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High-osmolarity signalling in Saccharomyces cerevisiae is modulated in a carbon-source-dependent fashion

机译:酿酒酵母中的高渗透压信号传导以碳源依赖的方式调节

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High-osmolarity-induced expression of the small heat-shock gene HSP12 is regulated by the HOG (high-osmolarity glycerol) pathway and PKA (protein kinase A). To analyse the regulatory input of both signal transduction pathways, high-salt-induced HSP12 expression in different genetic backgrounds on glucose-, ethanol- and glycerol-based culture media was examined. Upon exposure to high-osmolarity stress, the kinetics of induction of HSP12 in cells growing on the non-fermentable carbon sources are strikingly different from those on glucose. Derepression of HSP12 gene expression under non-stress conditions was observed in cells growing on non-fermentable carbon sources. High-salt challenge resulted in a lower induction of the HSP12 mRNA levels in ethanol-grown cells as compared to glucose-grown cells, whereas in glycerol-grown cells hardly any high-salt induction of HSP12 mRNA levels could be detected. Analysis of signalling through the HOG pathway suggested that glycerol may influence the activity of this signalling route, possibly via negative feedback. Furthermore, the cellular level of PKA activity was found to have a great impact on stress-responsive gene transcription. On the basis of the data obtained it was concluded that modulation of PKA activity plays a major role in the stress response. A glucose-dependent, PKA-regulated cellular component is postulated to affect high-osmolarity-induced HSP12 expression.
机译:小渗透性诱导的小型热休克基因Hsp12的表达由猪(高渗透甘油)途径和PKA(蛋白激酶A)调节。为了分析信号转导途径的调节性输入,研究了在不同遗传背景下的高盐诱导的HSP12表达在葡萄糖,乙醇和甘油基培养基上的不同遗传背景中。在暴露于高渗透压后,诱导Hsp12在不可发酵的碳源的细胞中诱导的动力学与葡萄糖的细胞中的尖锐区别不同。在不可发酵的碳源的细胞中观察到在非应激条件下的HSP12基因表达的DEREPLACE。与葡萄糖生长的电池相比,高盐攻击导致乙醇生长细胞中HSP12 mRNA水平的诱导诱导,而在甘油生长的细胞中几乎不能检测到HSP12 mRNA水平的任何高盐诱导。通过猪通路的信号传导的分析表明,甘油可能影响该信号路径的活动,可能通过负反馈。此外,发现PKA活性的细胞水平对应力响应基因转录产生很大影响。在获得的数据的基础上,得出结论认为PKA活动的调节在压力反应中起主要作用。依赖于葡萄糖PKA调节的细胞成分被假设以影响高渗透性诱导的HSP12表达。

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