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光诱导豌豆AS1基因的转录抑制:顺式元件和反式作用因子的鉴定

Light-induced transcriptional repression of the pea AS1 gene: identification of cis-elements and transfactors.

作者信息

Ngai N, Tsai F Y, Coruzzi G

机构信息

New York University, Department of Biology, New York, NY 10003, USA.

出版信息

Plant J. 1997 Nov;12(5):1021-34. doi: 10.1046/j.1365-313x.1997.12051021.x.

DOI:10.1046/j.1365-313x.1997.12051021.x
PMID:9418044
Abstract

Here, we examine the cis-elements and trans-factors affecting the expression of asparagine synthetase (AS) genes whose transcription is negatively regulated by light. The promoters for the AS1 and AS2 genes of pea were isolated, sequenced, and functionally dissected for their ability to confer regulated expression to the GUS reporter gene in transgenic tobacco. Histochemical analysis of transgenic plants demonstrated that the AS1 and AS2 promoters show identical patterns of cell-specific expression. The more highly active AS1 promoter was further demonstrated to confer negative light-regulation to the GUS gene in transgenic tobacco. Deletion analysis and gain-of-function experiments showed that 124 bp of the AS1 promoter was sufficient to confer light-activated repression to a heterologous promoter. Potential conserved transcription regulatory elements, Box B, Box C, and Box C' within this region were shown to bind to nuclear proteins by gel shift analysis. A light-specific DNA:protein interaction was detected with Box B. The nuclear factors that bind to Box C and C' elements of AS1 are competed by a putative repressor element 'RE1' defined previously in the oat phytochrome gene whose transcription is also repressed by light. The Box B and C/C'-Box/RE1-binding factors were found in nuclear extracts of tobacco, pea, and Arabidopsis and may therefore be universal factors involved in light-activated transcriptional repression.

摘要

在此,我们研究了影响天冬酰胺合成酶(AS)基因表达的顺式元件和反式因子,这些基因的转录受到光的负调控。分离了豌豆AS1和AS2基因的启动子,对其进行测序,并对它们在转基因烟草中赋予GUS报告基因调控表达的能力进行了功能分析。对转基因植物的组织化学分析表明,AS1和AS2启动子表现出相同的细胞特异性表达模式。进一步证明,活性更高的AS1启动子在转基因烟草中赋予GUS基因负光调控。缺失分析和功能获得实验表明,AS1启动子的124 bp足以赋予异源启动子光激活抑制作用。通过凝胶迁移分析表明,该区域内潜在的保守转录调控元件Box B、Box C和Box C'与核蛋白结合。用Box B检测到光特异性的DNA:蛋白质相互作用。与AS1的Box C和C'元件结合的核因子被先前在燕麦光敏色素基因中定义的假定阻遏元件“RE1”竞争,该基因的转录也受到光的抑制。在烟草、豌豆和拟南芥的核提取物中发现了与Box B和C/C'-Box/RE1结合的因子,因此它们可能是参与光激活转录抑制的通用因子。

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