An induced population of Trypanosoma cruzi epimastigotes more resistant to complement lysis promotes a phenotype with greater differentiation, invasiveness, and release of extracellular vesicles

Chagas disease is a neglected tropical disease caused by , which uses blood-feeding triatomine bugs as a vector to finally infect mammalian hosts. Upon entering the host, the parasite needs to effectively evade the attack of the complement system and quickly invade cells to guarantee an infection. In order to accomplish this, expresses different molecules on its surface and releases extracellular vesicles (EVs). Here, we have selected a population of epimastigotes (a replicative form) from through two rounds of exposure to normal human serum (NHS), to reach 30% survival (2R population). This 2R population was characterized in several aspects and compared to Wild type population. The 2R population had a favored metacyclogenesis compared with wild-type (WT) parasites. 2R metacyclic trypomastigotes had a two-fold increase in resistance to complementmediated lysis and were at least three times more infective to eukaryotic cells, probably due to a higher GP82 expression in the resistant population. Moreover, we have shown that EVs from resistant parasites can transfer the invasive phenotype to the WT population. In addition, we showed that the virulence phenotype of the selected population remains in the trypomastigote form derived from cell culture, which is more infective and also has a higher rate of release of trypomastigotes from infected cells. Altogether, these data indicate that it is possible to select parasites after exposure to a particular stress factor and that the phenotype of epimastigotes remained in the infective stage. Importantly, EVs seem to be an important virulence fator increasing mechanism in this context of survival and persistence in the host

An Essential Nuclear Protein in Trypanosomes Is a Component of mRNA Transcription/Export Pathway

In eukaryotic cells, different RNA species are exported from the nucleus via specialized pathways. The mRNA export machinery is highly integrated with mRNA processing, and includes a different set of nuclear transport adaptors as well as other mRNA binding proteins, RNA helicases, and NPC-associated proteins. The protozoan parasite Trypanosoma cruzi is the causative agent of Chagas disease, a widespread and neglected human disease which is endemic to Latin America. Gene expression in Trypanosoma has unique characteristics, such as constitutive polycistronic transcription of protein-encoding genes and mRNA processing by trans-splicing. In general, post-transcriptional events are the major points for regulation of gene expression in these parasites. However, the export pathway of mRNA from the nucleus is poorly understood. The present study investigated the function of TcSub2, which is a highly conserved protein ortholog to Sub2/ UAP56, a component of the Transcription/Export (TREX) multiprotein complex connecting transcription with mRNA export in yeast/human. Similar to its orthologs, TcSub2 is a nuclear protein, localized in dispersed foci all over the nuclei —except the fibrillar center of nucleolus— and at the interface between dense and non-dense chromatin areas, proposing the association of TcSub2 with transcription/processing sites. These findings were analyzed further by BrUTP incorporation assays and confirmed that TcSub2 is physically associated with active RNA polymerase II (RNA pol II), but not RNA polymerase I (RNA pol I) or Spliced Leader (SL) transcription, demonstrating participation particularly in nuclear mRNA metabolism in T. cruzi. The double knockout of the TcSub2 gene is lethal in T. cruzi, suggesting it has an essential function. Alternatively, RNA interference assays were performed in Trypanosoma brucei. It allowed demonstrating that besides being an essential protein, its knockdown causes mRNA accumulation in the nucleus and decrease of translation levels, reinforcing that Trypanosoma-Sub2 (Tryp-Sub2) is a component of mRNA transcription/export pathway in trypanosomes

An induced population of Trypanosoma cruzi epimastigotes more resistant to complement lysis promotes a phenotype with greater differentiation, invasiveness, and release of extracellular vesicles

