Detection of Mycoplasma anatis, M. anseris, M. cloacale and Mycoplasma sp. 1220 in waterfowl using species-specific PCR assays.
Animals
Animals, Wild
/ microbiology
Bird Diseases
/ microbiology
Birds
/ microbiology
Chickens
/ microbiology
DNA Primers
/ genetics
DNA, Bacterial
/ genetics
Ducks
/ microbiology
Geese
/ microbiology
Genes, Bacterial
Mycoplasma
/ classification
Mycoplasma Infections
/ microbiology
Polymerase Chain Reaction
/ methods
Species Specificity
Turkeys
/ microbiology
Journal
PloS one
ISSN: 1932-6203
Titre abrégé: PLoS One
Pays: United States
ID NLM: 101285081
Informations de publication
Date de publication:
2019
2019
Historique:
received:
17
12
2018
accepted:
14
06
2019
entrez:
12
7
2019
pubmed:
12
7
2019
medline:
3
3
2020
Statut:
epublish
Résumé
Mycoplasma anatis, M. anseris, M. cloacale and M. sp. 1220 colonise geese and ducks, and could be associated with infections of avian respiratory and nervous systems, cause mild to severe inflammation of cloaca and genital tracts, and embryo lethality. Co-occurrence of these Mycoplasma species in waterfowl is frequently detected and the identification of these mycoplasmas to the species level at a regular microbiology laboratory is difficult due to their similar morphological, cultural and biochemical properties. Moreover, species differentiation is only possible based on the sequence analysis of the product of a genus-specific PCR assay. Therefore, the aim of the current study was to develop an effective and robust method for the identification of these species in avian clinical specimens. Polymerase chain reaction (PCR) assays using species-specific primers, which target housekeeping genes in order to identify these species, were designed in the present study. The developed PCR assays can precisely identify these four mycoplasmas to the species level directly from DNA samples extracted from clinical specimens, and no cross-amplification was observed among these species and with other well-known avian mycoplasmas. The average sensitivity of the assays was 101-102 genomic equivalents per reaction. These conventional PCR assays can be run simultaneously at the same PCR cycling program, and the species can be differentiated directly (without sequence analysis) by gel electrophoresis due to the specific sizes of the amplicons. In conclusion, the presented species-specific assays were found to be suitable for routine use at regular veterinary diagnostic laboratories and promote the rapid, simple and cost-effective differentiation of these waterfowl Mycoplasma species.
Identifiants
pubmed: 31295269
doi: 10.1371/journal.pone.0219071
pii: PONE-D-18-35971
pmc: PMC6622482
doi:
Substances chimiques
DNA Primers
0
DNA, Bacterial
0
Types de publication
Journal Article
Research Support, Non-U.S. Gov't
Langues
eng
Sous-ensembles de citation
IM
Pagination
e0219071Déclaration de conflit d'intérêts
The TOLL 96 Kft. provided support in the form of salaries for MJK. This does not alter our adherence to PLOS ONE policies on sharing data and materials.
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