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酵母中MAL基因表达的调控:基因剂量效应

Regulation of MAL gene expression in yeast: gene dosage effects.

作者信息

Goldenthal M J, Vanoni M, Buchferer B, Marmur J

机构信息

Department of Biochemistry, Albert Einstein College of Medicine, Bronx, NY 10461.

出版信息

Mol Gen Genet. 1987 Oct;209(3):508-17. doi: 10.1007/BF00331157.

Abstract

Both the MAL1 and MAL6 loci in Saccharomyces strains have been shown by functional and structural studies to comprise a cluster of at least three genes necessary for maltose utilization. They include regulatory, maltose transport and maltase genes designated MALR, MALT and MALS, respectively. Subclones of each gene derived from the MAL6 locus were inserted into the multicopy shuttle plasmid YEp13, introduced into MAL1 and mal1 strains and the effects of altered gene dosage of each gene, or a combination of them, on MAL gene expression investigated. MAL1 strains transformed with a plasmid carrying the MAL6S gene showed coordinate four to five fold increases in both maltase enzyme activity and its mRNA, whereas no increase in maltose transport activity or of MALT mRNA was observed when MAL6T was present on multicopy plasmids. The presence of the MAL6R gene on a multicopy plasmid led to greatly increased transcription of both inducible and constitutive mRNAs with homology to the regulatory gene; it also gave rise to two fold increases in both induced maltase mRNA levels and enzyme activity, but only in the presence of maltose. However, it had no apparent effect on the accumulation of MALT mRNA. Finally, the induction kinetics of plasmid-borne and chromosomal MALS and MALT gene expression were examined under conditions of altered gene dosage of the MAL6 regulatory and structural genes. The results of these experiments indicate that MALR encodes a trans-acting positive activator that requires maltose for induction of MALS and MALT transcription even when the regulatory gene is present on a multicopy plasmid. Maltose transport can be a rate-limiting factor in MAL gene expression, at least in the early stages of induction. The regulation of the MALS and MALT genes, whose activities are coordinately induced in MAL1 strains by maltose, may in fact exhibit some important differences.

摘要

通过功能和结构研究表明,酿酒酵母菌株中的MAL1和MAL6位点均包含一组至少三个利用麦芽糖所必需的基因。它们分别包括调控基因、麦芽糖转运基因和麦芽糖酶基因,命名为MALR、MALT和MALS。从MAL6位点衍生的每个基因的亚克隆被插入到多拷贝穿梭质粒YEp13中,导入MAL1和mal1菌株,并研究每个基因或它们的组合基因剂量改变对MAL基因表达的影响。用携带MAL6S基因的质粒转化的MAL1菌株,麦芽糖酶活性及其mRNA均协同增加了四到五倍,而当MAL6T存在于多拷贝质粒上时,未观察到麦芽糖转运活性或MALT mRNA增加。多拷贝质粒上存在MAL6R基因导致与调控基因具有同源性的诱导型和组成型mRNA的转录大幅增加;它还使诱导的麦芽糖酶mRNA水平和酶活性均增加了两倍,但仅在有麦芽糖存在的情况下。然而,它对MALT mRNA的积累没有明显影响。最后,在MAL6调控基因和结构基因剂量改变的条件下,检测了质粒携带的和染色体上的MALS和MALT基因表达的诱导动力学。这些实验结果表明,MALR编码一种反式作用的正激活因子,即使调控基因存在于多拷贝质粒上,诱导MALS和MALT转录也需要麦芽糖。麦芽糖转运可能是MAL基因表达中的一个限速因素,至少在诱导的早期阶段是这样。MALS和MALT基因的活性在MAL1菌株中由麦芽糖协同诱导,其调控实际上可能存在一些重要差异。

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