4.7 Article

LsrR, the effector of AI-2 quorum sensing, is vital for the H2O2 stress response in mammary pathogenic Escherichia coli

期刊

VETERINARY RESEARCH
卷 52, 期 1, 页码 -

出版社

BMC
DOI: 10.1186/s13567-021-00998-8

关键词

cow mastitis; mammary pathogenic Escherichia coli; H2O2; AI-2 quorum sensing; LsrR

资金

  1. National Natural Science Foundation of China [31672571]
  2. Doctoral Start-Up Foundation of Linyi University [LYDX2020BS031]

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This study revealed the crucial role of LsrR in the oxidative stress response of MPEC, showing that mutation of lsrR significantly impacted the survival ability of the pathogenic Escherichia coli, further confirming that LsrR affects oxidative stress response by regulating the expression of specific genes in bacteria.
Mammary pathogenic Escherichia coli (MPEC) is an important causative agent of mastitis in dairy cows that results in reduced milk quality and production, and is responsible for severe economic losses in the dairy industry worldwide. Oxidative stress, as an imbalance between reactive oxygen species (ROS) and antioxidants, is a stress factor that is common in most bacterial habitats. The presence of ROS can damage cellular sites, including iron-sulfur clusters, cysteine and methionine protein residues, and DNA, and may cause bacterial cell death. Previous studies have reported that Autoinducer 2 (AI-2) can regulate E. coli antibiotic resistance and pathogenicity by mediating the intracellular receptor protein LsrR. This study explored the regulatory mechanism of LsrR on the H2O2 stress response in MPEC, showing that the transcript levels of lsrR significantly decreased under H2O2 stress conditions. The survival cell count of lsrR mutant XW10/pSTV28 was increased about 3080-fold when compared with that of the wild-type WT/pSTV28 in the presence of H2O2 and overexpression of lsrR (XW10/pUClsrR) resulted in a decrease in bacterial survival rates under these conditions. The beta-galactosidase reporter assays showed that mutation of lsrR led to a remarkable increase in expression of the promoters of ahpCF, katG and oxyR, while lsrR-overexpressing significantly reduced the expression of ahpCF and katG. The electrophoretic mobility shift assays confirmed that LsrR could directly bind to the promoter regions of ahpCF and katG. These results revealed the important role played by LsrR in the oxidative stress response of MPEC.

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