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Functional distinctions between yeast TATA elements.   总被引:28,自引:18,他引:10       下载免费PDF全文
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Ecdysteroid signaling in insects is transduced by a heterodimer of the EcR and USP nuclear receptors. In order to monitor the temporal and spatial patterns of ecdysteroid signaling in vivo we established transgenic animals that express a fusion of the GAL4 DNA binding domain and the ligand binding domain (LBD) of EcR or USP, combined with a GAL4-dependent lacZ reporter gene. The patterns of beta-galactosidase expression in these animals indicate where and when the GAL4-LBD fusion protein has been activated by its ligand in vivo. We show that the patterns of GAL4-EcR and GAL4-USP activation at the onset of metamorphosis reflect what would be predicted for ecdysteroid activation of the EcR/USP heterodimer. No activation is seen in mid-third instar larvae when the ecdysteroid titer is low, and strong widespread activation is observed at the end of the instar when the ecdysteroid titer is high. In addition, both GAL4-EcR and GAL4-USP are activated in larval organs cultured with 20-hydroxyecdysone (20E), consistent with EcR/USP acting as a 20E receptor. We also show that GAL4-USP activation depends on EcR, suggesting that USP requires its heterodimer partner to function as an activator in vivo. Interestingly, we observe no GAL4-LBD activation in the imaginal discs and ring glands of late third instar larvae. Addition of 20E to cultured mid-third instar imaginal discs results in GAL4-USP activation, but this response is not seen in imaginal discs cultured from late third instar larvae, suggesting that EcR/USP loses its ability to function as an efficient activator in this tissue. We conclude that EcR/USP activation by the systemic ecdysteroid signal may be spatially restricted in vivo. Finally, we show that GAL4-EcR functions as a potent and specific dominant negative at the onset of metamorphosis, providing a new tool for characterizing ecdysteroid signaling pathways during development.  相似文献   

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酵母PHO2与PHO4蛋白的激活活性的分析及两者的相互作用   总被引:3,自引:3,他引:0  
PHO2与PHO4是酵母PHO5基因的两个正调控因子,本文发现,PHO2与酵母转录因子GAL4的DNA结合功能域融合后就能激活报道基因lacZ的表达,其激活力受高低磷影响,表明PHO2蛋白上存在酸性转录激活区。PHO2蛋白上酸性氨基酸丰富的287-326肽段并非PHO2的激活区。在PHO2蛋白上230位Ser处于磷酸化状态2PHO2才有激活作用,表明了这一磷酸化位点可能与PHO2的转录激活能力有关  相似文献   

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