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Development and evaluation of recombinant GRA8 protein for the serodiagnosis of Toxoplasma gondii infection in goats
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Abstract
Background
The development of sensitive and specific methods for detecting
Toxoplasma gondii
infection is critical for preventing and controlling toxoplasmosis in humans and other animals. Recently, various recombinant proteins have been used in serological tests for diagnosing toxoplasmosis. The production of these antigens is associated with live tachyzoites obtained from cell cultures or laboratory animals for genomic extraction to amplify target genes. Synthetic genes have gained a key role in recombinant protein production. For the first time, we demonstrated the production of the recombinant protein of the
T. gondii
dense granular antigen 8 (TgGRA8) gene based on commercial gene synthesis. Recombinant TgGRA8 plasmids were successfully expressed in an
Escherichia coli
system. The recombinant protein was affinity-purified and characterized via sodium dodecyl sulfate-polyacrylamide gel electrophoresis and Western blotting. Furthermore, the diagnostic potential of the recombinant protein was assessed using 306 field serum samples from goats via indirect enzyme-linked immunosorbent assay (iELISA) and the latex agglutination test (LAT).
Results
Western blotting using known positive serum samples from goats identified a single antigen at the expected molecular weight of TgGRA8 (27 kDa). iELISA illustrated that 15.40% of goat samples were positive for
T. gondii
-specific IgG antibodies. In addition, TgGRA8 provided high sensitivity and specificity, with significant concordance (91.83) and kappa values (0.69) compared with the results obtained using LAT.
Conclusion
Our findings highlight the production of a recombinant protein from a synthetic TgGRA8 gene and the ability to detect
T. gondii
infection in field samples. The sensitivity and specificity of TgGRA8 demonstrated that this protein could be a good serological marker for detecting specific IgG in goat sera.
Springer Science and Business Media LLC
Title: Development and evaluation of recombinant GRA8 protein for the serodiagnosis of Toxoplasma gondii infection in goats
Description:
Abstract
Background
The development of sensitive and specific methods for detecting
Toxoplasma gondii
infection is critical for preventing and controlling toxoplasmosis in humans and other animals.
Recently, various recombinant proteins have been used in serological tests for diagnosing toxoplasmosis.
The production of these antigens is associated with live tachyzoites obtained from cell cultures or laboratory animals for genomic extraction to amplify target genes.
Synthetic genes have gained a key role in recombinant protein production.
For the first time, we demonstrated the production of the recombinant protein of the
T.
gondii
dense granular antigen 8 (TgGRA8) gene based on commercial gene synthesis.
Recombinant TgGRA8 plasmids were successfully expressed in an
Escherichia coli
system.
The recombinant protein was affinity-purified and characterized via sodium dodecyl sulfate-polyacrylamide gel electrophoresis and Western blotting.
Furthermore, the diagnostic potential of the recombinant protein was assessed using 306 field serum samples from goats via indirect enzyme-linked immunosorbent assay (iELISA) and the latex agglutination test (LAT).
Results
Western blotting using known positive serum samples from goats identified a single antigen at the expected molecular weight of TgGRA8 (27 kDa).
iELISA illustrated that 15.
40% of goat samples were positive for
T.
gondii
-specific IgG antibodies.
In addition, TgGRA8 provided high sensitivity and specificity, with significant concordance (91.
83) and kappa values (0.
69) compared with the results obtained using LAT.
Conclusion
Our findings highlight the production of a recombinant protein from a synthetic TgGRA8 gene and the ability to detect
T.
gondii
infection in field samples.
The sensitivity and specificity of TgGRA8 demonstrated that this protein could be a good serological marker for detecting specific IgG in goat sera.
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