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Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities

The bacterium Yersinia pestis has developed various strategies to sense and respond to the complex stresses encountered during its transmission and pathogenic processes. PurR is a common transcriptional regulator of purine biosynthesis among microorganisms, and it modulates the transcription level o...

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Autores principales: Xiao, Liting, Jin, Junyan, Song, Kai, Qian, Xiuwei, Wu, Yarong, Sun, Zhulin, Xiong, Ziyao, Li, Yanbing, Zhao, Yanting, Shen, Leiming, Cui, Yiming, Yao, Wenwu, Cui, Yujun, Song, Yajun
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2023
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10673613/
https://www.ncbi.nlm.nih.gov/pubmed/38004812
http://dx.doi.org/10.3390/microorganisms11112801
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author Xiao, Liting
Jin, Junyan
Song, Kai
Qian, Xiuwei
Wu, Yarong
Sun, Zhulin
Xiong, Ziyao
Li, Yanbing
Zhao, Yanting
Shen, Leiming
Cui, Yiming
Yao, Wenwu
Cui, Yujun
Song, Yajun
author_facet Xiao, Liting
Jin, Junyan
Song, Kai
Qian, Xiuwei
Wu, Yarong
Sun, Zhulin
Xiong, Ziyao
Li, Yanbing
Zhao, Yanting
Shen, Leiming
Cui, Yiming
Yao, Wenwu
Cui, Yujun
Song, Yajun
author_sort Xiao, Liting
collection PubMed
description The bacterium Yersinia pestis has developed various strategies to sense and respond to the complex stresses encountered during its transmission and pathogenic processes. PurR is a common transcriptional regulator of purine biosynthesis among microorganisms, and it modulates the transcription level of the pur operon to suppress the production of hypoxanthine nucleotide (IMP). This study aims to understand the functions and regulatory mechanisms of purR in Y. pestis. Firstly, we constructed a purR knockout mutant of Y. pestis strain 201 and compared certain phenotypes of the null mutant (201-ΔpurR) and the wild-type strain (201-WT). The results show that deleting purR has no significant impact on the biofilm formation, growth rate, or viability of Y. pestis under different stress conditions (heat and cold shock, high salinity, and hyperosmotic pressure). Although the cytotoxicity of the purR knockout mutant on HeLa and 293 cells is reduced, the animal-challenging test found no difference of the virulence in mice between 201-ΔpurR and 201-WT. Furthermore, RNA-seq and EMSA analyses demonstrate that PurR binds to the promoter regions of at least 15 genes in Y. pestis strain 201, primarily involved in purine biosynthesis, along with others not previously observed in other bacteria. Additionally, RNA-seq results suggest the presence of 11 potential operons, including a newly identified co-transcriptional T6SS cluster. Thus, aside from its role as a regulator of purine biosynthesis, purR in Y. pestis may have additional regulatory functions.
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spelling pubmed-106736132023-11-17 Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities Xiao, Liting Jin, Junyan Song, Kai Qian, Xiuwei Wu, Yarong Sun, Zhulin Xiong, Ziyao Li, Yanbing Zhao, Yanting Shen, Leiming Cui, Yiming Yao, Wenwu Cui, Yujun Song, Yajun Microorganisms Article The bacterium Yersinia pestis has developed various strategies to sense and respond to the complex stresses encountered during its transmission and pathogenic processes. PurR is a common transcriptional regulator of purine biosynthesis among microorganisms, and it modulates the transcription level of the pur operon to suppress the production of hypoxanthine nucleotide (IMP). This study aims to understand the functions and regulatory mechanisms of purR in Y. pestis. Firstly, we constructed a purR knockout mutant of Y. pestis strain 201 and compared certain phenotypes of the null mutant (201-ΔpurR) and the wild-type strain (201-WT). The results show that deleting purR has no significant impact on the biofilm formation, growth rate, or viability of Y. pestis under different stress conditions (heat and cold shock, high salinity, and hyperosmotic pressure). Although the cytotoxicity of the purR knockout mutant on HeLa and 293 cells is reduced, the animal-challenging test found no difference of the virulence in mice between 201-ΔpurR and 201-WT. Furthermore, RNA-seq and EMSA analyses demonstrate that PurR binds to the promoter regions of at least 15 genes in Y. pestis strain 201, primarily involved in purine biosynthesis, along with others not previously observed in other bacteria. Additionally, RNA-seq results suggest the presence of 11 potential operons, including a newly identified co-transcriptional T6SS cluster. Thus, aside from its role as a regulator of purine biosynthesis, purR in Y. pestis may have additional regulatory functions. MDPI 2023-11-17 /pmc/articles/PMC10673613/ /pubmed/38004812 http://dx.doi.org/10.3390/microorganisms11112801 Text en © 2023 by the authors. https://creativecommons.org/licenses/by/4.0/Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Xiao, Liting
Jin, Junyan
Song, Kai
Qian, Xiuwei
Wu, Yarong
Sun, Zhulin
Xiong, Ziyao
Li, Yanbing
Zhao, Yanting
Shen, Leiming
Cui, Yiming
Yao, Wenwu
Cui, Yujun
Song, Yajun
Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities
title Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities
title_full Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities
title_fullStr Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities
title_full_unstemmed Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities
title_short Regulatory Functions of PurR in Yersinia pestis: Orchestrating Diverse Biological Activities
title_sort regulatory functions of purr in yersinia pestis: orchestrating diverse biological activities
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10673613/
https://www.ncbi.nlm.nih.gov/pubmed/38004812
http://dx.doi.org/10.3390/microorganisms11112801
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