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The PEP4 gene encodes an aspartyl protease implicated in the posttranslational regulation of Saccharomyces cerevisiae vacuolar hydrolases.

机译:PEP4基因编码一个天冬氨酰蛋白酶参与了酿酒酵母液泡水解酶的翻译后调控。

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摘要

pep4 mutants of Saccharomyces cerevisiae accumulate inactive precursors of vacuolar hydrolases. The PEP4 gene was isolated from a genomic DNA library by complementation of the pep4-3 mutation. Deletion analysis localized the complementing activity to a 1.5-kilobase pair EcoRI-XhoI restriction enzyme fragment. This fragment was used to identify an 1,800-nucleotide mRNA capable of directing the synthesis of a 44,000-dalton polypeptide. Southern blot analysis of yeast genomic DNA showed that the PEP4 gene is unique; however, several related sequences exist in yeasts. Tetrad analysis and mitotic recombination experiments localized the PEP4 gene proximal to GAL4 on chromosome XVI. Analysis of the DNA sequence indicated that PEP4 encodes a polypeptide with extensive homology to the aspartyl protease family. A comparison of the PEP4 predicted amino acid sequence with the yeast protease A protein sequence revealed that the two genes are, in fact, identical (see also Ammerer et al., Mol. Cell. Biol. 6:2490-2499, 1986). Based on our observations, we propose a model whereby inactive precursor molecules produced from the PEP4 gene self-activate within the yeast vacuole and subsequently activate other vacuolar hydrolases.
机译:酿酒酵母的pep4突变体积累液泡水解酶的无活性前体。通过互补pep4-3突变从基因组DNA库中分离出PEP4基因。缺失分析将互补活性定位于1.5碱基对的EcoRI-XhoI限制酶片段。该片段用于鉴定能够指导44,000道尔顿多肽的合成的1,800个核苷酸的mRNA。酵母基因组DNA的Southern印迹分析表明,PEP4基因是独特的。然而,酵母中存在一些相关序列。四联体分析和有丝分裂重组实验在XVI染色体上将PEP4基因定位在GAL4附近。 DNA序列分析表明PEP4编码与天冬氨酰蛋白酶家族具有广泛同源性的多肽。 PEP4预测的氨基酸序列与酵母蛋白酶A蛋白序列的比较表明,这两个基因实际上是相同的(另见Ammerer等人,Mol.Cell.Biol.6:2490-2499,1986)。基于我们的观察,我们提出了一个模型,在该模型中,由PEP4基因产生的无活性前体分子在酵母液泡中自我激活,随后激活其他液泡水解酶。

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