4.7 Article

Natural diversity of lactococci in γ-aminobutyric acid (GABA) production and genetic and phenotypic determinants

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MICROBIAL CELL FACTORIES
卷 22, 期 1, 页码 -

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BMC
DOI: 10.1186/s12934-023-02181-4

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Lactococcus lactis; Lactococcus cremoris; gamma-aminobutyric acid; GAD system

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This study combined genotypic and phenotypic approaches to investigate the diversity of GABA production in lactococci. Through comparative genomic analysis and phenotypic analysis, it was found that GABA production varied widely among different strains and species, and the regulation of GAD gene expression was identified as the major contributor to this diversity.
Background gamma-aminobutyric acid (GABA) is a bioactive compound produced by lactic acid bacteria (LAB). The diversity of GABA production in the Lactococcus genus is poorly understood. Genotypic and phenotypic approaches were therefore combined in this study to shed light on this diversity. A comparative genomic study was performed on the GAD-system genes (gadR, gadC and gadB) involved in GABA production in 36 lactococci including L. lactis and L. cremoris species. In addition, 132 Lactococcus strains were screened for GABA production in culture medium supplemented with 34 mM L-glutamic acid with or without NaCl (0.3 M). Results Comparative analysis of the nucleotide sequence alignments revealed the same genetic organization of the GAD system in all strains except one, which has an insertion sequence element (IS981) into the P-gadCB promoter. This analysis also highlighted several deletions including a 3-bp deletion specific to the cremoris species located in the P-gadR promoter, and a second 39-bp deletion specific to L. cremoris strains with a cremoris phenotype. Phenotypic analysis revealed that GABA production varied widely, but it was higher in L. lactis species than in L. cremoris, with an exceptional GABA production of up to 14 and 24 mM in two L. lactis strains. Moreover, adding chloride increased GABA production in some L. cremoris and L. lactis strains by a factor of up to 16 and GAD activity correlated well with GABA production. Conclusions This genomic analysis unambiguously characterized the cremoris phenotype of L. cremoris species and modified GadB and GadR proteins explain why the corresponding strains do not produce GABA. Finally, we found that glutamate decarboxylase activity revealing GadB protein amount, varied widely between the strains and correlated well with GABA production both with and without chloride. As this protein level is associated to gene expression, the regulation of GAD gene expression was identified as a major contributor to this diversity.

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