Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay

In the search for antigens with serodiagnostic potentials, the Neospora caninum immunodominant dense granule antigen, NCDG1 homologue was obtained after immunoscreening a N. caninum tachyzoite cDNA library. The hydrophobic signal peptide of this gene was truncated and expressed in E. coli as a solub...

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Main Author: Hara, Olgga Arriesgado
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Language:English
Published: Animo Repository 2005
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Online Access:https://animorepository.dlsu.edu.ph/etd_masteral/3301
https://animorepository.dlsu.edu.ph/cgi/viewcontent.cgi?article=10139&context=etd_masteral
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spelling oai:animorepository.dlsu.edu.ph:etd_masteral-101392022-06-01T02:26:42Z Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay Hara, Olgga Arriesgado In the search for antigens with serodiagnostic potentials, the Neospora caninum immunodominant dense granule antigen, NCDG1 homologue was obtained after immunoscreening a N. caninum tachyzoite cDNA library. The hydrophobic signal peptide of this gene was truncated and expressed in E. coli as a soluble fusion protein tagged with glutathione sepharose transferase (GST). With mouse anti-NCDG1t antibodies, NCDG1 was localized as granular, punctuate structures in the anterior and posterior portions of the N. caninum tachyzoites with an expected 33kda molecular weight. The recombinant antigen (GST-NCDG1t) retained its immunoreactivity in immune sera from N. caninum experimentally-infected dogs, and showed no cross reactivity with Toxoplasma gondii and other dog-related parasites such as Babesia gibsoni, Babesia canis canis, Babesia canis rossi, Babesia canis vogeli and Leishemania infantum. For large-scale screening of canine and bovine populations, the NCDG1t was evaluated for its diagnostic potential using enzyme linked immunosorbent assay (ELISA). The NCDG1t-ELISA clearly distinguished between N. caninum-positive and negative control dog and cow serum samples. Using NCDG1t-ELISA, 33 (23%) canine and 40 (40%) bovine and 9 (9.6%) canine and 9 (8.24%) bovine serum samples from selected areas in Japan and China tested positive, respectively. Test specificity for canine assay was demonstrated when NCDG1t-ELISA showed no reactivity with antibodies from dog sera experimentally infected with other parasites. In addition, 39 ELISA positive dog serum samples from Japan and China were confirmed positive by Western blot analysis while three samples were shown to be negative, showing 93% agreement between the two methods. For the bovine assay, a gold standard panel of bovine sera for ELISA was established to assess its diagnostic performance in terms of sensitivity and specificity. Although the specificity of NCDG1t-ELISA with respect to Western blot defined negative reference cow sera was high (97.6%), false-negatives were observed. But with a calculated sensitivity of 84.4%, NCDG1t-ELISA proved to be relatively reliable for the diagnosis of bovine neosporosis. However, the combined application of two recombinant antigens (e.g. NCDG1 and Nc SAG1) in the same immunoassay, is worth considering to further improve the sensitivity of NCDG1t-ELISA for diagnosis of bovine neosporosis. To date, this is the first N. caninum dense granule antigen-based ELISA for the diagnosis of canine neosporosis. Furthermore, this is the first reported survey of canine neosporosis in Nanjing and Yanbian provinces in China; and constitutes the second report in Japan using IFAT. 2005-05-01T07:00:00Z text application/pdf https://animorepository.dlsu.edu.ph/etd_masteral/3301 https://animorepository.dlsu.edu.ph/cgi/viewcontent.cgi?article=10139&context=etd_masteral Master's Theses English Animo Repository Serodiagnosis Immunoassay Antigens Dogs Immunoenzyme technique Biology
institution De La Salle University
building De La Salle University Library
continent Asia
country Philippines
Philippines
content_provider De La Salle University Library
collection DLSU Institutional Repository
language English
topic Serodiagnosis
Immunoassay
Antigens
Dogs
Immunoenzyme technique
Biology
spellingShingle Serodiagnosis
Immunoassay
Antigens
Dogs
Immunoenzyme technique
Biology
Hara, Olgga Arriesgado
Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay
description In the search for antigens with serodiagnostic potentials, the Neospora caninum immunodominant dense granule antigen, NCDG1 homologue was obtained after immunoscreening a N. caninum tachyzoite cDNA library. The hydrophobic signal peptide of this gene was truncated and expressed in E. coli as a soluble fusion protein tagged with glutathione sepharose transferase (GST). With mouse anti-NCDG1t antibodies, NCDG1 was localized as granular, punctuate structures in the anterior and posterior portions of the N. caninum tachyzoites with an expected 33kda molecular weight. The recombinant antigen (GST-NCDG1t) retained its immunoreactivity in immune sera from N. caninum experimentally-infected dogs, and showed no cross reactivity with Toxoplasma gondii and other dog-related parasites such as Babesia gibsoni, Babesia canis canis, Babesia canis rossi, Babesia canis vogeli and Leishemania infantum. For large-scale screening of canine and bovine populations, the NCDG1t was evaluated for its diagnostic potential using enzyme linked immunosorbent assay (ELISA). The NCDG1t-ELISA clearly distinguished between N. caninum-positive and negative control dog and cow serum samples. Using NCDG1t-ELISA, 33 (23%) canine and 40 (40%) bovine and 9 (9.6%) canine and 9 (8.24%) bovine serum samples from selected areas in Japan and China tested positive, respectively. Test specificity for canine assay was demonstrated when NCDG1t-ELISA showed no reactivity with antibodies from dog sera experimentally infected with other parasites. In addition, 39 ELISA positive dog serum samples from Japan and China were confirmed positive by Western blot analysis while three samples were shown to be negative, showing 93% agreement between the two methods. For the bovine assay, a gold standard panel of bovine sera for ELISA was established to assess its diagnostic performance in terms of sensitivity and specificity. Although the specificity of NCDG1t-ELISA with respect to Western blot defined negative reference cow sera was high (97.6%), false-negatives were observed. But with a calculated sensitivity of 84.4%, NCDG1t-ELISA proved to be relatively reliable for the diagnosis of bovine neosporosis. However, the combined application of two recombinant antigens (e.g. NCDG1 and Nc SAG1) in the same immunoassay, is worth considering to further improve the sensitivity of NCDG1t-ELISA for diagnosis of bovine neosporosis. To date, this is the first N. caninum dense granule antigen-based ELISA for the diagnosis of canine neosporosis. Furthermore, this is the first reported survey of canine neosporosis in Nanjing and Yanbian provinces in China; and constitutes the second report in Japan using IFAT.
format text
author Hara, Olgga Arriesgado
author_facet Hara, Olgga Arriesgado
author_sort Hara, Olgga Arriesgado
title Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay
title_short Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay
title_full Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay
title_fullStr Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay
title_full_unstemmed Serodiagnosis of canine and bovine neosporosis using a recombinant truncated NCDG1 protein in an enzyme-linked immunosorbent assay
title_sort serodiagnosis of canine and bovine neosporosis using a recombinant truncated ncdg1 protein in an enzyme-linked immunosorbent assay
publisher Animo Repository
publishDate 2005
url https://animorepository.dlsu.edu.ph/etd_masteral/3301
https://animorepository.dlsu.edu.ph/cgi/viewcontent.cgi?article=10139&context=etd_masteral
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