Literature DB >> 17942612

Use of recombinant antigens to detect antibodies against Mycoplasma suis, with correlation of serological results to hematological findings.

Katharina Hoelzle1, Julia Grimm, Mathias Ritzmann, Karl Heinritzi, Paul Torgerson, Anja Hamburger, Max M Wittenbrink, Ludwig E Hoelzle.   

Abstract

Porcine eperythrozoonosis is a disease with worldwide distribution caused by the unculturable hemotrophic bacterium Mycoplasma suis. Current serological testing utilizes crude M. suis antigens purified from the blood of experimentally infected pigs. These antigens show high variability and are restricted to specialized laboratories. We evaluated a novel serological assay based on two recombinant M. suis antigens (rMSG1 and rHspA1). Antigen specificity was proven by means of sera raised against nonhemotrophic mycoplasma and other relevant bacteria. Using experimental and convalescent-phase sera, rMSG1 and rHspA1 enzyme-linked immunosorbent assays (ELISAs) demonstrated sensitivities, specificities, and predictive values (94.0 to 100.0%) equal to or higher than those of the M. suis whole-cell ELISA. Field samples from 120 weaning piglets grouped by quantitative PCR results were used to evaluate the diagnostic capability of the new ELISA systems in comparison to that of the whole-cell ELISA. Assuming a 100.0% specificity of the PCR, the whole-cell ELISA, rHspA1 ELISA, and rMSG1 ELISA showed specificities of 84.8%, 83.8%, and 90.6% and sensitivities of 61.5%, 74.0% and 58.1%, respectively. Cohen's kappa coefficients comparing the recombinant ELISAs to the whole-cell ELISA indicate moderate to substantial agreement. The detection of anti-MSG1 and/or anti-HspA1 antibodies in pigs was significantly correlated with decreased hematocrit, erythrocyte numbers, and hemoglobin concentrations, indicating that a single seropositive result is connected with clinical and etiological significance. In conclusion, rMSG1 and rHspA1 are sensitive and specific serological and infection markers which are for the first time used independently of animal experiments. They are especially fit to be used in routine diagnosis, pathogenesis studies, and large-scale epidemiological investigations.

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Year:  2007        PMID: 17942612      PMCID: PMC2168379          DOI: 10.1128/CVI.00345-07

Source DB:  PubMed          Journal:  Clin Vaccine Immunol        ISSN: 1556-679X


  17 in total

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Journal:  J Microbiol Methods       Date:  2007-05-29       Impact factor: 2.363

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  5 in total

1.  Seroprevalence of Mycoplasma suis infection in pigs in eastern China as estimated by a blocking enzyme-linked immunosorbent assay.

Authors:  Liang Zhongyang; Zhang Jiansong; Shen Yijuan; Xia Yuting; Li Yufeng; Xu Jiarong
Journal:  Can J Vet Res       Date:  2017-10       Impact factor: 1.310

2.  Identification of B cell epitopes in the MSG1 protein of Mycoplasma suis.

Authors:  Chen Chang; Yao Zou; Yufeng Li
Journal:  Monoclon Antib Immunodiagn Immunother       Date:  2014-08

3.  Cloning and expression of P67 protein of Mycoplasma leachii.

Authors:  Sabarinath Thankappan; Rajneesh Rana; Arun Thachappully Remesh; Valsala Rekha; Viswas Konasagara Nagaleekar; Bhavani Puvvala
Journal:  Vet World       Date:  2017-09-21

4.  In vivo transmission studies of 'Candidatus Mycoplasma turicensis' in the domestic cat.

Authors:  Kristina Museux; Felicitas S Boretti; Barbara Willi; Barbara Riond; Katharina Hoelzle; Ludwig E Hoelzle; Max M Wittenbrink; Séverine Tasker; Nicole Wengi; Claudia E Reusch; Hans Lutz; Regina Hofmann-Lehmann
Journal:  Vet Res       Date:  2009-05-16       Impact factor: 3.683

5.  New insights on the biology of swine respiratory tract mycoplasmas from a comparative genome analysis.

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Journal:  BMC Genomics       Date:  2013-03-14       Impact factor: 3.969

  5 in total

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