IntroductionChagas disease is a neglected tropical disease caused by Trypanosoma cruzi, which uses blood-feeding triatomine bugs as a vector to finally infect mammalian hosts. Upon entering the host, the parasite needs to effectively evade the attack of the complement system and quickly invade cells to guarantee an infection. In order to accomplish this, T. cruzi expresses different molecules on its surface and releases extracellular vesicles (EVs).MethodsHere, we have selected a population of epimastigotes (a replicative form) from T. cruzi through two rounds of exposure to normal human serum (NHS), to reach 30% survival (2R population). This 2R population was characterized in several aspects and compared to Wild type population.ResultsThe 2R population had a favored metacyclogenesis compared with wild-type (WT) parasites. 2R metacyclic trypomastigotes had a two-fold increase in resistance to complementmediated lysis and were at least three times more infective to eukaryotic cells, probably due to a higher GP82 expression in the resistant population. Moreover, we have shown that EVs from resistant parasites can transfer the invasive phenotype to the WT population. In addition, we showed that the virulence phenotype of the selected population remains in the trypomastigote form derived from cell culture, which is more infective and also has a higher rate of release of trypomastigotes from infected cells.ConclusionsAltogether, these data indicate that it is possible to select parasites after exposure to a particular stress factor and that the phenotype of epimastigotes remained in the infective stage. Importantly, EVs seem to be an important virulence fator increasing mechanism in this context of survival and persistence in the host

Glucose transport in Trichoderma reesei: structural and functional characterization of the Trhxt1 and Trhxt2 genes

O fungo filamentoso Trichoderma reesei é caracteristicamente reconhecido pela produção de celulases e hemicelulases, que lhe permitem utilizar uma ampla variedade de polissacarídeos como fonte de carbono. Neste trabalho, descrevemos a caracterização de dois genes de T. reesei, Trhxt1 e Trhxt2, que codificam proteínas com alta similaridade a transportadores de glicose de vários microorganismos. Os dois genes foram identificados em um banco de dados de ESTs de T. reesei. A análise computacional de Trhxt1 e Trhxt2 indica que ambos fazem parte da major facilitator superfamily (MFS), apresentando, tipicamente, 12 segmentos transmembrânicos. A expressão de Trhxt1 ocorre apenas em baixos níveis de glicose(≈ 100 µmol 1-1), enquanto a de Trhxt2 parece ocorrer de forma constitutiva, independentemente da fonte de carbono. Em baixas concentrações de oxigênio, a expressão de Trhxt1 é induzida e a de Trhxt2, reprimida. O sistema de transporte em T. reesei apresenta um componente de afinidade muito alta por glicose (Km ≈ 20 µmol 1-1) semelhante ao de outros fungos filamentosos. Dados sobre o transporte de glicose em uma cepa mutante ΔTrhxt1 indicam que o gene Trhxt1 está envolvido com o transporte em baixos níveis de glicose (≤ 100 µmol 1-1) que correspondem, provavelmente, aos valores encontrados no solo, o habitat natural de T. reesei.. Interessantemente, a indução do sistema de celulases de T. reesei por celulose está retardada no mutante ΔTrhxt1, o que sugere a importância do transporte de glicose na expressão dos genes das celulases. Finalmente, além de descrever os primeiros genes de transportadores de glicose em T. reesei, esperamos que este trabalho possa contribuir para o preenchimento de uma lacuna em relação ao transporte de açúcares em fungos filamentosos em geral.The filamentous fungus Trichoderma reesei is a natural soil inhabitant capable of metabolizing a vast number of polysaccharide substrates. In this work, we describe two genes of T. reesei, named Trhxt1 and Trhxt2, which code for proteins with significant similarities to glucose transporters from other fungi. These genes were identified in an EST database of T. reesei. Sequence analysis of TrHXT1 and TrHXT2 revealed 12 putative transmembrane domains and several other characteristic motifs found in members of the major facilitator superfamily (MFS). Trhxt1 is transcriptionally induced only by low levels of glucose(≈ 100 µmol 1-1), while Trhxt2 expressionis independent of both glucose concentration and carbon source. We also show that Trhxt1 expression is enhanced when cells are exposured to low oxygen levels; in contrast, Trhxt2 expression seems to be repressed at these conditions. Glucose transport in T. reesei is apparently mediated by a multicomponent uptake system, in which the high-affiníty component has a Km of approximately 20 µmol 1-1. This low Km value is similar to the values reported for glucose uptake by other filamentous fungi. Kinetics of glucose transport in a T. reesei ΔTrhxt1 strain suggests that Trhxt1 is involved in glucose uptake in conditions of low glucose (≤ 100 µmol 1-1), which are most probably found in the soil, a low-nutrient environment. Interestingly, índuction ofthe T. reesei cellulase system by cellulose ís significantly delayed in the ΔTrhxt1 mutant, suggesting that glucose transport may be important to the mechanisms of expression of the cellulase genes. Finally, we hope that this work may be helpful to provide a better understanding of sugar uptake in filamentous fungi, for which there is little information available

