Trypanosoma cruzi: effects of heat shock on ecto-ATPase activity

Giarola, Naira Lígia Lima; Amaral, Elmo Eduardo de Almeida; Collopy Júnior, Itallo; Souza, André Luiz Fonseca de; Majerowicz, David; Paes, Lisvane Silva; Gondim, Katia C.; Fernandes, José Roberto Meyer

Article

Registro en:

GIAROLA, Naíra Lígia Lima; et al. Trypanosoma cruzi: Effects of heat shock on ecto-ATPase activity. Experimental Parasitology, v.133, n.4, p.434-441, Apr. 2013.

0014-4894

https://www.arca.fiocruz.br/handle/icict/15386

10.1016/j.exppara.2012.12.014

https://repositorioslatinoamericanos.uchile.cl/handle/2250/8863856

Autor

Giarola, Naira Lígia Lima

Amaral, Elmo Eduardo de Almeida

Collopy Júnior, Itallo

Souza, André Luiz Fonseca de

Majerowicz, David

Paes, Lisvane Silva

Gondim, Katia C.

Fernandes, José Roberto Meyer

Institución

Instituto de Comunicação e Informação Científica e Tecnológica em Saúde (Brasil)

Resumen

In this work, we demonstrate that Trypanosoma cruzi Y strain epimastigotes exhibit Mg2+-dependent ecto-ATPase activity that is stimulated by heat shock. When the epimastigotes were incubated at 37°C for 2h, the ecto-ATPase activity of the cells was 43.95±0.97 nmol Pi/h×10(7) cells, whereas the ecto-ATPase activity of cells that were not exposed to heat shock stress was 16.97±0.30 nmol Pi/h×10(7) cells. The ecto-ATPase activities of cells, that were exposed or not exposed to heat shock stress had approximately the same Km values (2.25±0.26 mM ATP and 1.55±0.23 mM ATP, respectively) and different Vmax values. The heat-shocked cells had higher Vmax values (54.38±3.07 nmol Pi/h×10(7) cells) than the cells that were not exposed to heat shock (19.38±1.76 nmol Pi/h×10(7) cells). We also observed that the ecto-phosphatase and ecto-5'nucleotidase activities of cells that had been incubated at 28°C or 37°C were the same. Interestingly, cycloheximide, an inhibitor of protein synthesis, suppressed the heat shock effect of ecto-ATPase activity on T. cruzi. The Mg2+-dependent ecto-ATPase activity from the Y strain (high virulence) was approximately 2-fold higher than that of Dm28c (a clone with low virulence). In addition, these two strains presented different responses to heat shock with regard to their ecto-ATPase activities; Y strain epimastigotes had a stimulation of 2.52-fold while the Dm28c strain had a 1.71-fold stimulation. In this context, the virulent trypomastigote form of T. cruzi, Dm28c, had an ecto-ATPase activity that was more than 7-fold higher (66.67±5.98 nmol Pi/h×10(7) cells) than that of the insect epimastigote forms (8.91±0.76 nmol Pi/h×10(7) cells). This difference increased to approximately 10-fold when both forms were subjected to heat shock stress (181.14±16.48 nmol Pi/h×10(7) cells for trypomastigotes and 16.71±1.17 nmol Pi/h×10(7) cells for epimastigotes at 37°C). The ecto-ATPase activity of a plasma membrane-enriched fraction obtained from T. cruzi epimastigotes was not increased by heat treatment, which suggested that cytoplasmic components had an influence on enzyme activation by heat shock stress.

2030-01-01

Materias

Mostrar el registro completo del ítem