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利用拟南芥中的pOp/LhG4反式激活系统从单个基因座可预测地激活组织特异性表达。

Predictable activation of tissue-specific expression from a single gene locus using the pOp/LhG4 transactivation system in Arabidopsis.

作者信息

Baroux Célia, Blanvillain Robert, Betts Hazel, Batoko Henri, Craft Judith, Martinez Alberto, Gallois Patrick, Moore Ian

机构信息

Laboratoire de Génome et Développement des Plantes, Université de Perpignan, 52 avenue de Villeneuve, 66860 Perpignan Cedex, France.

出版信息

Plant Biotechnol J. 2005 Jan;3(1):91-101. doi: 10.1111/j.1467-7652.2004.00104.x.

DOI:10.1111/j.1467-7652.2004.00104.x
PMID:17168902
Abstract

The pOp/LhG4 transcription factor system was used to determine whether the synthetic pOp promoter, integrated at one position in the Arabidopsis genome, could be efficiently and faithfully activated by the heterologous transcription factor, LhG4, expressed in a variety of different patterns. This is a precondition for the development and exploitation of large collections of LhG4 activation lines that direct predictable tissue-specific expression of transgenes. We selected a pOp-GUS reporter insertion that was efficiently activated after crossing to an activator line that expressed the synthetic transcription factor LhG4 from the Cauliflower Mosaic Virus 35S promoter. This reporter line, pOp-GUS(g2), was then combined with activator loci that expressed LhG4 from one of seven different promoters, each with a different tissue specificity. pOp-GUS(g2) was activated faithfully in combination with six of these seven activator constructs, but generated an unexpected expression pattern in combination with the seventh construct, a fusion to a cyclin promoter (CYC-LhG4). The aberrant expression pattern could be attributed to the pOp-GUS(g2) insertion site, as the CYC-LhG4 activator lines directed the expected pattern of expression from a second pOp-GUS insertion. These results show that it is feasible to construct an activator collection in which LhG4 is expressed from diverse promoters or enhancer traps, but that individual pOp reporter loci can vary in their competence to respond to certain activator patterns. We discuss the implications for the design and use of mis-expression technology in Arabidopsis.

摘要

利用pOp/LhG4转录因子系统来确定整合于拟南芥基因组中某一位置的合成pOp启动子是否能被以多种不同模式表达的异源转录因子LhG4有效且如实地激活。这是开发和利用大量LhG4激活系的前提条件,这些激活系可指导转基因的可预测组织特异性表达。我们选择了一个pOp-GUS报告基因插入系,当它与一个从花椰菜花叶病毒35S启动子表达合成转录因子LhG4的激活系杂交后能被有效激活。然后将这个报告系pOp-GUS(g2)与从七个不同启动子之一表达LhG4的激活位点组合,每个启动子具有不同的组织特异性。pOp-GUS(g2)与这七个激活构建体中的六个组合时能如实地被激活,但与第七个构建体(与细胞周期蛋白启动子的融合体CYC-LhG4)组合时产生了意外的表达模式。这种异常的表达模式可归因于pOp-GUS(g2)的插入位点,因为CYC-LhG4激活系从第二个pOp-GUS插入产生了预期的表达模式。这些结果表明构建一个激活系集合是可行的,其中LhG4从不同的启动子或增强子陷阱表达,但单个pOp报告基因位点对某些激活模式的响应能力可能会有所不同。我们讨论了这些结果对拟南芥中错误表达技术的设计和使用的影响。

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