Glucose transport in Trichoderma reesei: structural and functional characterization of the Trhxt1 and Trhxt2 genes

O fungo filamentoso Trichoderma reesei é caracteristicamente reconhecido pela produção de celulases e hemicelulases, que lhe permitem utilizar uma ampla variedade de polissacarídeos como fonte de carbono. Neste trabalho, descrevemos a caracterização de dois genes de T. reesei, Trhxt1 e Trhxt2, que codificam proteínas com alta similaridade a transportadores de glicose de vários microorganismos. Os dois genes foram identificados em um banco de dados de ESTs de T. reesei. A análise computacional de Trhxt1 e Trhxt2 indica que ambos fazem parte da major facilitator superfamily (MFS), apresentando, tipicamente, 12 segmentos transmembrânicos. A expressão de Trhxt1 ocorre apenas em baixos níveis de glicose(≈ 100 µmol 1-1), enquanto a de Trhxt2 parece ocorrer de forma constitutiva, independentemente da fonte de carbono. Em baixas concentrações de oxigênio, a expressão de Trhxt1 é induzida e a de Trhxt2, reprimida. O sistema de transporte em T. reesei apresenta um componente de afinidade muito alta por glicose (Km ≈ 20 µmol 1-1) semelhante ao de outros fungos filamentosos. Dados sobre o transporte de glicose em uma cepa mutante ΔTrhxt1 indicam que o gene Trhxt1 está envolvido com o transporte em baixos níveis de glicose (≤ 100 µmol 1-1) que correspondem, provavelmente, aos valores encontrados no solo, o habitat natural de T. reesei.. Interessantemente, a indução do sistema de celulases de T. reesei por celulose está retardada no mutante ΔTrhxt1, o que sugere a importância do transporte de glicose na expressão dos genes das celulases. Finalmente, além de descrever os primeiros genes de transportadores de glicose em T. reesei, esperamos que este trabalho possa contribuir para o preenchimento de uma lacuna em relação ao transporte de açúcares em fungos filamentosos em geral.The filamentous fungus Trichoderma reesei is a natural soil inhabitant capable of metabolizing a vast number of polysaccharide substrates. In this work, we describe two genes of T. reesei, named Trhxt1 and Trhxt2, which code for proteins with significant similarities to glucose transporters from other fungi. These genes were identified in an EST database of T. reesei. Sequence analysis of TrHXT1 and TrHXT2 revealed 12 putative transmembrane domains and several other characteristic motifs found in members of the major facilitator superfamily (MFS). Trhxt1 is transcriptionally induced only by low levels of glucose(≈ 100 µmol 1-1), while Trhxt2 expressionis independent of both glucose concentration and carbon source. We also show that Trhxt1 expression is enhanced when cells are exposured to low oxygen levels; in contrast, Trhxt2 expression seems to be repressed at these conditions. Glucose transport in T. reesei is apparently mediated by a multicomponent uptake system, in which the high-affiníty component has a Km of approximately 20 µmol 1-1. This low Km value is similar to the values reported for glucose uptake by other filamentous fungi. Kinetics of glucose transport in a T. reesei ΔTrhxt1 strain suggests that Trhxt1 is involved in glucose uptake in conditions of low glucose (≤ 100 µmol 1-1), which are most probably found in the soil, a low-nutrient environment. Interestingly, índuction ofthe T. reesei cellulase system by cellulose ís significantly delayed in the ΔTrhxt1 mutant, suggesting that glucose transport may be important to the mechanisms of expression of the cellulase genes. Finally, we hope that this work may be helpful to provide a better understanding of sugar uptake in filamentous fungi, for which there is little information available

An induced population of Trypanosoma cruzi epimastigotes more resistant to complement lysis promotes a phenotype with greater differentiation, invasiveness, and release of extracellular vesicles

