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Shuffling of Promoters for Multiple Genes To Optimize Xylose Fermentation in an Engineered Saccharomyces cerevisiae Strain

机译:多个基因的启动子改组,以优化酿酒酵母菌株中的木糖发酵。

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We describe here a useful metabolic engineering tool, multiple-gene-promoter shuffling (MGPS), to optimize expression levels for multiple genes. This method approaches an optimized gene overexpression level by fusing promoters of various strengths to genes of interest for a particular pathway. Selection of these promoters is based on the expression levels of the native genes under the same physiological conditions intended for the application. MGPS was implemented in a yeast xylose fermentation mixture by shuffling the promoters for GND2 and HXK2 with the genes for transaldolase (TAL1), transketolase (TKL1), and pyruvate kinase (PYK1) in the Saccharomyces cerevisiae strain FPL-YSX3. This host strain has integrated xylose-metabolizing genes, including xylose reductase, xylitol dehydrogenase, and xylulose kinase. The optimal expression levels for TAL1, TKL1, and PYK1 were identified by analysis of volumetric ethanol production by transformed cells. We found the optimal combination for ethanol production to be GND2-TAL1-HXK2-TKL1-HXK2-PYK1. The MGPS method could easily be adapted for other eukaryotic and prokaryotic organisms to optimize expression of genes for industrial fermentation.
机译:我们在这里描述了一种有用的代谢工程工具,即多基因启动子改组(MGPS),可以优化多个基因的表达水平。该方法通过将各种强度的启动子融合到特定途径的目标基因上来达到优化的基因过表达水平。这些启动子的选择基于在预期用于该应用的相同生理条件下天然基因的表达水平。通过将酿酒酵母菌株FPL-YSX3中的转醛酶(TAL1),转酮醇酶(TKL1)和丙酮酸激酶(PYK1)的基因改组为GND2和HXK2的启动子,在酵母木糖发酵混合物中实现了MGPS。该宿主菌株具有整合的木糖代谢基因,包括木糖还原酶,木糖醇脱氢酶和木酮糖激酶。通过分析转化细胞产生的乙醇体积,确定了TAL1,TKL1和PYK1的最佳表达水平。我们发现生产乙醇的最佳组合是GND2-TAL1-HXK2-TKL1-HXK2-PYK1。 MGPS方法很容易适用于其他真核生物和原核生物,以优化用于工业发酵的基因表达。

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