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Detection of Salmonella spp. Using a Generic and Differential FRET-PCR

To facilitate the detection of Salmonella and to be able to rapidly and conveniently determine the species/subspecies present, we developed and tested a generic and differential FRET-PCR targeting their tetrathionate reductase response regulator gene. The differential pan-Salmonella FRET-PCR we deve...

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Autores principales: Zhang, Jilei, Wei, Lanjing, Kelly, Patrick, Freeman, Mark, Jaegerson, Kirsten, Gong, Jiansen, Xu, Bu, Pan, Zhiming, Xu, Chuanling, Wang, Chengming
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2013
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3797804/
https://www.ncbi.nlm.nih.gov/pubmed/24146814
http://dx.doi.org/10.1371/journal.pone.0076053
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author Zhang, Jilei
Wei, Lanjing
Kelly, Patrick
Freeman, Mark
Jaegerson, Kirsten
Gong, Jiansen
Xu, Bu
Pan, Zhiming
Xu, Chuanling
Wang, Chengming
author_facet Zhang, Jilei
Wei, Lanjing
Kelly, Patrick
Freeman, Mark
Jaegerson, Kirsten
Gong, Jiansen
Xu, Bu
Pan, Zhiming
Xu, Chuanling
Wang, Chengming
author_sort Zhang, Jilei
collection PubMed
description To facilitate the detection of Salmonella and to be able to rapidly and conveniently determine the species/subspecies present, we developed and tested a generic and differential FRET-PCR targeting their tetrathionate reductase response regulator gene. The differential pan-Salmonella FRET-PCR we developed successfully detected seven plasmids that contained partial sequences of S. bongori and the six S. enterica subspecies. The detection limit varied from ∼5 copies of target gene/per PCR reaction for S. enterica enterica to ∼200 for S. bongori. Melting curve analysis demonstrated a T (m) of ∼68°C for S. enterica enterica, ∼62.5°C for S. enterica houtenae and S. enterica diarizonae, ∼57°C for S. enterica indica, and ∼54°C for S. bongori, S. enterica salamae and S. enterica arizonae. The differential pan-Salmonella FRET-PCR also detected and determined the subspecies of 4 reference strains and 47 Salmonella isolated from clinically ill birds or pigs. Finally, we found it could directly detect and differentiate Salmonella in feline (5/50 positive; 10%; one S. enterica salamae and 4 S. enterica enterica) and canine feces (15/114 positive; 13.2%; all S. enterica enterica). The differential pan-Salmonella FRET-PCR failed to react with 96 non-Salmonella bacterial strains. Our experiments show the differential pan-Salmonella FRET-PCR we developed is a rapid, sensitive and specific method to detect and differentiate Salmonella.
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spelling pubmed-37978042013-10-21 Detection of Salmonella spp. Using a Generic and Differential FRET-PCR Zhang, Jilei Wei, Lanjing Kelly, Patrick Freeman, Mark Jaegerson, Kirsten Gong, Jiansen Xu, Bu Pan, Zhiming Xu, Chuanling Wang, Chengming PLoS One Research Article To facilitate the detection of Salmonella and to be able to rapidly and conveniently determine the species/subspecies present, we developed and tested a generic and differential FRET-PCR targeting their tetrathionate reductase response regulator gene. The differential pan-Salmonella FRET-PCR we developed successfully detected seven plasmids that contained partial sequences of S. bongori and the six S. enterica subspecies. The detection limit varied from ∼5 copies of target gene/per PCR reaction for S. enterica enterica to ∼200 for S. bongori. Melting curve analysis demonstrated a T (m) of ∼68°C for S. enterica enterica, ∼62.5°C for S. enterica houtenae and S. enterica diarizonae, ∼57°C for S. enterica indica, and ∼54°C for S. bongori, S. enterica salamae and S. enterica arizonae. The differential pan-Salmonella FRET-PCR also detected and determined the subspecies of 4 reference strains and 47 Salmonella isolated from clinically ill birds or pigs. Finally, we found it could directly detect and differentiate Salmonella in feline (5/50 positive; 10%; one S. enterica salamae and 4 S. enterica enterica) and canine feces (15/114 positive; 13.2%; all S. enterica enterica). The differential pan-Salmonella FRET-PCR failed to react with 96 non-Salmonella bacterial strains. Our experiments show the differential pan-Salmonella FRET-PCR we developed is a rapid, sensitive and specific method to detect and differentiate Salmonella. Public Library of Science 2013-10-16 /pmc/articles/PMC3797804/ /pubmed/24146814 http://dx.doi.org/10.1371/journal.pone.0076053 Text en © 2013 Zhang et al 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
Zhang, Jilei
Wei, Lanjing
Kelly, Patrick
Freeman, Mark
Jaegerson, Kirsten
Gong, Jiansen
Xu, Bu
Pan, Zhiming
Xu, Chuanling
Wang, Chengming
Detection of Salmonella spp. Using a Generic and Differential FRET-PCR
title Detection of Salmonella spp. Using a Generic and Differential FRET-PCR
title_full Detection of Salmonella spp. Using a Generic and Differential FRET-PCR
title_fullStr Detection of Salmonella spp. Using a Generic and Differential FRET-PCR
title_full_unstemmed Detection of Salmonella spp. Using a Generic and Differential FRET-PCR
title_short Detection of Salmonella spp. Using a Generic and Differential FRET-PCR
title_sort detection of salmonella spp. using a generic and differential fret-pcr
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3797804/
https://www.ncbi.nlm.nih.gov/pubmed/24146814
http://dx.doi.org/10.1371/journal.pone.0076053
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