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利用改良的酵母单杂交系统分离出一类新型bZIP转录因子,这些转录因子与Dc3启动子中的ABA响应元件和胚胎特异性元件相互作用。

Isolation of a novel class of bZIP transcription factors that interact with ABA-responsive and embryo-specification elements in the Dc3 promoter using a modified yeast one-hybrid system.

作者信息

Kim S Y, Chung H J, Thomas T L

机构信息

Department of Biology, Texas A&M University, College Station 77843-3258, USA.

出版信息

Plant J. 1997 Jun;11(6):1237-51. doi: 10.1046/j.1365-313x.1997.11061237.x.

DOI:10.1046/j.1365-313x.1997.11061237.x
PMID:9225465
Abstract

Dc3 is a carrot lea class gene that is abundantly expressed during somatic and zygotic embryogenesis. Its expression is normally embryo-specific and also can be induced by abscisic acid. The regulatory elements mediating the embryo-specific expression of Dc3 reside within the proximal promoter region (-117 to +26), which is also essential for ABA-induced expression. In this study, an optimized version of the yeast one-hybrid system has been used to clone factors that bind to the promoter region of the Dc3 gene. Twenty-five million yeast transformants were screened in a single experiment, and nine independent cDNA clones were isolated from a sunflower library that encode proteins that specifically bind to functional cis-regulatory elements in the Dc3 promoter. Analysis of these clones showed that they are derived from three different mRNA species that encode two basic leucine zipper proteins. The basic regions of these proteins, named DPBF-1 and 2 (Dc3 Promoter-Binding Factor-1 and 2), respectively, are nearly identical to each other and are similar to the plant G-box binding factor GBF-4. Outside the basic region, however, DPBF-1 and 2 diverge significantly from each other and from other known factors. Both factors have transcriptional activity in yeast, and bind to DNA as dimers. Unlike other plant bZIP factors, DPBF-1 and 2 recognize sequences containing the ACACNNG core. Cloning of these factors demonstrates the power of the one-hybrid approach when optimally applied.

摘要

Dc3是一种胡萝卜lea类基因,在体细胞胚和合子胚发生过程中大量表达。其表达通常具有胚胎特异性,也可由脱落酸诱导。介导Dc3胚胎特异性表达的调控元件位于近端启动子区域(-117至+26)内,该区域对脱落酸诱导的表达也至关重要。在本研究中,优化后的酵母单杂交系统被用于克隆与Dc3基因启动子区域结合的因子。在一次实验中筛选了2500万个酵母转化体,并从向日葵文库中分离出9个独立的cDNA克隆,这些克隆编码的蛋白质能特异性结合Dc3启动子中的功能性顺式调控元件。对这些克隆的分析表明,它们来自三种不同的mRNA种类,编码两种碱性亮氨酸拉链蛋白。这些蛋白质的碱性区域分别命名为DPBF-1和2(Dc3启动子结合因子-1和2),彼此几乎相同,且与植物G-box结合因子GBF-4相似。然而,在碱性区域之外,DPBF-1和2彼此以及与其他已知因子有很大差异。这两种因子在酵母中都具有转录活性,并以二聚体形式与DNA结合。与其他植物bZIP因子不同,DPBF-1和2识别含有ACACNNG核心的序列。这些因子的克隆证明了单杂交方法在最佳应用时的强大功能。

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