Roles of Bacillus subtilis RecA, Nucleotide Excision Repair, and Translesion Synthesis Polymerases in Counteracting Cr(VI)-Promoted DNA Damage

Fernando Santos-Escobar; Hilda C Leyva-Sánchez; Norma Ramírez-Ramírez; Armando Obregón-Herrera; Mario Pedraza-Reyes

doi:10.1128/JB.00073-19

Roles of Bacillus subtilis RecA, Nucleotide Excision Repair, and Translesion Synthesis Polymerases in Counteracting Cr(VI)-Promoted DNA Damage

J Bacteriol. 2019 Mar 26;201(8):e00073-19. doi: 10.1128/JB.00073-19. Print 2019 Apr 15.

Authors

Fernando Santos-Escobar¹, Hilda C Leyva-Sánchez¹, Norma Ramírez-Ramírez¹, Armando Obregón-Herrera¹, Mario Pedraza-Reyes²

Affiliations

¹ Department of Biology, Division of Natural and Exact Sciences, University of Guanajuato, Guanajuato, Mexico.
² Department of Biology, Division of Natural and Exact Sciences, University of Guanajuato, Guanajuato, Mexico pedrama@ugto.mx.

Abstract

Bacteria deploy global programs of gene expression, including components of the SOS response, to counteract the cytotoxic and genotoxic effects of environmental DNA-damaging factors. Here we report that genetic damage promoted by hexavalent chromium elicited the SOS response in Bacillus subtilis, as evidenced by the induction of transcriptional uvrA-lacZ, recA-lacZ, and P _recA-gfp fusions. Accordingly, B. subtilis strains deficient in homologous recombination (RecA) and nucleotide excision repair (NER) (UvrA), components of the SOS response, were significantly more sensitive to Cr(VI) treatment than were cells of the wild-type strain. These results strongly suggest that Cr(VI) induces the formation in growing B. subtilis cells of cytotoxic and genotoxic bulky DNA lesions that are processed by RecA and/or the NER pathways. In agreement with this notion, Cr(VI) significantly increased the formation of DNA-protein cross-links (DPCs) and induced mutagenesis in recA- and uvrA-deficient B. subtilis strains, through a pathway that required YqjH/YqjW-mediated translesion synthesis. We conclude that Cr(VI) promotes mutagenesis and cell death in B. subtilis by a mechanism that involves the formation of DPCs and that such deleterious effects are counteracted by both the NER and homologous recombination pathways, belonging to the RecA-dependent SOS system.IMPORTANCE It has been shown that, following permeation of cell barriers, Cr(VI) kills B. subtilis cells following a mechanism of reactive oxygen species-promoted DNA damage, which is counteracted by the guanine oxidized repair system. Here we report a distinct mechanism of Cr(VI)-promoted DNA damage that involves production of DPCs capable of eliciting the bacterial SOS response. We also report that the NER and homologous recombination (RecA) repair pathways, as well as low-fidelity DNA polymerases, counteract this metal-induced mechanism of killing in B. subtilis Hence, our results contribute to an understanding of how environmental pollutants activate global programs of gene expression that allow bacteria to contend with the cytotoxic and genotoxic effects of heavy metals.

Keywords: Bacillus subtilis; DNA damage; SOS system; chromate; environmental pollutants.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Bacillus subtilis / drug effects*
Bacillus subtilis / enzymology*
Bacillus subtilis / metabolism
Chromium / toxicity*
DNA Damage / drug effects*
DNA Repair*
Mutagens / toxicity*
Rec A Recombinases / metabolism*
SOS Response, Genetics

Substances

Mutagens
Chromium
chromium hexavalent ion
Rec A Recombinases