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Deciphering Dynamic Dose Responses of Natural Promoters and Single cis Elements upon Osmotic and Oxidative Stress in Yeast

机译:酵母中天然启动子和单个顺式元素对渗透压和氧化应激的动态剂量反应的破译

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摘要

Fine-tuned activation of gene expression in response to stress is the result of dynamic interactions of transcription factors with specific promoter binding sites. In the study described here we used a time-resolved luciferase reporter assay in living Saccharomyces cerevisiae yeast cells to gain insights into how osmotic and oxidative stress signals modulate gene expression in a dose-sensitive manner. Specifically, the dose-response behavior of four different natural promoters (GRE2, CTT1, SOD2, and CCP1) reveals differences in their sensitivity and dynamics in response to different salt and oxidative stimuli. Characteristic dose-response profiles were also obtained for artificial promoters driven by only one type of stress-regulated consensus element, such as the cyclic AMP-responsive element, stress response element, or AP-1 site. Oxidative and osmotic stress signals activate these elements separately and with different sensitivities through different signaling molecules. Combination of stress-activated cis elements does not, in general, enhance the absolute expression levels; however, specific combinations can increase the inducibility of the promoter in response to different stress doses. Finally, we show that the stress tolerance of the cell critically modulates the dynamics of its transcriptional response in the case of oxidative stress.
机译:响应压力而微调的基因表达激活是转录因子与特定启动子结合位点动态相互作用的结果。在本文所述的研究中,我们在活酿酒酵母酵母细胞中使用了时间分辨的荧光素酶报告基因检测法,以了解渗透压和氧化应激信号如何以剂量敏感性方式调节基因表达。具体来说,四种不同的自然启动子( GRE2 CTT1 SOD2 CCP1 )的剂量反应行为揭示了它们对不同盐和氧化刺激的敏感性和动力学差异。还获得了仅由一种类型的应激调节共有元件(例如环状AMP应答元件,应激反应元件或AP-1位点)驱动的人工启动子的特征性剂量反应曲线。氧化和渗透应激信号分别激活这些元素,并通过不同的信号分子以不同的敏感性激活。应力激活的 cis 元素的组合通常不会提高绝对表达水平;但是,特定的组合可以增加启动子对不同应激剂量的诱导能力。最后,我们表明,在氧化应激的情况下,细胞的应激耐受性会关键地调节其转录反应的动力学。

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