Your search keyword '"Cimino, Rubén"' showing total 5 results

1. Mapping the global distribution of Strongyloides stercoralis and hookworms by ecological niche modeling

Author

Fleitas, Pedro Emanuel, Kehl, Sebastián Dario, Lopez, Walter, Travacio, Marina, Nieves, Elvia, Gil, José Fernando, Cimino, Rubén Oscar, and Krolewiecki, Alejandro Javier

Published

2022

2. Impact of intestinal parasites on microbiota and cobalamin gene sequences: a pilot study

Author

Mejia, Rojelio, Damania, Ashish, Jeun, Rebecca, Bryan, Patricia E., Vargas, Paola, Juarez, Marisa, Cajal, Pamela S., Nasser, Julio, Krolewiecki, Alejandro, Lefoulon, Emilie, Long, Courtney, Drake, Evan, Cimino, Rubén O., and Slatko, Barton

Published

2020

3. Effects of IFN-γ coding plasmid supplementation in the immune response and protection elicited by Trypanosoma cruzi attenuated parasites.

Author

Brandán, Cecilia Pérez, Mesías, Andrea C., Parodi, Cecilia, Cimino, Rubén O., Brandán, Carolina Pérez, Diosque, Patricio, Basombrío, Miguel Ángel, Pérez Brandán, Cecilia, and Pérez Brandán, Carolina

Subjects

TRYPANOSOMA cruzi, IMMUNE response, PARASITES, IMMUNOGLOBULINS, MICROBIAL virulence, ANIMAL experimentation, CYTOKINES, ENZYME-linked immunosorbent assay, GENES, HEART, INTERFERONS, MICE, PROTOZOA, RESEARCH funding, TRYPANOSOMIASIS, VACCINES, PHENOMENOLOGICAL biology

Abstract

Background: Previous studies showed that a naturally attenuated strain from Trypanosoma cruzi triggers an immune response mainly related to a Th2-type profile. Albeit this, a strong protection against virulent challenge was obtained after priming mice with this attenuated strain. However, this protection is not enough to completely clear parasites from the host. In T. cruzi infection, early Interferon-gamma (IFN-γ) is critical to lead type 1 responses able to control intracellular parasites. Therefore we evaluated whether the co-administration of a plasmid encoding murine IFN-γ could modify the immune response induced by infection with attenuated parasites and improve protection against further infections.Methods: C57BL/6J mice were infected intraperitoneally with three doses of live attenuated parasites in combination with plasmid pVXVR-mIFN-γ. Before each infection dose, sera samples were collected for parasite specific antibodies determination and cytokine quantification. To evaluate the recall response to T. cruzi, mice were challenged with virulent parasites 30 days after the last dose and parasite load in peripheral blood and heart was evaluated.Results: As determined by ELISA, significantly increase in T. cruzi specific antibodies response was detected in the group in which pVXVR-mIFN-γ was incorporated, with a higher predominance of IgG2a subtype in comparison to the group of mice only inoculated with attenuated parasites. At our limit of detection, serum levels of IFN-γ were not detected, however a slight decrease in IL-10 concentrations was observed in groups in which pVXVR-mIFN-γ was supplemented. To analyze if the administration of pVXVR-mIFN-γ has any beneficial effect in protection against subsequent infections, all experimental groups were submitted to a lethal challenge with virulent bloodstream trypomastigotes. Similar levels of challenge parasites were detected in peripheral blood and heart of mice primed with attenuated parasites alone or combined with plasmid DNA. Expansion of IgG antibodies was not significant in TCC+ pVXVR-mIFN-γ; however, the overall tendency to sustain a Th2 profile was maintained.Conclusions: Overall, these results suggest that administration of plasmid pVXVR-mIFN-γ could have beneficial effects on host specific antibody production in response to T. cruzi attenuated infection; however, this outcome is not reflected in an improved protection against further virulent infections. [ABSTRACT FROM AUTHOR]

Published

2017

4. Identification of human intestinal parasites affecting an asymptomatic peri-urban Argentinian population using multi-parallel quantitative real-time polymerase chain reaction.

Author

Cimino, Rubén O., Jeun, Rebecca, Juarez, Marisa, Cajal, Pamela S., Vargas, Paola, Echazú, Adriana, Bryan, Patricia E., Nasser, Julio, Krolewiecki, Alejandro, and Mejia, Rojelio

Subjects

*INTESTINAL parasites, *DIAGNOSTIC use of polymerase chain reaction, *PUBLIC health, *DISEASE prevalence, *FECAL analysis, *MICROSCOPY, *HELMINTHS, *PROTOZOA, *DIAGNOSIS

