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首页> 外文期刊>Scientific reports. >Redirection of pyruvate flux toward desired metabolic pathways through substrate channeling between pyruvate kinase and pyruvate-converting enzymes in Saccharomyces cerevisiae
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Redirection of pyruvate flux toward desired metabolic pathways through substrate channeling between pyruvate kinase and pyruvate-converting enzymes in Saccharomyces cerevisiae

机译:通过丙酮酸激酶与丙酮酸酿酒酶与丙酮酸癌酶与丙酮酸丙酮酸丙氨酸酶与丙酮酸胆汁转化酶的底物窜料重定向

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Spatial organization of metabolic enzymes allows substrate channeling, which accelerates processing of intermediates. Here, we investigated the effect of substrate channeling on the flux partitioning at a metabolic branch point, focusing on pyruvate metabolism in Saccharomyces cerevisiae. As a platform strain for the channeling of pyruvate flux, PYK1-Coh-Myc strain was constructed in which PYK1 gene encoding pyruvate kinase is tagged with cohesin domain. By using high-affinity cohesin-dockerin interaction, the pyruvate-forming enzyme Pyk1 was tethered to heterologous pyruvate-converting enzymes, lactate dehydrogenase and α-acetolactate synthase, to produce lactic acid and 2,3-butanediol, respectively. Pyruvate flux was successfully redirected toward desired pathways, with a concomitant decrease in ethanol production even without genetic attenuation of the ethanol-producing pathway. This pyruvate channeling strategy led to an improvement of 2,3-butanediol production by 38%, while showing a limitation in improving lactic acid production due to a reduced activity of lactate dehydrogenase by dockerin tagging.
机译:代谢酶的空间组织允许衬底通道,其加速了中间体的加工。在这里,我们研究了基质沟槽对代谢分支点的助焊剂分配的影响,侧重于糖酵母酿酒酵母中的丙酮酸代谢。作为丙酮酸通量的通道的平台菌株,构建了Pyk1-Coh-Myc菌株,其中编码丙酮酸激酶的Pyk1基因被互联域标记。通过使用高亲和力休闲蛋白 - Dockerin相互作用,将丙酮酸形成酶PYK1拴在异源丙酮酸转化酶,乳酸脱氢酶和α-乙酸盐合酶,分别产生乳酸和2,3-丁二醇。丙酮酸液相成功地重定向到所需的途径,即使在没有乙醇产生途径的遗传衰减,乙醇产量也会随着乙醇的遗传而降低。这种丙酮酸渠道策略导致了2,3-丁二醇产量的提高38%,同时显示出改善乳酸产生的限制由于Dockerin标记的减少活性乳酸脱氢酶的活性。

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