Development of a Recombinant Protein-Based Enzyme-Linked Immunosorbent Assay for Diagnosis of Mycoplasma bovis Infection in Cattle

Wawegama, Nadeeka K.; Browning, Glenn F.; Kanci, Anna; Marenda, Marc S.; Markham, Philip F.

doi:10.1128/cvi.00670-13

Cited by 81 publications

(111 citation statements)

References 34 publications

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“…It was indicated that the identification of M. bovis strains in cattle herds and the evaluation of their pathogenicity and antigenic variation is important (Behrens et al, 1994). P48 is a membranous lipoprotein of 48kDa weight that is homologous to the family of the Macrophage Activator Lipoproteins (MALPs) and is coded via a conserved sequence specific to the M. bovis species (Wawegama et al, 2014). As the P48 gene is a conserved sequence in all M. bovis strains, designed primers by Fu (Fu et al, 2014), were used for amplification the P48 gene in this study.…”

Section: Mycoplasmamentioning

confidence: 99%

“…Traditional methods of detection and isolation of Mycoplasma strains such as serological and culture methods are time consuming, so the more sensitive biological methods such as PCR, are widely used for the detection and molecular analysis of various bacteria such as M. bovis strains in every microbial laboratories worldwide (Kirk and Lauerman, 1994). P48 is a membranous lipoprotein of slightly lower than 48kDa that is homologous to the family of the Macrophage Activator Lipoproteins (MALPs) and it is coded via a conserved sequences specific to the M. bovis species (Wawegama et al, 2014), so the sequence of M. bovis strain PG45 under accession number of CP002188 was selected (Wise et al, 2011) to compare with the strains detected in this study. The encoding gene sequence of lipoprotein P48 is recorded as accession numbers of DQ020481 and DQ020482 at Gene Bank (Lysnyansky et al, 2008) and it is known as one of the virulence factors of M. bovis species (Li et al, 2011).…”

Section: Introductionmentioning

confidence: 99%

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Isolation, identification and molecular characterization of Mycoplasma bovis in mastitic dairy cattle by PCR and culture methods

Imandar

Pourbakhsh

Jamshidian

et al. 2018

J Hellenic Vet Med Soc

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Mycoplasma bovis is well known as one of the major causative agents of mastitis in dairy cattle herds. The aim of this study was the identification of Mycoplasma bovis strains by PCR and traditional culture methods from a total number of 328 milk samples collected from cows with clinical mastitis symptoms from all over Iran. First step cultures in PPLO broth and agar showed 58 samples (17.69%) as positive. Out of 328 samples, 97 samples (29.57%) were positive for Mycoplasma genus according to the amplification of the 16SrRNA gene performed by PCR and from them, 31 (31.97%) samples were positive by PCR on the P48 gene. The purified P48 positive PCR products were sequenced and results were compared to M. bovis reference strain PG45 (CP002188). A phylogenic tree was created using Neighbor-joining method in MEGA6 software. The studied strain IB220 showed 100% identity with the reference strain of M. bovis and followed the same phylogenetic roots while studied strain IB216 showed 99.7% homology with the reference strain. Twelve selected geographical isolated strains were subjected to Gene Bank under accession numbers of KX772789 to KX772800. This is the first study of the molecular characterization of Mycoplasma bovis in dairy cattle with clinical mastitis from Iran.

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Section: Mycoplasmamentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Isolation, identification and molecular characterization of Mycoplasma bovis in mastitic dairy cattle by PCR and culture methods

Imandar

Pourbakhsh

Jamshidian

et al. 2018

J Hellenic Vet Med Soc

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Section: Protein Milamentioning

confidence: 99%

“…More recently, a novel 226 kDa protein encoded by the milA gene (MBOVPG45_0710) was characterised from the M. bovis field strain 3683 and investigated for use in the sero-diagnosis of experimental M. bovis infections in calves in Australia (Wawegama et al, 2014). Analysis by the authors revealed that the milA protein contained a membrane spanning region at its amino terminal end, with the remainder of the protein predicted to be located extracellularly (Wawegama et al, 2014).…”

Section: Protein Milamentioning

confidence: 99%

“…Analysis by the authors revealed that the milA protein contained a membrane spanning region at its amino terminal end, with the remainder of the protein predicted to be located extracellularly (Wawegama et al, 2014). Homologues were found in both Hubei-1 and HB0801 M. bovis strains for which complete genome sequences are available, as well as M. agalactiae strains 5632 and PG2 (Wawegama et al, 2014). This high molecular weight protein was reported by the authors to be immuno-reactive by western blotting to M. bovis-specific calf sera and unlike the Vsps, the milA protein did not appear to undergo phase or antigenic variation (Wawegama et al, 2014).…”

Section: Protein Milamentioning

confidence: 99%

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Mycoplasma bovis in Australian feeder cattle

