Shuo Zhang, Tao Ma, Fu-Hui Zheng, Muhammad Aslam, Yu-Jie Wang, Zhen-Ming Chi, Guang-Lei Liu
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For auxotrophic selection system, the engineered strains harboring auxotrophic marker genes are typically supplemented with complex nutrient-rich components instead of precisely defined synthetic media in large-scale industrial fermentations, thus lack selection pressure to ensure the stability of heterologous metabolic pathways. Therefore, it is a critical to explore alternative selection systems that can be adapted for large-scale industrial fermentation.</p><h3>Results</h3><p>Here, a novel glucose-dependent selection system was developed in a high pullulan-producing non-conventional strain <i>A. melanogenum</i> P16. The system comprised a glucose-deficient chassis cell Δ<i>pfk</i> obtained through the knockout of the phosphofructokinase gene (<i>PFK</i>) and a series of chromosomal integration plasmids carrying a selection marker <i>PFK</i> controlled by different strength promoters. Utilizing the green fluorescent protein gene (<i>GFP</i>) as a reporter gene, this system achieved a 100% positive rate of transformation, and the chromosomal integration numbers of <i>GFP</i> showed an inverse relationship with promoter strength, with a customizable copy number ranging from 2 to 54. More importantly, the chromosomal integration numbers of target genes remained stable during successive inoculation and fermentation process, facilitated simply by using glucose as a cost-effective and environmental-friendly selectable molecule to maintain a constant and rigorous screening pressure. Moreover, this glucose-dependent selection system exhibited no significant effect on cell growth and product synthesis, and the glucose-deficient related selectable marker <i>PFK</i> has universal application potential in non-conventional yeasts.</p><h3>Conclusion</h3><p>Here, we have developed a novel glucose-dependent selection system to achieve customizable and stable multilocus chromosomal integration of target genes. 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引用次数: 0
摘要
背景非常规酵母作为微生物生物生产的生物精炼细胞工厂具有巨大潜力。目前,用于这些酵母的基因编辑系统依赖于抗生素和辅助选择机制。然而,抗生素的缺点,包括高成本、环境问题和抗性基因的传播,使其不适合大规模工业发酵。就辅助营养选择系统而言,在大规模工业发酵中,携带辅助营养标记基因的工程菌株通常需要补充富含复杂营养成分的培养基,而不是精确定义的合成培养基,因此缺乏选择压力来确保异源代谢途径的稳定性。因此,探索可适用于大规模工业发酵的替代选择系统至关重要。结果在高产拉普兰的非常规菌株 A. melanogenum P16 中开发了一种新的葡萄糖依赖性选择系统。该系统包括通过敲除磷酸果糖激酶基因(PFK)获得的葡萄糖缺陷底盘细胞 Δpfk,以及一系列携带由不同强度启动子控制的选择标记 PFK 的染色体整合质粒。利用绿色荧光蛋白基因(GFP)作为报告基因,该系统实现了100%的阳性转化率,而且GFP的染色体整合数量与启动子强度呈反比关系,可定制的拷贝数从2到54不等。更重要的是,目标基因的染色体整合数在连续的接种和发酵过程中保持稳定,这得益于使用葡萄糖这种经济、环保的选择性分子来维持恒定、严格的筛选压力。此外,这种葡萄糖依赖性选择系统对细胞生长和产物合成无明显影响,而葡萄糖缺陷相关选择标记 PFK 在非常规酵母中具有普遍应用潜力。因此,这项研究为非常规酵母的遗传操作和菌株改良提供了一种前景广阔的新工具,尤其适合工业发酵应用。
Customizable and stable multilocus chromosomal integration: a novel glucose-dependent selection system in Aureobasidium spp.
Background
Non-conventional yeasts hold significant potential as biorefinery cell factories for microbial bioproduction. Currently, gene editing systems used for these yeasts rely on antibiotic and auxotrophic selection mechanisms. However, the drawbacks of antibiotics, including high costs, environmental concerns, and the dissemination of resistance genes, make them unsuitable for large-scale industrial fermentation. For auxotrophic selection system, the engineered strains harboring auxotrophic marker genes are typically supplemented with complex nutrient-rich components instead of precisely defined synthetic media in large-scale industrial fermentations, thus lack selection pressure to ensure the stability of heterologous metabolic pathways. Therefore, it is a critical to explore alternative selection systems that can be adapted for large-scale industrial fermentation.
Results
Here, a novel glucose-dependent selection system was developed in a high pullulan-producing non-conventional strain A. melanogenum P16. The system comprised a glucose-deficient chassis cell Δpfk obtained through the knockout of the phosphofructokinase gene (PFK) and a series of chromosomal integration plasmids carrying a selection marker PFK controlled by different strength promoters. Utilizing the green fluorescent protein gene (GFP) as a reporter gene, this system achieved a 100% positive rate of transformation, and the chromosomal integration numbers of GFP showed an inverse relationship with promoter strength, with a customizable copy number ranging from 2 to 54. More importantly, the chromosomal integration numbers of target genes remained stable during successive inoculation and fermentation process, facilitated simply by using glucose as a cost-effective and environmental-friendly selectable molecule to maintain a constant and rigorous screening pressure. Moreover, this glucose-dependent selection system exhibited no significant effect on cell growth and product synthesis, and the glucose-deficient related selectable marker PFK has universal application potential in non-conventional yeasts.
Conclusion
Here, we have developed a novel glucose-dependent selection system to achieve customizable and stable multilocus chromosomal integration of target genes. Therefore, this study presents a promising new tool for genetic manipulation and strain enhancement in non-conventional yeasts, particularly tailored for industrial fermentation applications.
期刊介绍:
Biotechnology for Biofuels is an open access peer-reviewed journal featuring high-quality studies describing technological and operational advances in the production of biofuels, chemicals and other bioproducts. The journal emphasizes understanding and advancing the application of biotechnology and synergistic operations to improve plants and biological conversion systems for the biological production of these products from biomass, intermediates derived from biomass, or CO2, as well as upstream or downstream operations that are integral to biological conversion of biomass.
Biotechnology for Biofuels focuses on the following areas:
• Development of terrestrial plant feedstocks
• Development of algal feedstocks
• Biomass pretreatment, fractionation and extraction for biological conversion
• Enzyme engineering, production and analysis
• Bacterial genetics, physiology and metabolic engineering
• Fungal/yeast genetics, physiology and metabolic engineering
• Fermentation, biocatalytic conversion and reaction dynamics
• Biological production of chemicals and bioproducts from biomass
• Anaerobic digestion, biohydrogen and bioelectricity
• Bioprocess integration, techno-economic analysis, modelling and policy
• Life cycle assessment and environmental impact analysis
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