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Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni

Campylobacter jejuni genetic manipulation is restricted by the limited number of antibiotic resistance cassettes available for use in this diarrheal pathogen. In this study, two antibiotic resistance cassettes were developed, encoding for hygromycin B and apramycin resistance, for use in mutagenesis...

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Autores principales: Cameron, Andrew, Gaynor, Erin C.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2014
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3994027/
https://www.ncbi.nlm.nih.gov/pubmed/24751825
http://dx.doi.org/10.1371/journal.pone.0095084
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author Cameron, Andrew
Gaynor, Erin C.
author_facet Cameron, Andrew
Gaynor, Erin C.
author_sort Cameron, Andrew
collection PubMed
description Campylobacter jejuni genetic manipulation is restricted by the limited number of antibiotic resistance cassettes available for use in this diarrheal pathogen. In this study, two antibiotic resistance cassettes were developed, encoding for hygromycin B and apramycin resistance, for use in mutagenesis or for selection of gene expression and complementation constructs in C. jejuni. First, the marker genes were successfully modified to allow for insertional mutagenesis or deletion of a gene-of-interest, and were bracketed with restriction sites for the facilitation of site-specific cloning. These hygromycin B and apramycin markers are encoded by plasmids pAC1H and pAC1A, respectively. We also modified an insertional gene-delivery vector to create pRRH and pRRA, containing the hygromycin B and apramycin resistance genes, and 3 unique restriction sites for the directional introduction of genes into the conserved multi-copy rRNA gene clusters of the C. jejuni chromosome. We determined the effective antibiotic concentrations required for selection, and established that no harmful effects or fitness costs were associated with carrying hygromycin B or apramycin resistance under standard C. jejuni laboratory conditions. Using these markers, the arylsulfatase reporter gene astA was deleted, and the ability to genetically complement the astA deletion using pRRH and pRRA for astA gene insertion was demonstrated. Furthermore, the relative levels of expression from the endogenous astA promoter were compared to that of polycistronic mRNA expression from the constitutive promoter upstream of the resistance gene. The development of additional antibiotic resistance cassettes for use in Campylobacter will enable multiple gene deletion and expression combinations as well as more in-depth study of multi-gene systems important for the survival and pathogenesis of this important bacterium.
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spelling pubmed-39940272014-04-25 Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni Cameron, Andrew Gaynor, Erin C. PLoS One Research Article Campylobacter jejuni genetic manipulation is restricted by the limited number of antibiotic resistance cassettes available for use in this diarrheal pathogen. In this study, two antibiotic resistance cassettes were developed, encoding for hygromycin B and apramycin resistance, for use in mutagenesis or for selection of gene expression and complementation constructs in C. jejuni. First, the marker genes were successfully modified to allow for insertional mutagenesis or deletion of a gene-of-interest, and were bracketed with restriction sites for the facilitation of site-specific cloning. These hygromycin B and apramycin markers are encoded by plasmids pAC1H and pAC1A, respectively. We also modified an insertional gene-delivery vector to create pRRH and pRRA, containing the hygromycin B and apramycin resistance genes, and 3 unique restriction sites for the directional introduction of genes into the conserved multi-copy rRNA gene clusters of the C. jejuni chromosome. We determined the effective antibiotic concentrations required for selection, and established that no harmful effects or fitness costs were associated with carrying hygromycin B or apramycin resistance under standard C. jejuni laboratory conditions. Using these markers, the arylsulfatase reporter gene astA was deleted, and the ability to genetically complement the astA deletion using pRRH and pRRA for astA gene insertion was demonstrated. Furthermore, the relative levels of expression from the endogenous astA promoter were compared to that of polycistronic mRNA expression from the constitutive promoter upstream of the resistance gene. The development of additional antibiotic resistance cassettes for use in Campylobacter will enable multiple gene deletion and expression combinations as well as more in-depth study of multi-gene systems important for the survival and pathogenesis of this important bacterium. Public Library of Science 2014-04-21 /pmc/articles/PMC3994027/ /pubmed/24751825 http://dx.doi.org/10.1371/journal.pone.0095084 Text en © 2014 Cameron, Gaynor http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Cameron, Andrew
Gaynor, Erin C.
Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni
title Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni
title_full Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni
title_fullStr Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni
title_full_unstemmed Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni
title_short Hygromycin B and Apramycin Antibiotic Resistance Cassettes for Use in Campylobacter jejuni
title_sort hygromycin b and apramycin antibiotic resistance cassettes for use in campylobacter jejuni
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3994027/
https://www.ncbi.nlm.nih.gov/pubmed/24751825
http://dx.doi.org/10.1371/journal.pone.0095084
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