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dc.contributor.author
Pérez Filgueira, Daniel Mariano  
dc.contributor.author
González Camacho, F.  
dc.contributor.author
Gallardo, C.  
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Resino Talavan, P.  
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Blanco, E.  
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Gomez Casado, E.  
dc.contributor.author
Alonso, C.  
dc.contributor.author
Escribano, J. M.  
dc.date.available
2024-09-20T10:46:37Z  
dc.date.issued
2006-12  
dc.identifier.citation
Pérez Filgueira, Daniel Mariano; González Camacho, F.; Gallardo, C.; Resino Talavan, P.; Blanco, E.; et al.; Optimization and Validation of Recombinant Serological Tests for African Swine Fever Diagnosis Based on Detection of the p30 Protein Produced in Trichoplusia ni Larvae; American Society for Microbiology; Journal of Clinical Microbiology; 44; 9; 12-2006; 3114-3121  
dc.identifier.issn
0095-1137  
dc.identifier.uri
http://hdl.handle.net/11336/244667  
dc.description.abstract
We describe the validation of an enzyme-linked immunosorbent assay (ELISA) and confirmatory immunoblotting assays based on a recombinant p30 protein (p30r) produced in insect larvae using a baculovirus vector. Such validation included the following: (i) the scaling up and standardization of p30r production and the associated immunoassays, (ii) a broad immunological analysis using a large number of samples (a total of 672) from Spain and different African locations, and (iii) the detection of the ASF virus (ASFV)-antibody responses at different times after experimental infection. Yields of p30r reached up to 15% of the total protein recovered from the infected larvae at 3 days postinfection. Serological analysis of samples collected in Spain revealed that the p30r-based ELISA presented similar sensitivity to and higher specificity than the conventional Office International des Epizooties-approved ASFV ELISA. Moreover, the p30r ELISA was more sensitive than the conventional ELISA test in detecting ASFV-specific antibodies in experimentally infected animals at early times postinfection. Both the recombinant and conventional ELISAs presented variable rates of sensitivity and specificity with African samples, apparently related to their geographical origin. Comparative analyses performed on the sequences, predicted structures, and antigenicities of p30 proteins from different Spanish and African isolates suggested that variability among isolates might correlate with changes in antigenicity, thus affecting detection by the p30r ELISA. Our estimations indicate that more than 40,000 ELISA determinations and 2,000 confirmatory immunoblotting tests can be performed with the p30r protein obtained from a single infected larva, making this a feasible and inexpensive strategy for production of serological tests with application in developing countries.  
dc.format
application/pdf  
dc.language.iso
eng  
dc.publisher
American Society for Microbiology  
dc.rights
info:eu-repo/semantics/openAccess  
dc.rights.uri
https://creativecommons.org/licenses/by-nc-sa/2.5/ar/  
dc.subject
p30  
dc.subject.classification
Virología  
dc.subject.classification
Ciencias Biológicas  
dc.subject.classification
CIENCIAS NATURALES Y EXACTAS  
dc.title
Optimization and Validation of Recombinant Serological Tests for African Swine Fever Diagnosis Based on Detection of the p30 Protein Produced in Trichoplusia ni Larvae  
dc.type
info:eu-repo/semantics/article  
dc.type
info:ar-repo/semantics/artículo  
dc.type
info:eu-repo/semantics/publishedVersion  
dc.date.updated
2024-09-19T13:48:41Z  
dc.journal.volume
44  
dc.journal.number
9  
dc.journal.pagination
3114-3121  
dc.journal.pais
Estados Unidos  
dc.description.fil
Fil: Pérez Filgueira, Daniel Mariano. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina  
dc.description.fil
Fil: González Camacho, F.. No especifíca;  
dc.description.fil
Fil: Gallardo, C.. No especifíca;  
dc.description.fil
Fil: Resino Talavan, P.. No especifíca;  
dc.description.fil
Fil: Blanco, E.. No especifíca;  
dc.description.fil
Fil: Gomez Casado, E.. No especifíca;  
dc.description.fil
Fil: Alonso, C.. No especifíca;  
dc.description.fil
Fil: Escribano, J. M.. No especifíca;  
dc.journal.title
Journal of Clinical Microbiology  
dc.relation.alternativeid
info:eu-repo/semantics/altIdentifier/url/https://journals.asm.org/doi/10.1128/jcm.00406-06  
dc.relation.alternativeid
info:eu-repo/semantics/altIdentifier/doi/http://dx.doi.org/10.1128/jcm.00406-06