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Isolation of Saccharomyces cerevisiae mutants constitutive for invertase synthesis.

机译:构成转化酶合成的酿酒酵母突变体的分离。

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A new method for detecting invertase activity in Saccharomyces cerevisiae colonies was used to screen for mutants resistant to catabolite repression of invertase. Mutations causing the highest level of derepression were located in two previously identified genes, cyc8 and tup1. Several of the cyc8 mutations, notably cyc8-10 and cyc8-11, were temperature dependent, repressed at 23 degrees C, and derepressed at 37 degrees C. The kinetics of derepression of invertase mRNA in cyc8-10 cells shifted from 23 to 37 degrees C was determined by Northern blots. Invertase mRNA was detectable at 5 min after the shift, with kinetics of accumulation very similar to that of wild-type cells shifted from high-glucose to low-glucose medium. Assays of representative enzymes showed that many but not all glucose-repressible enzymes are derepressed in both cyc8 and tup1 mutants. cyc8 and tup1 appear to be the major negative regulatory genes controlling catabolite repression in yeasts.
机译:一种用于检测酿酒酵母菌落中转化酶活性的新方法用于筛选对转化酶的分解代谢阻遏有抗性的突变体。引起最高抑制水平的突变位于两个先前鉴定的基因cyc8和tup1中。几个cyc8突变,特别是cyc8-10和cyc8-11,是温度依赖性的,在23°C时受到抑制,在37°C时受到抑制。cyc8-10细胞中转化酶mRNA抑制的动力学从23转变为37度。 C通过Northern印迹确定。转移后5分钟可检测到转化酶mRNA,其累积动力学与野生型细胞从高葡萄糖培养基转移至低葡萄糖培养基非常相似。代表性酶的分析表明,cyc8和tup1突变体均抑制了许多但不是全部的葡萄糖可抑制酶。 cyc8和tup1似乎是控制酵母中分解代谢物阻遏的主要负调控基因。

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