Role of PumB antitoxin as a transcriptional regulator of the PumAB type-II toxin–antitoxin system and its endoribonuclease activity on the PumA (toxin) transcript

被引:0
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作者
K. C. Hernández-Ramírez
M. I. Valle-Maldonado
J. A. Patiño-Medina
S. Calo
I. E. Jácome-Galarza
V. Garre
V. Meza-Carmen
M. I. Ramírez-Díaz
机构
[1] Universidad Michoacana de San Nicolás de Hidalgo,Laboratorio de Microbiología, Instituto de Investigaciones Químico
[2] Universidad Michoacana de San Nicolás de Hidalgo,Biológicas
[3] Ciudad Universitaria,Laboratorio de Diferenciación Celular, Instituto de Investigaciones Químico
[4] Secretaría de Salud Michoacán,Biológicas
[5] Pontificia Universidad Católica Madre y Maestra,Laboratorio Estatal de Salud Pública
[6] Universidad de Murcia,School of Natural and Exact Sciences
来源
Molecular Genetics and Genomics | 2023年 / 298卷
关键词
PumAB toxin–antitoxin system; Transcriptional regulator; Endoribonuclease activity;
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学科分类号
摘要
The PumAB type-II toxin–antitoxin (TA) system is encoded by pumAB genes that are organized into an operon. This system is encoded by the pUM505 plasmid, isolated from a Pseudomonas aeruginosa clinical strain. The pumA gene encodes a putative RelE toxin protein (toxic component), whereas the pumB gene encodes a putative HTH antitoxin protein. The expression of the PumAB system in Escherichia coli confers plasmid stability. In addition, PumA toxin overexpression in P. aeruginosa possesses the capability to increase bacterial virulence, an effect that is neutralized by the PumB antitoxin. The aim of this study was to establish the mechanism of regulation of the PumAB toxin–antitoxin system from pUM505. By an in silico analysis of the putative regulatory elements, we identified two putative internal promoters, PpumB and PpumB-AlgU (in addition to the already reported PpumAB), located upstream of pumB. By RT-qPCR assays, we determined that the pumAB genes are transcribed differentially, in that the mRNA of pumB is more abundant than the pumA transcript. We also observed that pumB could be expressed individually and that its mRNA levels decreased under oxidative stress, during individual expression as well as co-expression of pumAB. However, under stressful conditions, the pumA mRNA levels were not affected. This suggests the negative regulation of pumB by stressful conditions. The PumB purified protein was found to bind to a DNA region located between the PpumAB and the pumA coding region, and PumA participates in PumB binding, suggesting that a PumA–PumB complex co-regulates the transcription of the pumAB operon. Interestingly, the pumA mRNA levels decreased after incubation in vitro with PumB protein. This effect was repressed by ribonuclease inhibitors, suggesting that PumB could function as an RNAse toward the mRNA of the toxin. Taken together, we conclude that the PumAB TA system possesses multiple mechanisms to regulate its expression, as well as that the PumB antitoxin generates a decrease in the mRNA toxin levels, suggesting an RNase function. Our analysis provides new insights into the understanding of the control of TA systems from mobile plasmid-encoded genes from a human pathogen.
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页码:455 / 472
页数:17
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