Genetically engineered Lactococcus lactis strain constitutively expresses GABA-producing genes and produces high levels of GABA.

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-06-03 DOI:10.1093/lambio/ovae051
Marcos P Monteiro, Hannah M Kohl, Jean-Baptiste Roullet, K Michael Gibson, Javier Ochoa-Repáraz, Andrea R Castillo
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Abstract

γ-Aminobutyric acid (GABA) is an inhibitory neurotransmitter of the central nervous system that impacts physical and mental health. Low GABA levels have been documented in several diseases, including multiple sclerosis and depression, and studies suggest that GABA could improve disease outcomes in those conditions. Probiotic bacteria naturally produce GABA and have been engineered to enhance its synthesis. Strains engineered thus far use inducible expression systems that require the addition of exogenous molecules, which complicates their development as therapeutics. This study aimed to overcome this challenge by engineering Lactococcus lactis with a constitutive GABA synthesis gene cassette. GABA synthesizing and transport genes (gadB and gadC) were cloned onto plasmids downstream of constitutive L. lactis promoters [P2, P5, shortened P8 (P8s)] of different strengths and transformed into L. lactis. Fold increase in gadCB expression conferred by these promoters (P2, P5, and P8s) was 322, 422, and 627, respectively, compared to the unmodified strain (P = 0.0325, P8s). GABA synthesis in the highest gadCB expressing strain, L. lactis-P8s-glutamic acid decarboxylase (GAD), was dependent on media supplementation with glutamic acid and significantly higher than the unmodified strain (P < 0.0001, 125 mM, 200 mM glutamic acid). Lactococcus lactis-P8s-GAD is poised for therapeutic testing in animal models of low-GABA-associated disease.

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经过基因工程改造的乳酸乳球菌菌株可连续表达 GABA 生成基因,并产生大量 GABA。
GABA 是中枢神经系统的一种抑制性神经递质,对身心健康有影响。研究表明,GABA 可以改善这些疾病的治疗效果。益生菌能自然产生 GABA,并通过改造来提高 GABA 的合成。迄今为止,改造的菌株使用的是需要添加外源分子的诱导表达系统,这使其作为治疗药物的开发变得复杂。本研究旨在通过改造乳酸乳球菌(Lactococcus lactis)的组成型 GABA 合成基因盒来克服这一难题。GABA 合成和转运基因(gadB 和 gadC)被克隆到不同强度的组成型乳球菌启动子(P2、P5 和 P8s)下游的质粒上,并被转化到乳球菌中。与未修饰菌株相比,这些启动子(P2、P5 和 P8s)所赋予的 gadCB 表达量分别增加了 322、422 和 627 倍(P = 0.0325,P8s)。在 gadCB 表达量最高的菌株 L. lactis P8s-GAD 中,GABA 的合成依赖于培养基中谷氨酸的补充,并显著高于未修饰菌株(P=0.0325,P8s)。
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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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