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实验进化揭示了通过增强 Glk 活性和 cAMP 独立的 CRP 突变,从葡萄糖-木糖混合物中有效生产 d-乳酸的途径。

Experimental evolution reveals an effective avenue for d-lactic acid production from glucose-xylose mixtures via enhanced Glk activity and a cAMP-independent CRP mutation.

机构信息

College of Chemistry and Life Sciences, Changchun University of Technology, Changchun, China.

Haihe Laboratory of Synthetic Biology, Tianjin, China.

出版信息

Biotechnol Bioeng. 2024 Nov;121(11):3514-3526. doi: 10.1002/bit.28819. Epub 2024 Jul 31.

DOI:10.1002/bit.28819
PMID:39082641
Abstract

d-Lactic acid holds significant industrial importance due to its versatility and serves as a crucial component in the synthesis of environmentally friendly and biodegradable thermal-resistant poly-lactic acid. This polymer exhibits promising potential as a substitute for nonbiodegradable, petroleum-based plastics. The production of d-lactic acid from lignocellulosic biomass, a type of biorenewable and nonfood resources, can lower costs and improve product competitiveness. Glucose and xylose are the most abundant sugar monomers in lignocellulosic biomass materials. Despite Escherichia coli possessing native xylose catabolic pathways and transport, their ability to effectively utilize xylose is often hindered in the presence of glucose. Here, the E. coli strain Rec1.0, previously engineered to overcome carbon catabolite repression, was selected as the initial strain for reengineering to produce d-lactic acid. An adaptive evolution approach was employed to achieve highly efficient fermentation of glucose-xylose mixtures. The resulting strain, QJL010, could produce d-lactic acid of 87.5 g/L with a carbon yield of 0.99 mol/mol. Notably, the consumption rates of glucose and xylose reached 0.75 and 0.82 g/gDCW/h, respectively. Further analysis revealed that increased Glk activity, resulting from glk mutations (A142V and R188H), along with their upregulated expression, contributed to an elevated glucose consumption rate. Additionally, a CRP G141D mutation, cAMP-independent, stimulated the expression of the xylR, xylE, and galABC* genes, resulting in an accelerated xylose consumption rate. These findings provide valuable support for the utilization of E. coli platform strains in the production of value-added chemicals from lignocellulosic biomass.

摘要

d-乳酸由于其多功能性而具有重要的工业意义,是合成环保和可生物降解的耐热聚乳酸的关键组成部分。这种聚合物作为不可生物降解的石油基塑料的替代品具有很大的潜力。从木质纤维素生物质(一种可再生和非食用资源)生产 d-乳酸可以降低成本并提高产品竞争力。葡萄糖和木糖是木质纤维素生物质材料中最丰富的糖单体。尽管大肠杆菌具有天然的木糖分解代谢途径和运输途径,但在葡萄糖存在的情况下,其有效利用木糖的能力常常受到阻碍。在这里,选择先前经过工程改造以克服碳分解代谢阻遏的大肠杆菌菌株 Rec1.0 作为初始菌株进行重新工程改造以生产 d-乳酸。采用适应性进化方法实现了葡萄糖-木糖混合物的高效发酵。得到的菌株 QJL010 可以产生 87.5 g/L 的 d-乳酸,碳产率为 0.99 mol/mol。值得注意的是,葡萄糖和木糖的消耗速率分别达到 0.75 和 0.82 g/gDCW/h。进一步分析表明,由于 glk 突变(A142V 和 R188H)导致 Glk 活性增加,以及它们的上调表达,葡萄糖消耗速率提高。此外,一种 CRP G141D 突变(cAMP 非依赖性)刺激了 xylR、xylE 和 galABC*基因的表达,从而加速了木糖的消耗速率。这些发现为利用大肠杆菌平台菌株从木质纤维素生物质生产高附加值化学品提供了有价值的支持。

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