Distribution of Epitopes of Trypanosoma cruzi Amastigotes During the Intracellular Life Cycle within Mammalian Cells

In this study we have examined the distribution of epitopes defined by monoclonal antibodies raised against Trypanosoma cruzi amastigotes during the intraceullar life cycle of the parasite. We have raised monoclonal antibodies towards amastigote forms and performed preliminary immunochemical charact...

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Bibliographic Details
Published in:The Journal of eukaryotic microbiology 1997-07, Vol.44 (4), p.332-344
Main Authors: BARROS, HELENA C., VERBISCK, NEWTON V., SILVA, SOLANGE DA, ARAGUTH, MARCIA F., MORTARA, RENATO A.
Format: Article
Language:English
Subjects:
Amastigote antigens
Animals
Antibodies, Monoclonal - immunology
Antibodies, Protozoan - immunology
Antigens, Protozoan - analysis
Biological and medical sciences
Carbohydrates - immunology
Cercopithecus aethiops
confocal microscopy
Epitopes - analysis
Fundamental and applied biological sciences. Psychology
immuno-electron microscopy
Life cycle. Host-agent relationship. Pathogenesis
Mice
Mice, Inbred BALB C
monoclonal antibodies
Protozoa
Trypanosoma cruzi
Trypanosoma cruzi - growth & development
Trypanosoma cruzi - immunology
Trypanosoma cruzi - ultrastructure
Vero Cells
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Summary:In this study we have examined the distribution of epitopes defined by monoclonal antibodies raised against Trypanosoma cruzi amastigotes during the intraceullar life cycle of the parasite. We have raised monoclonal antibodies towards amastigote forms and performed preliminary immunochemical characterization of their reactivities. MAB 1D9, 3G8, 2B7, 3B9, and 4B9, and 4B9 react with carbohydrate epitopes of the parasite major surface glycoprotein—Ssp‐4 defined by MAB 2C2 [5]: MAB 4B5 reacts with a noncarbohydrate epitope in all developmental stages of the parasite, and MAB 3B2 also detects a noncarbohydrate epitope preferentially in T. cruzi flagellared forms. Vero cells infected with tissue culture‐derived trypomastigotes of clone D11 (G strain) were fixed at different times during the intraceullular proliferation of parasites, and processed for immjno‐electron microscopy and confocal immunoflurescence with the different monoclonal antibodies. We observed that while the surface distribution of MAB 2C2 and 4B9 epitopes was uniform throughout the cycle, MAB 1D9, 3G8, and 2B7 reacted with cytoplasmic membrance‐bound compartments of the amastigotes. MAB 3B9 displayed a unique surface dentate pattern in some amastigotes. MAB 4B5 recognized a curved‐shaped structure at the flagellar pocket region in some intracellular amastigotes and localized to the membrane in dividing forms. In intracellular trypomastigotes, MAB 4B5 also displayed a punctate pattern near the flagellar pocket.
ISSN:1066-5234
1550-7408
DOI:10.1111/j.1550-7408.1997.tb05675.x