Eimeria bovis meront I-carrying host cells express parasite-specific antigens on their surface membrane
| Autor: | Anja Taubert, Horst Zahner, Carlos Hermosilla, Ahmed Ibrahem I. Badawy, Kathleen Lutz |
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| Rok vydání: | 2009 |
| Předmět: |
Male
Antibodies Protozoan Cattle Diseases Antigens Protozoan Biology Host-Parasite Interactions Immune system Antigen Immunity Chlorocebus aethiops Animals Parasite hosting Fluorescent Antibody Technique Indirect Microscopy Immunoelectron Vero Cells Host cell surface Microscopy Confocal General Veterinary Coccidiosis Endothelial Cells General Medicine Molecular biology Rats Rats Inbred Lew Antigens Surface biology.protein Vero cell Cattle Eimeria Apical complex Antibody |
| Zdroj: | Veterinary Research Communications. 34:103-118 |
| ISSN: | 1573-7446 0165-7380 |
| DOI: | 10.1007/s11259-009-9336-y |
| Popis: | Host immune responses conducted against antigens of Eimeria bovis are key factors for the development of protective immunity against this protozoan disease. In this study we investigated the expression of E. bovis-derived antigens on the host cell surface membrane during E. bovis first merogony in vitro. Host cells carrying E. bovis-meront I stages expressed E. bovis host cell surface antigens (EbHCSAg) on their surface membrane which were recognised by hyperimmune sera of calves and by sera from rats immunized with E. bovis merozoites I, when tested by indirect immune fluorescent antibody test (IIFAT), laser scanning confocal microscopy (LSCM) and immune electron microscopy. Expression of EbHCSAg on permissive host cells was earliest detected 7 days p. i., thus coinciding with the onset of the parasite replication. Membrane-associated EbHCSAg were removed from infected host cells by proteinase K, partially by Triton X-100, Triton X-114 and Triton X-405, but not by 1 M NaCl, CHAPS or phospholipase C treatment. Antibodies, affinity-purified on paraformaldehyde/glutardialdehyde (PAGA)-fixed E. bovis meront I-infected bovine host cells bound to the surface meront I-carrying cells and to merozoites I (IIFAT, LSCM) but, in contrast to untreated sera, not to sporozoites. When tested on methanol-fixed merozoites I and sporozoites by IIFAT, affinity-purified antibodies bound to structures in the apical complex area of merozoites I, but not to sporozoites, whilst untreated sera caused diffuse labelling of internal structures of both parasite stages. Immune electron microscopy demonstrated binding of affinity-purified antibodies to micronemes and dense granules of merozoites I. Although the function of EbHCSAg is still unknown, results of this study might suggest an involvement in the development of protective immunity against E. bovis infections. |
| Databáze: | OpenAIRE |
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