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控制酿酒酵母可阻遏酸性磷酸酶合成的PHO82-pho4基因座的结构与功能

Structure and function of the PHO82-pho4 locus controlling the synthesis of repressible acid phosphatase of Saccharomyces cerevisiae.

作者信息

Toh-e A, Inouye S, Oshima Y

出版信息

J Bacteriol. 1981 Jan;145(1):221-32. doi: 10.1128/jb.145.1.221-232.1981.

DOI:10.1128/jb.145.1.221-232.1981
PMID:7007314
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC217264/
Abstract

pho4 mutants of Saccharomyces cerevisiae, although rare among phosphatase-negative mutants isolated from wild-type strains, were isolated efficiently from pho80, pho85, or pho80 pho85 strains. The distribution of these pho4 mutants over the pho4 locus was determined by analyzing random spores of two- and three-factor crosses. The pho4-4 mutation confers temperature-sensitive synthesis of repressible acid phosphatase. An intragenic suppressor for the pho4-12 allele results in the temperature-sensitive synthesis of repressible acid phosphatase. Recombination between these sites occurs at 1.0 to 3.0%, the highest for any pair of sites within the pho4 locus. All these results strongly indicate that the information of the pho4 locus is translated into a protein. The PHO82 site was mapped inside the pho4 locus by random spore analysis. The order met10-pho4-1PHO82-1-pho4-9 on the right arm of chromosome VI was confirmed by tetrad analysis. Doubly heterozygous diploids, pho3 PHO82c PHO4+/pho3 pho82+ pho4, produce variable amounts of repressible acid phosphatase under repressive conditions depending on the combination of PHO82c and pho4 alleles. This phenomenon may reflect the constitutive production of the pho82+-pho4 product in the repressed condition, which interferes with the function of the PHO82c-PHO4+ product. The earlier model for the function of the PHO82-pho4 cluster, in which the PHO82 site acts as an operator of the pho4 gene, has been revised to a model in which the PHO82 site codes for the part of the pho4 protein that has affinity for the regulatory protein encoded by the pho80 and pho85 genes.

摘要

酿酒酵母的pho4突变体,虽然在从野生型菌株中分离出的磷酸酶阴性突变体中很罕见,但能从pho80、pho85或pho80 pho85菌株中高效分离出来。通过分析双因子和三因子杂交的随机孢子,确定了这些pho4突变体在pho4基因座上的分布。pho4 - 4突变赋予可阻遏酸性磷酸酶温度敏感型合成。pho4 - 12等位基因的一个基因内抑制子导致可阻遏酸性磷酸酶的温度敏感型合成。这些位点之间的重组发生率为1.0%至3.0%,是pho4基因座内任意一对位点之间重组率最高的。所有这些结果都有力地表明,pho4基因座的信息被翻译成了一种蛋白质。通过随机孢子分析,将PHO82位点定位在pho4基因座内。通过四分体分析,证实了在第六条染色体右臂上的顺序为met10 - pho4 - 1PHO82 - 1 - pho4 - 9。双杂合二倍体pho3 PHO82c PHO4 + /pho3 pho82 + pho4在阻遏条件下根据PHO82c和pho4等位基因的组合产生不同量的可阻遏酸性磷酸酶。这种现象可能反映了在阻遏条件下pho82 + - pho4产物的组成型产生,它干扰了PHO82c - PHO4 + 产物的功能。关于PHO82 - pho4簇功能的早期模型,即PHO82位点作为pho4基因的操纵子,已被修订为一个模型,其中PHO82位点编码pho4蛋白中对由pho80和pho85基因编码的调节蛋白具有亲和力的部分。

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