© 2022 Rossi, Nunes, Sabatke, Ribas, Winnischofer, Ramos, Inal and Ramirez. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). https://creativecommons.org/licenses/by/4.0/Introduction: Chagas disease is a neglected tropical disease caused by Trypanosoma cruzi, which uses blood-feeding triatomine bugs as a vector to finally infect mammalian hosts. Upon entering the host, the parasite needs to effectively evade the attack of the complement system and quickly invade cells to guarantee an infection. In order to accomplish this, T. cruzi expresses different molecules on its surface and releases extracellular vesicles (EVs). Methods: Here, we have selected a population of epimastigotes (a replicative form) from T. cruzi through two rounds of exposure to normal human serum (NHS), to reach 30% survival (2R population). This 2R population was characterized in several aspects and compared to Wild type population. Results: The 2R population had a favored metacyclogenesis compared with wild-type (WT) parasites. 2R metacyclic trypomastigotes had a two-fold increase in resistance to complementmediated lysis and were at least three times more infective to eukaryotic cells, probably due to a higher GP82 expression in the resistant population. Moreover, we have shown that EVs from resistant parasites can transfer the invasive phenotype to the WT population. In addition, we showed that the virulence phenotype of the selected population remains in the trypomastigote form derived from cell culture, which is more infective and also has a higher rate of release of trypomastigotes from infected cells. Conclusions: Altogether, these data indicate that it is possible to select parasites after exposure to a particular stress factor and that the phenotype of epimastigotes remained in the infective stage. Importantly, EVs seem to be an important virulence fator increasing mechanism in this context of survival and persistence in the host.Peer reviewe

Identification of a Golgi-localized UDP-Nacetylglucosamine transporter in Trypanosoma cruzi

Submitted by Luciane Willcox ([email protected]) on 2016-08-29T16:24:10Z No. of bitstreams: 1 Identification of a Golgi-localized UDP-N-acetylglucosamine.pdf: 1462528 bytes, checksum: 4ee82b612b65e97fc2bf07e38093715e (MD5)Approved for entry into archive by Luciane Willcox ([email protected]) on 2016-08-29T17:26:01Z (GMT) No. of bitstreams: 1 Identification of a Golgi-localized UDP-N-acetylglucosamine.pdf: 1462528 bytes, checksum: 4ee82b612b65e97fc2bf07e38093715e (MD5)Made available in DSpace on 2016-08-29T17:26:01Z (GMT). No. of bitstreams: 1 Identification of a Golgi-localized UDP-N-acetylglucosamine.pdf: 1462528 bytes, checksum: 4ee82b612b65e97fc2bf07e38093715e (MD5) Previous issue date: 2015-11-21Fundação Oswaldo Cruz. Conselho Nacional de Desenvolvimento e Tecnológico. Fundação AraucáriaUniversidade de São Paulo. Instituto de Ciências Biomédicas. Departamento de Parasitologia. São Paulo, SP, Brasil.Universidade de São Paulo. Instituto de Ciências Biomédicas. Departamento de Imunologia. São Paulo, SP, BrasilFundação Oswaldo Cruz. Instituto Carlos Chagas. Laboratório de Regulação da Expressão Gênica. Curitiba, PR, Brasil.Fundação Oswaldo Cruz. Instituto Carlos Chagas. Laboratório de Regulação da Expressão Gênica. Curitiba, PR, Brasil.Fundação Oswaldo Cruz. Instituto Carlos Chagas. Laboratório de Regulação da Expressão Gênica. Curitiba, PR, Brasil.Fundação Oswaldo Cruz. Instituto Carlos Chagas. Laboratório de Regulação da Expressão Gênica. Curitiba, PR, Brasil.Fundação Oswaldo Cruz. Instituto Carlos Chagas. Laboratório de Regulação da Expressão Gênica. Curitiba, PR, Brasil.Fundação Oswaldo Cruz. Instituto Carlos Chagas. Laboratório de Regulação da Expressão Gênica. Curitiba, PR, Brasil.Fundação Oswaldo Cruz. Instituto Carlos Chagas. Laboratório de Regulação da Expressão Gênica. Curitiba, PR, Brasil.Background Nucleotide sugar transporters (NSTs) play an essential role in translocating nucleotide sugars into the lumen of the endoplasmic reticulum and Golgi apparatus to be used as substrates in glycosylation reactions. This intracellular transport is an essential step in the biosynthesis of glycoconjugates. Results We have identified a family of 11 putative NSTs in Trypanosoma cruzi, the etiological agent of Chagas’ disease. A UDP-N-acetylglucosamine transporter, TcNST1, was identified by a yeast complementation approach. Based on a phylogenetic analysis four candidate genes were selected and used for complementation assays in a Kluyveromyces lactis mutant strain. The transporter is likely expressed in all stages of the parasite life cycle and during differentiation of epimastigotes to infective metacyclics. Immunofluorescence analyses of a GFP-TcNST1 fusion protein indicate that the transporter is localized to the Golgi apparatus. As many NSTs are multisubstrate transporters, we also tested the capacity of TcNST1 to transport GDP-Man. Conclusions We have identified a UDP-N-acetylglucosamine transporter in T. cruzi, which is specifically localized to the Golgi apparatus and seems to be expressed, at the mRNA level, throughout the parasite life cycle. Functional studies of TcNST1 will be important to unravel the role of NSTs and specific glycoconjugates in T. cruzi survival and infectivity

