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紫外线照射后酵母中的蛋白水解活性。II. DNA修复途径受阻的突变体中蛋白酶水平的变化。

Proteolytic activities in yeast after UV irradiation. II. Variation in proteinase levels in mutants blocked in DNA-repair pathways.

作者信息

Schwencke J, Moustacchi E

出版信息

Mol Gen Genet. 1982;185(2):296-301. doi: 10.1007/BF00330801.

Abstract

When the levels of three common yeast proteinases in exponentially growing cells of mutants blocked in different repair pathways are compared to that of isogenic wild-type cells, it can be seen that the level of proteinase B is enhanced in the mutants whereas the levels of leucin aminopeptidase (Leu.AP) and lysine aminopeptidase (Lys.AP) are similar in all strains. As in its corresponding wild type, the level of proteinase B activity is further enhanced after UV-irradiation in a mutant blocked in excision-repair (rad1-3). In contrast, following the same treatment the level of proteinase B remains almost constant in a mutant blocked in a general error-prone repair system (rad6-1) and in a mutant defective in a more specific mutagenic repair pathway (pso2-1). Cycloheximide, an inhibitor of protein synthesis, blocks the post-UV enhancement in proteinase B activity observed in rad1-3 indicating that, as in the wild-type cells, an inducible process is involved. The levels of Lys.AP and Leu.AP are, respectively, either unaffected or only moderately increased following UV-treatment of the repair defective mutants, as in wild-type strains. It is obvious that the induction of protease B activity following UV-treatment in Saccharomyces cannot be equated to the induction of the recA protein in Escherichia coli. However the correlation found between the block in mutagenic repair and the lack of UV-induction of protease B activity leads to questions on the possible role of certain protease activities in mutagenic repair in eucaryotic cells.

摘要

当将不同修复途径受阻的突变体在指数生长期细胞中的三种常见酵母蛋白酶水平与同基因野生型细胞的水平进行比较时,可以发现蛋白酶B的水平在突变体中有所提高,而亮氨酸氨肽酶(Leu.AP)和赖氨酸氨肽酶(Lys.AP)的水平在所有菌株中相似。与其相应的野生型一样,在切除修复受阻的突变体(rad1-3)中,紫外线照射后蛋白酶B的活性水平进一步提高。相反,经过相同处理后,在一般易错修复系统受阻的突变体(rad6-1)和在更特定的诱变修复途径有缺陷的突变体(pso2-1)中,蛋白酶B的水平几乎保持不变。蛋白质合成抑制剂环己酰亚胺可阻断rad1-3中观察到的紫外线照射后蛋白酶B活性的增强,这表明与野生型细胞一样,涉及一个诱导过程。与野生型菌株一样,修复缺陷突变体经紫外线处理后,Lys.AP和Leu.AP的水平分别不受影响或仅适度增加。显然,酿酒酵母经紫外线处理后蛋白酶B活性的诱导不能等同于大肠杆菌中recA蛋白的诱导。然而,在诱变修复受阻与蛋白酶B活性缺乏紫外线诱导之间发现的相关性引发了关于某些蛋白酶活性在真核细胞诱变修复中可能作用的问题。

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