A nested-PCR strategy for molecular diagnosis of mollicutes in uncultured biological samples from cows with vulvovaginitis

A nested-PCR strategy for molecular diagnosis of mollicutes in uncultured biological samples from cows with vulvovaginitis

•The nested-PCR designed was adequate for molecular diagnosis of mollicutes.•A high frequency of Ureaplasma diversum was observed within affected cows.•Mollicutes were detected in cattle herds with AI, FTAI, and ET implemented. Bacteria classified in Mycoplasma (M. bovis and M. bovigenitalium) and U...

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Veröffentlicht in:Animal reproduction science 2018-01, Vol.188, p.137-143
Hauptverfasser: Voltarelli, Daniele Cristina, de Alcântara, Brígida Kussumoto, Lunardi, Michele, Alfieri, Alice Fernandes, de Arruda Leme, Raquel, Alfieri, Amauri Alcindo
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Cattle
Mycoplasma bovigenitalium
Mycoplasma bovis
Reproductive disease
Ureaplasma diversum
Vaginal swab
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container_end_page 143
container_issue
container_start_page 137
container_title Animal reproduction science
container_volume 188
creator Voltarelli, Daniele Cristina
de Alcântara, Brígida Kussumoto
Lunardi, Michele
Alfieri, Alice Fernandes
de Arruda Leme, Raquel
Alfieri, Amauri Alcindo
description •The nested-PCR designed was adequate for molecular diagnosis of mollicutes.•A high frequency of Ureaplasma diversum was observed within affected cows.•Mollicutes were detected in cattle herds with AI, FTAI, and ET implemented. Bacteria classified in Mycoplasma (M. bovis and M. bovigenitalium) and Ureaplasma (U. diversum) genera are associated with granular vulvovaginitis that affect heifers and cows at reproductive age. The traditional means for detection and speciation of mollicutes from clinical samples have been culture and serology. However, challenges experienced with these laboratory methods have hampered assessment of their impact in pathogenesis and epidemiology in cattle worldwide. The aim of this study was to develop a PCR strategy to detect and primarily discriminate between the main species of mollicutes associated with reproductive disorders of cattle in uncultured clinical samples. In order to amplify the 16S-23S rRNA internal transcribed spacer region of the genome, a consensual and species-specific nested-PCR assay was developed to identify and discriminate between main species of mollicutes. In addition, 31 vaginal swab samples from dairy and beef affected cows were investigated. This nested-PCR strategy was successfully employed in the diagnosis of single and mixed mollicute infections of diseased cows from cattle herds from Brazil. The developed system enabled the rapid and unambiguous identification of the main mollicute species known to be associated with this cattle reproductive disorder through differential amplification of partial fragments of the ITS region of mollicute genomes. The development of rapid and sensitive tools for mollicute detection and discrimination without the need for previous cultures or sequencing of PCR products is a high priority for accurate diagnosis in animal health. Therefore, the PCR strategy described herein may be helpful for diagnosis of this class of bacteria in genital swabs submitted to veterinary diagnostic laboratories, not demanding expertise in mycoplasma culture and identification.
doi_str_mv 10.1016/j.anireprosci.2017.11.018
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This nested-PCR strategy was successfully employed in the diagnosis of single and mixed mollicute infections of diseased cows from cattle herds from Brazil. The developed system enabled the rapid and unambiguous identification of the main mollicute species known to be associated with this cattle reproductive disorder through differential amplification of partial fragments of the ITS region of mollicute genomes. The development of rapid and sensitive tools for mollicute detection and discrimination without the need for previous cultures or sequencing of PCR products is a high priority for accurate diagnosis in animal health. 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subjects Cattle
Mycoplasma bovigenitalium
Mycoplasma bovis
Reproductive disease
Ureaplasma diversum
Vaginal swab
title A nested-PCR strategy for molecular diagnosis of mollicutes in uncultured biological samples from cows with vulvovaginitis
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