。

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Plant Mol Biol. 1989 May;12(5):579-89. doi: 10.1007/BF00036971.
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Site-specific binding of a nuclear factor to the carrot extensin gene is influenced by both ethylene and wounding.
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