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UBI4是酿酒酵母的多聚泛素基因,是一个热休克基因,同时也受分解代谢物阻遏解除的调控。

UBI4, the polyubiquitin gene of Saccharomyces cerevisiae, is a heat shock gene that is also subject to catabolite derepression control.

作者信息

Watt R, Piper P W

机构信息

Department of Biochemistry and Molecular Biology, University College London, UK.

出版信息

Mol Gen Genet. 1997 Jan 27;253(4):439-47. doi: 10.1007/s004380050341.

DOI:10.1007/s004380050341
PMID:9037103
Abstract

Carbon and nitrogen regulation of UBI4, the stress-inducible polyubiquitin gene of Saccharomyces cerevisiae, was investigated using a UBI4 promoter-LacZ fusion gene (UBI4-LacZ). Expression of this gene in cells grown on different media indicated that the UBI4 promoter is more active during growth on respiratory than on fermentable carbon sources but is not subject to appreciable control by nitrogen catabolite repression. UBI4-LacZ expression was virtually identical in cells having constitutively high (ras2, sra1-13) or constitutively low (ras2) levels of cyclic AMP-dependent protein kinase activity, indicating that this kinase does not exert a major influence on UBI4 expression. Catabolite derepression control of the UBI4 promoter was confirmed by measurements of UBI4-LacZ expression in hap mutant and wild-type strains before and after transfer from glucose to lactate. Mutagenesis of the perfect consensus for HAP2/3/4 complex binding at position -542 resulted in considerable reduction of UBI4 promoter derepression with respiratory adaptation in HAP wild-type cells and abolished the reduced UBI4-LacZ derepression normally seen when aerobic cultures of the hap1 mutant are transferred from glucose to lactate. This HAP2/3/4 binding site is therefore a major element contributing to catabolite derepression of the UBI4 promoter, although data obtained with hapl mutant cells indicated that HAP1 also contributes to this derepression. The HAP2/3/4 and HAP1 systems are normally found to activate genes for mitochondrial (respiratory) functions. Their involvement in mediating higher activity of the UBI4 promoter during respiratory growth may reflect the contribution of UBI4 expression to tolerance of oxidative stress.

摘要

利用泛素4启动子-LacZ融合基因(UBI4-LacZ),对酿酒酵母应激诱导型多聚泛素基因UBI4的碳氮调节进行了研究。该基因在不同培养基上生长的细胞中的表达表明,UBI4启动子在呼吸性碳源上生长时比在可发酵碳源上生长时更活跃,但不受氮代谢物阻遏的明显调控。在具有组成型高(ras2,sra1-13)或组成型低(ras2)水平的环磷酸腺苷依赖性蛋白激酶活性的细胞中,UBI4-LacZ表达几乎相同,这表明该激酶对UBI4表达没有主要影响。通过测量从葡萄糖转移到乳酸前后hap突变体和野生型菌株中UBI4-LacZ的表达,证实了UBI4启动子的分解代谢物去阻遏调控。对位于-542位置的HAP2/3/4复合物结合的完美共有序列进行诱变,导致HAP野生型细胞在呼吸适应时UBI4启动子去阻遏显著降低,并消除了hap1突变体需氧培养物从葡萄糖转移到乳酸时通常出现的UBI4-LacZ去阻遏降低现象。因此,这个HAP2/3/4结合位点是导致UBI4启动子分解代谢物去阻遏的主要元件,尽管用hap1突变体细胞获得的数据表明HAP1也参与了这种去阻遏。通常发现HAP2/3/4和HAP1系统可激活线粒体(呼吸)功能的基因。它们参与介导呼吸生长期间UBI4启动子的更高活性,可能反映了UBI4表达对氧化应激耐受性的贡献。

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