Partial purification of integral membrane antigenic proteins from trypanosoma evansi that display immunological cross-reactivity with trypanosoma vivax

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Abstract

Trypanosoma evansi and Trypanosoma vivax, which are the major causative agents of animal trypanosomosis in Venezuela, have shown a very high immunological cross-reactivity. Since the production of T. vivax antigens is a limiting factor as this parasite is difficult to propagate in experimental animal models, our goal has been to identify and isolate antigens from T. evansi that cross-react with T. vivax. Here, we used the Venezuelan T. evansi TEVA1 isolate to prepare the total parasite lysate and its corresponding cytosolic and membranous fractions. In order to extract the T. evansi integral membrane proteins, the particulate portion was further extracted first with Triton X-100, and then with sodium dodecyl sulfate. After discarding the cytosolic and Triton X-100 solubilized proteins, we employed sedimentation by centrifugation on linear sucrose gradients to partially purify the sodium dodecyl sulfate-solubilized proteins from the Triton X-100 resistant particulate fraction of T. evansi. We obtained enriched pools containing polypeptide bands with apparent molecular masses of 27 kDa, 31 kDa, and 53 kDa, which were recognized by anti-T. vivax antibodies from experimentally and naturally infected bovines. © 2014 Norma P. Velásquez et al.

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Velásquez, N. P., Camargo, R. E., Uzcanga, G. L., & Bubis, J. (2014). Partial purification of integral membrane antigenic proteins from trypanosoma evansi that display immunological cross-reactivity with trypanosoma vivax. Journal of Parasitology Research, 2014. https://doi.org/10.1155/2014/965815

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