Image_2_An induced population of Trypanosoma cruzi epimastigotes more resistant to complement lysis promotes a phenotype with greater differentiation, invasiveness, and release of extracellular vesicles.tif

IntroductionChagas disease is a neglected tropical disease caused by Trypanosoma cruzi, which uses blood-feeding triatomine bugs as a vector to finally infect mammalian hosts. Upon entering the host, the parasite needs to effectively evade the attack of the complement system and quickly invade cells to guarantee an infection. In order to accomplish this, T. cruzi expresses different molecules on its surface and releases extracellular vesicles (EVs).MethodsHere, we have selected a population of epimastigotes (a replicative form) from T. cruzi through two rounds of exposure to normal human serum (NHS), to reach 30% survival (2R population). This 2R population was characterized in several aspects and compared to Wild type population.ResultsThe 2R population had a favored metacyclogenesis compared with wild-type (WT) parasites. 2R metacyclic trypomastigotes had a two-fold increase in resistance to complementmediated lysis and were at least three times more infective to eukaryotic cells, probably due to a higher GP82 expression in the resistant population. Moreover, we have shown that EVs from resistant parasites can transfer the invasive phenotype to the WT population. In addition, we showed that the virulence phenotype of the selected population remains in the trypomastigote form derived from cell culture, which is more infective and also has a higher rate of release of trypomastigotes from infected cells.ConclusionsAltogether, these data indicate that it is possible to select parasites after exposure to a particular stress factor and that the phenotype of epimastigotes remained in the infective stage. Importantly, EVs seem to be an important virulence fator increasing mechanism in this context of survival and persistence in the host.</p

Image_1_An induced population of Trypanosoma cruzi epimastigotes more resistant to complement lysis promotes a phenotype with greater differentiation, invasiveness, and release of extracellular vesicles.tif

IntroductionChagas disease is a neglected tropical disease caused by Trypanosoma cruzi, which uses blood-feeding triatomine bugs as a vector to finally infect mammalian hosts. Upon entering the host, the parasite needs to effectively evade the attack of the complement system and quickly invade cells to guarantee an infection. In order to accomplish this, T. cruzi expresses different molecules on its surface and releases extracellular vesicles (EVs).MethodsHere, we have selected a population of epimastigotes (a replicative form) from T. cruzi through two rounds of exposure to normal human serum (NHS), to reach 30% survival (2R population). This 2R population was characterized in several aspects and compared to Wild type population.ResultsThe 2R population had a favored metacyclogenesis compared with wild-type (WT) parasites. 2R metacyclic trypomastigotes had a two-fold increase in resistance to complementmediated lysis and were at least three times more infective to eukaryotic cells, probably due to a higher GP82 expression in the resistant population. Moreover, we have shown that EVs from resistant parasites can transfer the invasive phenotype to the WT population. In addition, we showed that the virulence phenotype of the selected population remains in the trypomastigote form derived from cell culture, which is more infective and also has a higher rate of release of trypomastigotes from infected cells.ConclusionsAltogether, these data indicate that it is possible to select parasites after exposure to a particular stress factor and that the phenotype of epimastigotes remained in the infective stage. Importantly, EVs seem to be an important virulence fator increasing mechanism in this context of survival and persistence in the host.</p