CcpA mutants influence selective carbon source utilization by changing interactions with target genes in Bacillus licheniformis

Zhang, Yupeng; Li, Youran; Xiao, Fengxu; Wang, Hanrong; Zhang, Liang; Ding, Zhongyang; Xu, Sha; Gu, Zhenghua; Shi, Guiyang

doi:10.1007/s43393-021-00055-7

Cited by 5 publications

(4 citation statements)

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“…Glucose is a preferred carbon source that can be quickly used to produce energy and metabolites in bacilli, including for the production of acetoin, 2,3-butanediol, acetic acid and so on [ 35 ]. A previous study has demonstrated that CcpA mutants can affect the use of other carbon sources and the synthesis of related metabolites in the presence of glucose [ 36 , 37 , 38 ]. In order to further research the regulation mechanism of CcpA on glucose utilization.…”

Section: Resultsmentioning

confidence: 99%

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A New Mechanism of Carbon Metabolism and Acetic Acid Balance Regulated by CcpA

Zhang,

Xiao,

Zhang

et al. 2023

Microorganisms

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Catabolite control protein A (CcpA) is a critical regulator in Gram-positive bacteria that orchestrates carbon metabolism by coordinating the utilization of different carbon sources. Although it has been widely proved that CcpA helps prioritize the utilization of glucose over other carbon sources, this global regulator’s precise mechanism of action remains unclear. In this study, a mutant Bacillus licheniformis deleted for CcpA was constructed. Cell growth, carbon utilization, metabolites and the transcription of key enzymes of the mutant strain were compared with that of the wild-type one. It was found that CcpA is involved in the regulation of glucose concentration metabolism in Bacillus. At the same time, CcpA regulates glucose metabolism by inhibiting acetic acid synthesis and pentose phosphate pathway key gene zwF. The conversion rate of acetic acid is increased by about 3.5 times after ccpA is deleted. The present study provides a new mechanism of carbon metabolism and acetic acid balance regulated by CcpA. On the one hand, this work deepens the understanding of the regulatory function of CcpA and provides a new view on the regulation of glucose metabolism. On the other hand, it is helpful to the transformation of B. licheniformis chassis microorganisms.

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Section: Resultsmentioning

confidence: 99%

“…B. licheniformis CA is a strain constructed by knocking out the ccpA on the basis of B. licheniformis . The method of ccpA gene knockout is carried out according to the method we reported earlier [ 36 ]. pET28a-CcpA was the plasmid used for the expression of CcpA.…”

Section: Methodsmentioning

confidence: 99%

A New Mechanism of Carbon Metabolism and Acetic Acid Balance Regulated by CcpA

Zhang,

Xiao,

Zhang

et al. 2023

Microorganisms

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“…Subsequently, the ps09-vgb fragment was cloned into pNZTT-D1 using the Sal I restriction site, and plasmid pNZTT-D2 was obtained. The gene knockout was performed according to the homologous recombination method, 43 and then, mutants BL2S and BL2K were constructed (Figure S4).…”

Section: ■ Materials and Methodsmentioning

confidence: 99%

Transcriptome Analysis of Bacillus licheniformis for Improving Bacitracin Production

et al. 2022

ACS Synth. Biol.

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This study aims to find the targets that may influence the production of bacitracin based on RNA sequencing in Bacillus licheniformis. Transcriptional profiling revealed that (i) the expression of the bacT gene, encoding a type II thioesterase (TEII bac ), was positively correlated with bacitracin production and (ii) the oxygen uptake exhibited significant influence on precursor synthesis. The verified experiments showed that the overexpression of TEII bac with an endogenous promoter increased the bacitracin A titer by 37.50%. Furthermore, the increase of oxygen availability through Vitreoscilla hemoglobin (VHb) expression increased the bacitracin A titer by 126.67% under oxygen-restricted conditions. From the transcriptome perspective, the results of this paper demonstrate that TEII bac and oxygen supply are crucial to bacitracin production. This study also provides insights into the construction of chassis cells for the industrial production of secondary metabolites with a preference for aerobic conditions.

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“…Improvement can be made by artificial mutation in the recognized nucleic acid binding region [76] , [77] , [78] . For the modification of transcription factors, site-directed mutagenesis strategy is usually adopted to meet the specific needs in application [79] , and the understanding of the mechanism can be built at the molecular-level [80] , [81] , [82] .…”

Section: Present and Potential Application For Synthetic Biologymentioning

confidence: 99%