Higher expression of proline dehydrogenase altered mitochondrial function and increased Trypanosoma cruzi differentiation in vitro and in the insect vector

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dc.contributor(LCC) Lab. Ciclo Celularpt_BR
dc.contributor(CeTICS) Centro de Toxinas, Resposta-imune e Sinalização Celularpt_BR
dc.contributor.authorMantilla, Brian S.pt_BR
dc.contributor.authorPaes-Vieira, Lisvanept_BR
dc.contributor.authorDias, Felipe de Almeidapt_BR
dc.contributor.authorCalderano, Simone Guedespt_BR
dc.contributor.authorElias, Maria Carolinapt_BR
dc.contributor.authorCosentino-Gomes, Danielapt_BR
dc.contributor.authorOliveira, Pedro L.pt_BR
dc.contributor.authorMeyer-Fernandes, José Robertopt_BR
dc.contributor.authorSilber, Ariel M.pt_BR
dc.date.accessioned2021-12-07T12:52:43Z-
dc.date.available2021-12-07T12:52:43Z-
dc.date.issued2021pt_BR
dc.identifier.citationMantilla BS., Paes-Vieira L, Dias FA, Calderano SG, Elias MC, Cosentino-Gomes D, et al. Higher expression of proline dehydrogenase altered mitochondrial function and increased Trypanosoma cruzi differentiation in vitro and in the insect vector. Biochem. J.. 2021 Nov;478(21):3891–3903. doi:10.1042/BCJ20210428.pt_BR
dc.identifier.urihttps://repositorio.butantan.gov.br/handle/butantan/4008-
dc.description.abstractThe pathogenic protist Trypanosoma cruzi uses kissing bugs as invertebrate hosts that vectorize the infection among mammals. This parasite oxidizes proline to glutamate through two enzymatic steps and one nonenzymatic step. In insect vectors, T. cruzi differentiates from a noninfective replicating form to nonproliferative infective forms. Proline sustains this differentiation, but to date, a link between proline metabolism and differentiation has not been established. In T. cruzi, the enzymatic steps of the proline-glutamate oxidation pathway are catalyzed exclusively by the mitochondrial enzymes proline dehydrogenase [TcPRODH, EC: 1.5.5.2] and Δ1-pyrroline-5-carboxylate dehydrogenase [TcP5CDH, EC: 1.2.1.88]. Both enzymatic steps produce reducing equivalents that are able to directly feed the mitochondrial electron transport chain (ETC) and thus produce ATP. In this study, we demonstrate the contribution of each enzyme of the proline-glutamate pathway to ATP production. In addition, we show that parasites overexpressing these enzymes produce increased levels of H2O2, but only those overexpressing TcP5CDH produce increased levels of superoxide anion. We show that parasites overexpressing TcPRODH, but not parasites overexpressing TcP5CDH, exhibit a higher rate of differentiation into metacyclic trypomastigotes in vitro. Finally, insect hosts infected with parasites overexpressing TcPRODH showed a diminished parasitic load but a higher percent of metacyclic trypomastigotes, when compared with controls. Our data show that parasites overexpressing both, PRODH and P5CDH had increased mitochondrial functions that orchestrated different oxygen signaling, resulting in different outcomes in relation to the efficiency of parasitic differentiation in the invertebrate host.pt_BR
dc.description.sponsorship(FAPESP) Fundação de Amparo à Pesquisa do Estado de São Paulopt_BR
dc.description.sponsorship(CNPq) Conselho Nacional de Desenvolvimento Científico e Tecnológicopt_BR
dc.description.sponsorshipResearch Councils UKpt_BR
dc.format.extent3891–3903pt_BR
dc.language.isoEnglishpt_BR
dc.relation.ispartofBiochemical Journalpt_BR
dc.rightsRestricted accesspt_BR
dc.titleHigher expression of proline dehydrogenase altered mitochondrial function and increased Trypanosoma cruzi differentiation in vitro and in the insect vectorpt_BR
dc.typeArticlept_BR
dc.identifier.doi10.1042/BCJ20210428pt_BR
dc.identifier.urlhttps://doi.org/10.1042/BCJ20210428pt_BR
dc.contributor.external(USP) Universidade de São Paulopt_BR
dc.contributor.external(UFRJ) Universidade Federal do Rio de Janeiropt_BR
dc.identifier.citationvolume478pt_BR
dc.identifier.citationissue21pt_BR
dc.subject.keywordcell differentiationpt_BR
dc.subject.keywordparasite–vector interactionpt_BR
dc.subject.keywordproline metabolismpt_BR
dc.subject.keywordTrypanosoma cruzipt_BR
dc.relation.ispartofabbreviatedBiochem Jpt_BR
dc.identifier.citationabntv. 478, n. 21, p. 3891–3903, nov. 2021pt_BR
dc.identifier.citationvancouver2021 Nov;478(21):3891–3903pt_BR
dc.contributor.butantanCalderano, Simone Guedes|:Pesquisador|:LCC - Laboratório de Ciclo Celularpt_BR
dc.contributor.butantanElias, Maria Carolina|:Pesquisador|:LCC - Laboratório de Ciclo Celularpt_BR
dc.sponsorship.butantan(FAPESP) Fundação de Amparo à Pesquisa do Estado de São Paulo¦¦2016/06034-2pt_BR
dc.sponsorship.butantan(FAPESP) Fundação de Amparo à Pesquisa do Estado de São Paulo¦¦2018/14432-3pt_BR
dc.sponsorship.butantan(CNPq) Conselho Nacional de Desenvolvimento Científico e Tecnológico¦¦308351/2013-4pt_BR
dc.sponsorship.butantan(CNPq) Conselho Nacional de Desenvolvimento Científico e Tecnológico¦¦404769/2018-7pt_BR
dc.sponsorship.butantanResearch Councils UK¦¦MR/P027989/1pt_BR
dc.identifier.bvsccBR78.1pt_BR
dc.identifier.bvsdbIBProdpt_BR
dc.description.dbindexedYespt_BR
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item.languageiso639-1English-
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