Schibrowski¹

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Mycoplasma bovis can be a commensal bacterial inhabitant of the upper respiratory tract of healthy bovines. However, under certain circumstances and conditions that are incompletely understood, M. bovis can be associated with a number of clinical syndromes, one of which is bovine respiratory disease (BRD). In Australia, there is little information on the prevalence and epidemiology M. bovis in beef production systems. The overall aim of this thesis was to help close this knowledge gap.Commercially available serological diagnostic methods for the detection of M. bovis-specific antibody have not been validated in the Australian cattle population. Arguably, more importantly, however is the fact that diagnostic sensitivity (Se) and specificity (Sp) and / or analytical sensitivity (ASe) and specificity (ASp) estimates for commercially available M. bovis sero-diagnostic tests are not available. 28% (95% CI: 1% -92%). However, in terms of Sp the commercial ELISAs out performed western blotting; BioK302: 96% (95% CI: 87% -99%); BioK260:100% (95% CI: 93% -100%) and western blotting: 88% (95% CI: 56% -98%) respectively. In terms of both Se and Sp combined, none of the methods assessed here performed well. As such, when interpreting the results obtained from these ELISAs, the potential impact imperfect Se and / or Sp can have needs to be considered.Despite the poor performance of the BioK302 and BioK260 ELISAs particularly in terms of Se, these tests were used to determine the sero-prevalence of M. bovis antibody in Australian feeder cattle at feedlot induction and draft (approximately 42 days on feed). Paired bovine sera from 1,354 randomly selected animals were sourced from a bovine serum bank (n = 35,160) collected as part of another study, The National Bovine Respiratory Disease Initiative. As the classification of the result of a single serum sample could differ between the BioK302 and BioK260, sero-prevalence estimates were obtained using the individual ELISA results in addition to series and parallel interpretation of the two ELISA kit results. The apparent sero-prevalence of M. bovis-specific antibody at feedlot induction estimates ranged from 2.4% -6.8% (95% CI: 1.3% -8.6%) and the apparent sero-prevalence estimates at draft ranged from 22.4% -44.2% (95% CI: 19.1% -48.6%). The level of sero-conversion to M. bovis between induction and draft was also determined. Only animals that were classified as sero-negative at induction were included in sero-conversion analyses. In the current study, 24.3% (95% iii CI: 20.8% -27.7%) and 19.5% (95% CI: 17.3% -21.7%) of animals sero-converted to M. bovis between induction and draft based on the BioK302 and dichotomised BioK260 ELISA results respectively.Using these ELISA results, an assessment of putative risk factors associated with sero-positivity at feedlot induction or sero-conversion between induction and draft was performed. An increased risk of sero-positivity at feedlot induction was found to be associated with; (i) history of exposure to a saleyard at least 27 d...

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Comparison and optimisation of screening cutoff values for Mycoplasma bovis antibody ELISAs using serum from youngstock

2022

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Background Mycoplasma bovis‐associated disease can cause tremendous production losses, welfare issues and high antimicrobial use. Therefore, screening cattle for M. bovis antibodies before entering the herd is a popular and possibly cost‐efficient way to reduce disease introduction. However, interpretation of results can be challenging due to variable accuracy between tests and populations. This study's objectives were to compare the diagnostic test accuracy of three commercially available M. bovis antibody ELISAs (ID‐screen, Bio K302 and Bio K432) and to explore optimal cutoff values for screening purposes. Methods A prospective diagnostic test accuracy study was performed on 170 serum samples from youngstock using Bayesian latent class modelling. Samples were categorised using manufacturer and generated cutoff values. Results Using the manufacturers' guidelines, ID‐screen, Bio K432 and Bio K302 showed 97.6%, 67.4% and 33.6% sensitivity, and 78.8%, 97.6% and 99.1% specificity, respectively. Optimised cutoffs resulted in 94.8%, 82.6% and 78.3% sensitivity, and 94.2%, 92.5% and 79.4% specificity, respectively. Conclusions The highest diagnostic accuracy for detecting M. bovis antibodies was obtained by ID‐screen (≥110%). However, by adjusting cutoff values, the sensitivity of Bio‐X tests could be markedly increased, making these tests also applicable as screening tools. Limitations Interpretation needs to be careful as antibodies may be linked to both infectious and non‐infectious status.

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Development of a Recombinant Protein-Based Enzyme-Linked Immunosorbent Assay for Diagnosis of Mycoplasma bovis Infection in Cattle

Cited by 81 publications

References 34 publications

Isolation, identification and molecular characterization of Mycoplasma bovis in mastitic dairy cattle by PCR and culture methods

Isolation, identification and molecular characterization of Mycoplasma bovis in mastitic dairy cattle by PCR and culture methods

Mycoplasma bovis in Australian feeder cattle

Comparison and optimisation of screening cutoff values for Mycoplasma bovis antibody ELISAs using serum from youngstock

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