Oxidative stress fuels Trypanosoma cruzi infection in mice
Claudia N. Paiva, … , Joseli Lannes-Vieira, Marcelo T. Bozza
Claudia N. Paiva, … , Joseli Lannes-Vieira, Marcelo T. Bozza
Published June 25, 2012
Citation Information: J Clin Invest. 2012;122(7):2531-2542. https://doi.org/10.1172/JCI58525.
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Research Article

Oxidative stress fuels Trypanosoma cruzi infection in mice

Abstract

Oxidative damage contributes to microbe elimination during macrophage respiratory burst. Nuclear factor, erythroid-derived 2, like 2 (NRF2) orchestrates antioxidant defenses, including the expression of heme-oxygenase–1 (HO-1). Unexpectedly, the activation of NRF2 and HO-1 reduces infection by a number of pathogens, although the mechanism responsible for this effect is largely unknown. We studied Trypanosoma cruzi infection in mice in which NRF2/HO-1 was induced with cobalt protoporphyrin (CoPP). CoPP reduced parasitemia and tissue parasitism, while an inhibitor of HO-1 activity increased T. cruzi parasitemia in blood. CoPP-induced effects did not depend on the adaptive immunity, nor were parasites directly targeted. We also found that CoPP reduced macrophage parasitism, which depended on NRF2 expression but not on classical mechanisms such as apoptosis of infected cells, induction of type I IFN, or NO. We found that exogenous expression of NRF2 or HO-1 also reduced macrophage parasitism. Several antioxidants, including NRF2 activators, reduced macrophage parasite burden, while pro-oxidants promoted it. Reducing the intracellular labile iron pool decreased parasitism, and antioxidants increased the expression of ferritin and ferroportin in infected macrophages. Ferrous sulfate reversed the CoPP-induced decrease in macrophage parasite burden and, given in vivo, reversed their protective effects. Our results indicate that oxidative stress contributes to parasite persistence in host tissues and open a new avenue for the development of anti–T. cruzi drugs.

Authors

Claudia N. Paiva, Daniel F. Feijó, Fabianno F. Dutra, Vitor C. Carneiro, Guilherme B. Freitas, Letícia S. Alves, Jacilene Mesquita, Guilherme B. Fortes, Rodrigo T. Figueiredo, Heitor S.P. Souza, Marcelo R. Fantappié, Joseli Lannes-Vieira, Marcelo T. Bozza

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Figure 6

Effects of gp91phox on T. cruzi infection.

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Effects of gp91phox on T. cruzi infection. (A) Effects of CoPP on the ...
(A) Effects of CoPP on the parasite burden of in vitro infected macrophages derived from wild-type or gp91phox–/– mice (Giemsa). (B) Flow cytometry quantification of ROS (CM-H2DCFDA probe) in BMMs from wild-type or gp91phox–/– mice after infection. Non-labeled controls are shown in gray. (C) Mean parasitemia of wild-type and gp91phox–/– mice (n = 7). (D) Parasite burden in peritoneal macrophages taken from wild-type and gp91phox–/– mice at 8 dpi. Cells were cultured for an additional 48 hours before they were fixed and stained. The graphs show the mean ± SEM of the parasite burden in each individual mouse (n = 4 mice/group). (E) Mean parasitemia (n = 5) and (F) survival of wild-type and gp91phox–/– mice left untreated (n = 12) or treated with CoPP (n = 5). Error bars represent SEM. *P < 0.05 compared with infected untreated controls.