The cssR gene of Corynebacterium glutamicum plays a negative regulatory role in stress responses

The cssR gene of Corynebacterium glutamicum plays a negative regulatory role in stress responses

CssR, the product of the Corynebacterium glutamicum ncgl1578 gene cotranscribed with ncgl1579, is a TetR (tetracycline regulator) family repressor. Although many TetR-type regulators in C. glutamicum have been extensively described, members of the TetR family involved in the stress response remain u...

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Veröffentlicht in:Microbial cell factories 2021-06, Vol.20 (1), p.1-110, Article 110
Hauptverfasser: Liu, Yang, Yang, Wenzhi, Su, Tao, Che, Chengchuan, Li, Guizhi, Chen, Can, Si, Meiru
Format: Artikel
Sprache:eng
Schlagworte:
Actinomycetes
Antibiotics
Antiinfectives and antibacterials
Bacteria
Binding sites
Biosynthesis
Corynebacterium glutamicum
Cysteine
Deoxyribonucleic acid
DNA
Drug resistance
E coli
Enzymes
Gene expression
Genes
Genetic aspects
Genetic transcription
Heavy metals
Homeostasis
Hydrogen peroxide
Ligand binding
Mutagenesis
Mutants
NADP
Oxidants
Oxidation
Oxidative stress
Oxidizing agents
Physiological aspects
Plasmids
Proteins
Residues
Strain
Stress (Physiology)
Stress response
TetR
Transcription
Transcription factors
Transcription regulation
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Zusammenfassung:CssR, the product of the Corynebacterium glutamicum ncgl1578 gene cotranscribed with ncgl1579, is a TetR (tetracycline regulator) family repressor. Although many TetR-type regulators in C. glutamicum have been extensively described, members of the TetR family involved in the stress response remain unidentified. In this study, we found that CssR regulated the transcription of its own gene and the ncgl1576-ncgl1577 operon. The ncgl1576-ncgl1577 operon, which is located upstream of cssR in the orientation opposite that of the cssR operon, encodes an ATP-binding cassette (ABC), some of which are involved in the export of a wide range of antimicrobial compounds. The cssR-deletion ([DELA]cssR) mutant displayed increased resistance to various stresses. An imperfect palindromic motif (5'-TAA(G)TGN.sub.13CA(G)TTA-3'; 25 bp) located at the intergenic region between cssR and ncgl1577 was identified as the sole binding site for CssR. Expression of cssR and ncgl1577 was induced by antibiotics and heavy metals but not H.sub.2O.sub.2 or diamide, and the DNA-binding activity of CssR was impaired by antibiotics and heavy metals but not H.sub.2O.sub.2. Antibiotics and heavy metals caused CssR dissociation from target gene promoters, thus derepressing their transcription. Oxidant treatment neither altered the conformation of CssR nor modified its cysteine residues, indicating that the cysteine residues in CssR have no redox activity. In the [DELA]cssR mutant strain, genes involved in redox homeostasis also showed increased transcription levels, and the NADPH/NADP.sup.+ ratio was higher than that of the parental strain. The stress response mechanism of CssR in C. glutamicum is realized via ligand-induced conformational changes of the protein, not via cysteine oxidation-based thiol modification. Moreover, the crucial role of CssR in the stress response was demonstrated by negatively controlling the expression of the ncgl1576-ncgl1577 operon, its structural gene, and/or redox homeostasis-related genes.
ISSN:1475-2859
1475-2859
DOI:10.1186/s12934-021-01600-8