Inducible engineering precursor metabolic flux for synthesizing hyaluronic acid of customized molecular weight in Streptococcus zooepidemicus.

IF 4.3 2区 生物学 Q1 BIOTECHNOLOGY & APPLIED MICROBIOLOGY
Rui Zhao, Jun Li, Yingtian Li, Xujuan Pei, Jingyi Di, Zhoujie Xie, Hao Liu, Weixia Gao
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引用次数: 0

Abstract

Background: Hyaluronic acid (HA) is extensively employed in various fields such as medicine, cosmetics, food, etc. The molecular weight (MW) of HA is crucial for its biological functions. Streptococcus zooepidemicus, a prominent HA industrial producer, naturally synthetizes HA with high MW. Currently, few effective approaches exist for the direct and precise regulation of HA MW through a one-step fermentation process, and S. zooepidemicus lacks metabolic regulatory elements with varying intensities. The ratio of HA's precursors, UDP-N-acetylglucosamine (UDP-GlcNAc) and UDP-glucuronic acid (UDP-GlcA), is critical for the extension and release of HA. An imbalance in the precursor proportions for HA synthesis leads to a significant decrease in HA MW, indicating that controlling the precursor ratio may serve as a potential method for regulating HA MW.

Results: In this study, the type and concentration of carbon sources were manipulated to disrupt the balance of precursor supply. Based on the results, it was speculated that the transcription level of hasE, which may connect the two HA synthesis precursors, is positively correlated with HA MW. Consequently, an endogenous expression component library for S. zooepidemicus was constructed, comprising 32 constitutive and 4 inducible expression elements. The expression of hasE was subsequently regulated in strain SE0 (S12 ΔhasE) using two constitutive promoters of differing strengths. The recombinant strain SE1, in which hasE was controlled by the stronger promoter PR31, produced HA with a MW of 1.96 MDa. In contrast, SE2, utilizing the weaker promoter PR22, synthesized shorter HA with a MW of 1.63 MDa, thereby verifying the hypothesis. Finally, to precisely regulate HA MW according to specific demands, an efficient sucrose-induced expression system was screened and employed to control the transcription level of hasE, obtaining recombinant strain SE3. When induced with sucrose concentrations of 3, 5-10 g/L, the HA MW of SE3 reached 0.78 to 1.77 MDa, respectively.

Conclusions: Studies on regulating the balance of the HA precursor substances indicate that an oversupply of either UDP-GlcNAc or UDP-GlcUA can reduce HA MW. The hasE gene serves as a crucial regulator for maintaining this balance. Precise regulation of hasE transcription was achieved through an efficient inducible expression system, enabling the customized production of HA with specific MW. The HA MW of strain SE3 can be accurately manipulated by adjusting sucrose concentration, establishing a novel strategy for customized HA fermentation.

动物流行病链球菌合成定制分子量透明质酸的诱导工程前体代谢通量。
背景:透明质酸(HA)广泛应用于医药、化妆品、食品等各个领域。透明质酸的分子量对其生物学功能至关重要。动物流行病链球菌是一个著名的HA工业生产者,自然合成高分子量的HA。目前,通过一步发酵过程直接精确调控HA MW的有效途径尚不多见,且动物流行病葡萄球菌缺乏不同强度的代谢调控元件。HA的前体,udp - n -乙酰氨基葡萄糖(UDP-GlcNAc)和udp -葡萄糖醛酸(UDP-GlcA)的比例对HA的延伸和释放至关重要。HA合成前体比例失衡导致HA MW显著降低,表明控制前体比例可能是调控HA MW的一种潜在方法。结果:在本研究中,通过控制碳源的类型和浓度来破坏前体供应的平衡。由此推测,连接两种HA合成前体的hasE的转录水平与HA分子量呈正相关。构建了动物疫病球菌内源表达元件库,包括32个组成元件和4个诱导元件。随后,菌株SE0 (S12 ΔhasE)使用两种不同强度的本构启动子调控了hasE的表达。重组菌株SE1酶受较强启动子PR31控制,产生的HA分子量为1.96 MDa。相比之下,SE2利用较弱的启动子PR22合成了较短的HA,分子量为1.63 MDa,从而验证了假设。最后,为了根据特定需求精确调节HA MW,我们筛选了高效的蔗糖诱导表达体系,用于控制hasE的转录水平,获得了重组菌株SE3。当蔗糖浓度为3、5 ~ 10 g/L时,SE3的HA MW分别达到0.78 ~ 1.77 MDa。结论:调节HA前体物质平衡的研究表明,过量供应UDP-GlcNAc或UDP-GlcUA均可降低HA MW。ase基因是维持这种平衡的关键调节因子。通过高效的诱导表达系统实现了对hasE转录的精确调控,从而实现了具有特定分子量的HA的定制生产。菌株SE3的HA MW可以通过调节蔗糖浓度来精确控制,建立了一种定制化HA发酵的新策略。
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来源期刊
Microbial Cell Factories
Microbial Cell Factories 工程技术-生物工程与应用微生物
CiteScore
9.30
自引率
4.70%
发文量
235
审稿时长
2.3 months
期刊介绍: Microbial Cell Factories is an open access peer-reviewed journal that covers any topic related to the development, use and investigation of microbial cells as producers of recombinant proteins and natural products, or as catalyzers of biological transformations of industrial interest. Microbial Cell Factories is the world leading, primary research journal fully focusing on Applied Microbiology. The journal is divided into the following editorial sections: -Metabolic engineering -Synthetic biology -Whole-cell biocatalysis -Microbial regulations -Recombinant protein production/bioprocessing -Production of natural compounds -Systems biology of cell factories -Microbial production processes -Cell-free systems
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