{"title":"利用新生成的拟南芥转基因植物分析温度对 FT-FD 模块蛋白质积累的影响。","authors":"Kyung-Ho Park, Sol-Bi Kim, Jae-Hoon Jung","doi":"10.1002/pld3.552","DOIUrl":null,"url":null,"abstract":"<p><p>Arabidopsis flowering is dependent on interactions between a component of the florigens FLOWERING LOCUS T (FT) and the basic leucine zipper (bZIP) transcription factor FD. These proteins form a complex that activates the genes required for flowering competence and integrates environmental cues, such as photoperiod and temperature. However, it remains largely unknown how FT and FD are regulated at the protein level. To address this, we created <i>FT</i> transgenic plants that express the N-terminal FLAG-tagged FT fusion protein under the control of its own promoter in <i>ft</i> mutant backgrounds. <i>FT</i> transgenic plants complemented the delayed flowering of the <i>ft</i> mutant and exhibited similar <i>FT</i> expression patterns to wild-type Col-0 plants in response to changes in photoperiod and temperature. Similarly, we generated <i>FD</i> transgenic plants in <i>fd</i> mutant backgrounds that express the N-terminal MYC-tagged FD fusion protein under the <i>FD</i> promoter, rescuing the late flowering phenotypes in the <i>fd</i> mutant. Using these transgenic plants, we investigated how temperature regulates the expression of FT and FD proteins. Temperature-dependent changes in FT and FD protein levels are primarily regulated at the transcript level, but protein-level temperature effects have also been observed to some extent. In addition, our examination of the expression patterns of FT and FD in different tissues revealed that similar to the spatial expression pattern of <i>FT</i>, <i>FD</i> mRNA was expressed in both the leaf and shoot apex, but FD protein was only detected in the apex, suggesting a regulatory mechanism that restricts FD protein expression in the leaf during the vegetative growth phase. 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These proteins form a complex that activates the genes required for flowering competence and integrates environmental cues, such as photoperiod and temperature. However, it remains largely unknown how FT and FD are regulated at the protein level. To address this, we created <i>FT</i> transgenic plants that express the N-terminal FLAG-tagged FT fusion protein under the control of its own promoter in <i>ft</i> mutant backgrounds. <i>FT</i> transgenic plants complemented the delayed flowering of the <i>ft</i> mutant and exhibited similar <i>FT</i> expression patterns to wild-type Col-0 plants in response to changes in photoperiod and temperature. Similarly, we generated <i>FD</i> transgenic plants in <i>fd</i> mutant backgrounds that express the N-terminal MYC-tagged FD fusion protein under the <i>FD</i> promoter, rescuing the late flowering phenotypes in the <i>fd</i> mutant. Using these transgenic plants, we investigated how temperature regulates the expression of FT and FD proteins. Temperature-dependent changes in FT and FD protein levels are primarily regulated at the transcript level, but protein-level temperature effects have also been observed to some extent. In addition, our examination of the expression patterns of FT and FD in different tissues revealed that similar to the spatial expression pattern of <i>FT</i>, <i>FD</i> mRNA was expressed in both the leaf and shoot apex, but FD protein was only detected in the apex, suggesting a regulatory mechanism that restricts FD protein expression in the leaf during the vegetative growth phase. 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引用次数: 0
摘要
拟南芥开花依赖于花原基花序定位点 T(FT)的一个组成部分与碱性亮氨酸拉链(bZIP)转录因子 FD 之间的相互作用。这些蛋白质形成一个复合体,激活开花能力所需的基因,并整合光周期和温度等环境线索。然而,人们对 FT 和 FD 如何在蛋白质水平上进行调控仍然知之甚少。为了解决这个问题,我们创建了FT转基因植株,在ft突变体背景下,在其自身启动子的控制下表达N-末端FLAG标记的FT融合蛋白。FT 转基因植株补充了ft突变体延迟开花的缺陷,并在光周期和温度变化时表现出与野生型 Col-0 植株相似的 FT 表达模式。同样,我们在 fd 突变体背景中产生了 FD 转基因植株,它们在 FD 启动子下表达 N 端 MYC 标记的 FD 融合蛋白,从而挽救了 fd 突变体的延迟开花表型。利用这些转基因植物,我们研究了温度如何调控 FT 和 FD 蛋白的表达。随温度变化的 FT 和 FD 蛋白水平主要受转录本水平的调控,但也在一定程度上观察到了蛋白质水平的温度效应。此外,我们对 FT 和 FD 在不同组织中的表达模式进行的研究发现,与 FT 的空间表达模式类似,FD mRNA 在叶片和嫩枝先端均有表达,但 FD 蛋白仅在先端被检测到,这表明存在一种调控机制,即在无性生长阶段限制 FD 蛋白在叶片中的表达。这些转基因植物为研究 FT-FD 模块在花期调控中的作用提供了一个宝贵的平台。
Analysis of temperature effects on the protein accumulation of the FT-FD module using newly generated Arabidopsis transgenic plants.
Arabidopsis flowering is dependent on interactions between a component of the florigens FLOWERING LOCUS T (FT) and the basic leucine zipper (bZIP) transcription factor FD. These proteins form a complex that activates the genes required for flowering competence and integrates environmental cues, such as photoperiod and temperature. However, it remains largely unknown how FT and FD are regulated at the protein level. To address this, we created FT transgenic plants that express the N-terminal FLAG-tagged FT fusion protein under the control of its own promoter in ft mutant backgrounds. FT transgenic plants complemented the delayed flowering of the ft mutant and exhibited similar FT expression patterns to wild-type Col-0 plants in response to changes in photoperiod and temperature. Similarly, we generated FD transgenic plants in fd mutant backgrounds that express the N-terminal MYC-tagged FD fusion protein under the FD promoter, rescuing the late flowering phenotypes in the fd mutant. Using these transgenic plants, we investigated how temperature regulates the expression of FT and FD proteins. Temperature-dependent changes in FT and FD protein levels are primarily regulated at the transcript level, but protein-level temperature effects have also been observed to some extent. In addition, our examination of the expression patterns of FT and FD in different tissues revealed that similar to the spatial expression pattern of FT, FD mRNA was expressed in both the leaf and shoot apex, but FD protein was only detected in the apex, suggesting a regulatory mechanism that restricts FD protein expression in the leaf during the vegetative growth phase. These transgenic plants provided a valuable platform for investigating the role of the FT-FD module in flowering time regulation.
期刊介绍:
Plant Direct is a monthly, sound science journal for the plant sciences that gives prompt and equal consideration to papers reporting work dealing with a variety of subjects. Topics include but are not limited to genetics, biochemistry, development, cell biology, biotic stress, abiotic stress, genomics, phenomics, bioinformatics, physiology, molecular biology, and evolution. A collaborative journal launched by the American Society of Plant Biologists, the Society for Experimental Biology and Wiley, Plant Direct publishes papers submitted directly to the journal as well as those referred from a select group of the societies’ journals.