Abstract

Background: In resource-limited countries, stool microscopy is the diagnostic test of choice for intestinal parasites (soil-transmitted helminths and/or intestinal protozoa). However, sensitivity and specificity is low. Improved diagnosis of intestinal parasites is especially important for accurate measurements of prevalence and intensity of infections in endemic areas. Methods: The study was carried out in Orán, Argentina. A total of 99 stool samples from a local surveillance campaign were analyzed by concentration microscopy and McMaster egg counting technique compared to the analysis by multi-parallel quantitative real-time polymerase chain reaction (qPCR). This study compared the performance of qPCR assay and stool microscopy for 8 common intestinal parasites that infect humans including the helminths Ascaris lumbricoides, Ancylostoma duodenale, Necator americanus, Strongyloides stercoralis, Trichuris trichiura, and the protozoa Giardia lamblia, Cryptosporidium parvum/hominis, and Entamoeba histolytica, and investigated the prevalence of polyparasitism in an endemic area. Results: qPCR showed higher detection rates for all parasites as compared to stool microscopy except T. trichiura. Species-specific primers and probes were able to distinguish between A. duodenale (19.1 %) and N. americanus (36.4 %) infections. There were 48.6 % of subjects co-infected with both hookworms, and a significant increase in hookworm DNA for A. duodenale versus N. americanus (119.6 fg/μL: 0.63 fg/μL, P < 0.001) respectively. qPCR outperformed microscopy by the largest margin in G. lamblia infections (63.6 % versus 8.1 %, P < 0.05). Polyparasitism was detected more often by qPCR compared to microscopy (64.7 % versus 24.2 %, P < 0.05). Conclusions: Multi-parallel qPCR is a quantitative molecular diagnostic method for common intestinal parasites in an endemic area that has improved diagnostic accuracy compared to stool microscopy. This first time use of multi-parallel qPCR in Argentina has demonstrated the high prevalence of intestinal parasites in a peri-urban area. These results will contribute to more accurate epidemiological survey, refined treatment strategies on a public scale, and better health outcomes in endemic settings. [ABSTRACT FROM AUTHOR]

Published

2015

5. Effects of IFN-γ coding plasmid supplementation in the immune response and protection elicited by Trypanosoma cruzi attenuated parasites.

Author

Pérez Brandán C, Mesías AC, Parodi C, Cimino RO, Pérez Brandán C, Diosque P, and Basombrío MÁ

Subjects

Animals, Antibodies, Protozoan blood, Chagas Disease mortality, Cytokines blood, Enzyme-Linked Immunosorbent Assay, Heart parasitology, Host-Parasite Interactions immunology, Immunoglobulin G blood, Interferon-gamma blood, Male, Mice, Mice, Inbred C57BL, Trypanosoma cruzi pathogenicity, Vaccines, Attenuated immunology, Chagas Disease immunology, Interferon-gamma genetics, Plasmids pharmacology, Trypanosoma cruzi immunology

Abstract

Background: Previous studies showed that a naturally attenuated strain from Trypanosoma cruzi triggers an immune response mainly related to a Th2-type profile. Albeit this, a strong protection against virulent challenge was obtained after priming mice with this attenuated strain. However, this protection is not enough to completely clear parasites from the host. In T. cruzi infection, early Interferon-gamma (IFN-γ) is critical to lead type 1 responses able to control intracellular parasites. Therefore we evaluated whether the co-administration of a plasmid encoding murine IFN-γ could modify the immune response induced by infection with attenuated parasites and improve protection against further infections., Methods: C57BL/6J mice were infected intraperitoneally with three doses of live attenuated parasites in combination with plasmid pVXVR-mIFN-γ. Before each infection dose, sera samples were collected for parasite specific antibodies determination and cytokine quantification. To evaluate the recall response to T. cruzi, mice were challenged with virulent parasites 30 days after the last dose and parasite load in peripheral blood and heart was evaluated., Results: As determined by ELISA, significantly increase in T. cruzi specific antibodies response was detected in the group in which pVXVR-mIFN-γ was incorporated, with a higher predominance of IgG2a subtype in comparison to the group of mice only inoculated with attenuated parasites. At our limit of detection, serum levels of IFN-γ were not detected, however a slight decrease in IL-10 concentrations was observed in groups in which pVXVR-mIFN-γ was supplemented. To analyze if the administration of pVXVR-mIFN-γ has any beneficial effect in protection against subsequent infections, all experimental groups were submitted to a lethal challenge with virulent bloodstream trypomastigotes. Similar levels of challenge parasites were detected in peripheral blood and heart of mice primed with attenuated parasites alone or combined with plasmid DNA. Expansion of IgG antibodies was not significant in TCC+ pVXVR-mIFN-γ; however, the overall tendency to sustain a Th2 profile was maintained., Conclusions: Overall, these results suggest that administration of plasmid pVXVR-mIFN-γ could have beneficial effects on host specific antibody production in response to T. cruzi attenuated infection; however, this outcome is not reflected in an improved protection against further virulent infections.

Published

2017