首页> 美国卫生研究院文献>Applied and Environmental Microbiology >Improvement of Galactose Uptake in Saccharomyces cerevisiae through Overexpression of Phosphoglucomutase: Example of Transcript Analysis as a Tool in Inverse Metabolic Engineering
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Improvement of Galactose Uptake in Saccharomyces cerevisiae through Overexpression of Phosphoglucomutase: Example of Transcript Analysis as a Tool in Inverse Metabolic Engineering

机译:通过过量表达磷酸葡萄糖突变酶改善酿酒酵母中半乳糖的摄取:转录分析作为逆代谢工程工具的实例

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摘要

Through genome-wide transcript analysis of a reference strain and two recombinant Saccharomyces cerevisiae strains with different rates of galactose uptake, we obtained information about the global transcriptional response to metabolic engineering of the GAL gene regulatory network. One of the recombinant strains overexpressed the gene encoding the transcriptional activator Gal4, and in the other strain the genes encoding Gal80, Gal6, and Mig1, which are negative regulators of the GAL system, were deleted. Even though the galactose uptake rates were significantly different in the three strains, we surprisingly did not find any significant changes in the expression of the genes encoding the enzymes catalyzing the first steps of the pathway (i.e., the genes encoding Gal2, Gal1, Gal7, and Gal10). We did, however, find that PGM2, encoding the major isoenzyme of phosphoglucomutase, was slightly up-regulated in the two recombinant strains with higher galactose uptake rates. This indicated that PGM2 is a target for overexpression in terms of increasing the flux through the Leloir pathway, and through overexpression of PGM2 the galactose uptake rate could be increased by 70% compared to that of the reference strain. Based on our findings, we concluded that phosphoglucomutase plays a key role in controlling the flux through the Leloir pathway, probably due to increased conversion of glucose-1-phosphate to glucose-6-phosphate. This conclusion was supported by measurements of sugar phosphates, which showed that there were increased concentrations of glucose-6-phosphate, galactose-6-phosphate, and fructose-6-phosphate in the strain construct overexpressing PGM2.
机译:通过参考菌株和两种重组半乳糖摄取率的酿酒酵母菌株的全基因组转录本分析,我们获得了有关GAL基因调控网络对代谢工程的全球转录反应的信息。一种重组菌株过表达编码转录激活因子Gal4的基因,而另一种菌株中缺失编码Gal80,Gal6和Mig1的基因,它们是GAL系统的负​​调控子。即使三种菌株中的半乳糖摄取率显着不同,但我们出乎意料的是并未发现编码催化该途径第一步的酶的基因的表达(即编码Gal2,Gal1,Gal7,和Gal10)。然而,我们确实发现,在两个具有较高半乳糖摄取率的重组菌株中,编码磷酸葡萄糖变位酶的主要同工酶的PGM2略有上调。这表明就增加通过Leloir途径的通量而言,PGM2是过量表达的目标,并且通过过量表达PGM2,与参考菌株相比,半乳糖摄取率可以提高70%。根据我们的发现,我们得出结论,磷酸葡萄糖变位酶在控制通过Leloir途径的通量中起关键作用,这可能是由于1磷酸葡萄糖向6磷酸葡萄糖的转化增加所致。对糖磷酸酯的测量支持了这一结论,该结果表明在过表达PGM2的菌株构建物中,葡萄糖6-磷酸酯,半乳糖6-磷酸酯和果糖6-磷酸酯的浓度增加。

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