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Transient and stable expression of the firefly luciferase gene in plant cells and transgenic plants.在植物细胞和转基因植物中萤火虫荧光素酶基因的瞬时和稳定表达。
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Transient expression of chimeric genes delivered into pollen by microprojectile bombardment.花粉管通道介导的花粉管中瞬时表达嵌合基因。
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Functional regions of the cauliflower mosaic virus 35S RNA promoter determined by use of the firefly luciferase gene as a reporter of promoter activity.利用萤火虫荧光素酶基因作为启动子活性的报告基因鉴定花椰菜花叶病毒 35S RNA 启动子的功能区。
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Tissue-Specific Expression of as-1 in Transgenic Tobacco.as-1在转基因烟草中的组织特异性表达
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A 22-bp fragment of the pea lectin promoter containing essential TGAC-like motifs confers seed-specific gene expression.含有必需的类TGAC基序的豌豆凝集素启动子的一个22碱基对片段赋予种子特异性基因表达。
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Molecular cloning of the olfactory neuronal transcription factor Olf-1 by genetic selection in yeast.通过酵母中的遗传筛选对嗅觉神经元转录因子Olf-1进行分子克隆。
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8
The transcriptional activator Opaque2 recognizes two different target sequences in the 22-kD-like alpha-prolamin genes.转录激活因子不透明2在类22-kDα-醇溶蛋白基因中识别两种不同的靶序列。
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10
Separate cis sequences and trans factors direct metabolic and developmental regulation of a potato tuber storage protein gene.不同的顺式作用序列和反式作用因子指导马铃薯块茎贮藏蛋白基因的代谢与发育调控。
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花粉特异性元件存在于两个花粉表达基因近端启动子的30个碱基对中。

Pollen specificity elements reside in 30 bp of the proximal promoters of two pollen-expressed genes.

作者信息

Eyal Y, Curie C, McCormick S

机构信息

Plant Gene Expression Center, United States Department of Agriculture-Agricultural Research Service, Albany.

出版信息

Plant Cell. 1995 Mar;7(3):373-84. doi: 10.1105/tpc.7.3.373.

DOI:10.1105/tpc.7.3.373
PMID:7734969
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC160789/
Abstract

Functional analyses previously identified minimal promoter regions required for maintaining high-level expression of the late anther tomato LAT52 and LAT59 genes in tomato pollen. Here, we now define elements that direct pollen specificity. We used a transient assay system consisting of two cell types that differentially express the LAT genes and both "loss-of-function" and "gain-of-function" approaches. Linker substitution mutants analyzed in the transient assay and in transgenic plants identified 30-bp proximal promoter regions of LAT52 and LAT59 that are essential for their expression in pollen and that confer pollen specificity when fused to the heterologous cauliflower mosaic virus 35S core promoter. In vivo competition experiments demonstrated that a common trans-acting factor interacts with the pollen specificity region of both LAT gene promoters and suggested that a common mechanism regulates their coordinate expression. Adjacent upstream elements, the 52/56 box in LAT52 and the 56/59 box in LAT59, are involved in modulating the level of expression in pollen. The 52/56 box may be a target for the binding of a member of the GT-1 transcription factor family.

摘要

功能分析先前已确定了维持番茄花粉中晚期花药番茄LAT52和LAT59基因高水平表达所需的最小启动子区域。在此,我们现在定义了指导花粉特异性的元件。我们使用了一个由两种差异表达LAT基因的细胞类型组成的瞬时分析系统,以及“功能丧失”和“功能获得”方法。在瞬时分析和转基因植物中分析的接头取代突变体确定了LAT52和LAT59的30 bp近端启动子区域,这些区域对于它们在花粉中的表达至关重要,并且当与异源花椰菜花叶病毒35S核心启动子融合时赋予花粉特异性。体内竞争实验表明,一个共同的反式作用因子与两个LAT基因启动子的花粉特异性区域相互作用,并表明一种共同机制调节它们的协同表达。相邻的上游元件,LAT52中的52/56框和LAT59中的56/59框,参与调节花粉中的表达水平。52/56框可能是GT-1转录因子家族成员结合的靶标。