Dissecting the RecA-(In)dependent Response to Mitomycin C in Mycobacterium tuberculosis Using Transcriptional Profiling and Proteomics Analyses

Anna Brzostek; Przemysław Płociński; Alina Minias; Aneta Ciszewska; Filip Gąsior; Jakub Pawełczyk; Bożena Dziadek; Marcin Słomka; Jarosław Dziadek

doi:10.3390/cells10051168

Dissecting the RecA-(In)dependent Response to Mitomycin C in Mycobacterium tuberculosis Using Transcriptional Profiling and Proteomics Analyses

Cells. 2021 May 11;10(5):1168. doi: 10.3390/cells10051168.

Authors

Anna Brzostek¹, Przemysław Płociński^{1

2}, Alina Minias¹, Aneta Ciszewska¹, Filip Gąsior¹, Jakub Pawełczyk¹, Bożena Dziadek³, Marcin Słomka⁴, Jarosław Dziadek¹

Affiliations

¹ Institute of Medical Biology of the Polish Academy of Sciences, Lodowa 106, 93-232 Łódź, Poland.
² Department of Immunology and Infectious Biology, Faculty of Biology and Environmental Protection, University of Łódź, Banacha 12/16, 90-237 Łódź, Poland.
³ Department of Molecular Microbiology, Faculty of Biology and Environmental Protection, University of Łódź, Banacha 12/16, 90-237 Łódź, Poland.
⁴ Biobank Lab, Department of Molecular Biophysics, Faculty of Biology and Environmental Protection, University of Łódź, Pomorska 139, 90-235 Łódź, Poland.

Abstract

Mycobacteria exploit at least two independent global systems in response to DNA damage: the LexA/RecA-dependent SOS response and the PafBC-regulated pathway. Intracellular pathogens, such as Mycobacterium tuberculosis, are exposed to oxidative and nitrosative stress during the course of infection while residing inside host macrophages. The current understanding of RecA-independent responses to DNA damage is based on the saprophytic model of Mycobacterium smegmatis, a free-living and nonpathogenic mycobacterium. The aim of the present study was to identify elements of RecA-independent responses to DNA damage in pathogenic intracellular mycobacteria. With the help of global transcriptional profiling, we were able to dissect RecA-dependent and RecA-independent pathways. We profiled the DNA damage responses of an M. tuberculosis strain lacking the recA gene, a strain with an undetectable level of the PafBC regulatory system, and a strain with both systems tuned down simultaneously. RNA-Seq profiling was correlated with the evaluation of cell survival in response to DNA damage to estimate the relevance of each system to the overall sensitivity to genotoxic agents. We also carried out whole-cell proteomics analysis of the M. tuberculosis strains in response to mitomycin C. This approach highlighted that LexA, a well-defined key element of the SOS system, is proteolytically inactivated during RecA-dependent DNA repair, which we found to be transcriptionally repressed in response to DNA-damaging agents in the absence of RecA. Proteomics profiling revealed that AlkB was significantly overproduced in the ΔrecA pafBC^{CRISPRi/dCas9} strain and that Holliday junction resolvase RuvX was a DNA damage response factor that was significantly upregulated regardless of the presence of functional RecA and PafBC systems, thus falling into a third category of DNA damage factors: RecA- and PafBC-independent. While invisible to the mass spectrometer, the genes encoding alkA, dnaB, and dnaE2 were significantly overexpressed in the ΔrecA pafBC^{CRISPRi/dCas9} strain at the transcript level.

Keywords: DNA damage repair; SOS response; tuberculosis.

Publication types

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

MeSH terms

Bacterial Proteins / metabolism
DNA Damage
DNA Repair
Gene Expression Profiling
Gene Expression Regulation, Bacterial
Humans
Macrophages / metabolism
Mitomycin / pharmacology*
Mycobacterium tuberculosis / drug effects
Mycobacterium tuberculosis / metabolism*
Proteomics
Rec A Recombinases / metabolism*
Serine Endopeptidases / metabolism
Transcription, Genetic
Transcriptional Activation
Tuberculosis / microbiology

Substances

Bacterial Proteins
LexA protein, Bacteria
Mitomycin
Rec A Recombinases
Serine Endopeptidases

Abstract

Publication types

MeSH terms

Substances

Grants and funding