ABSTRACT
BACKGROUND Different strategies for improvement of malaria control and elimination are based on the blockage of malaria parasite transmission to the mosquito vector. These strategies include the drugs that target the plasmodial sexual stages in humans and the early developmental stages inside mosquitoes. OBJECTIVES Here we tested Malaria Box compounds in order to evaluate their activity against male and female gametocytes in Plasmodium berghei, mosquito infection in P. vivax and ookinete formation in both species. METHODS/FINDINGS The membrane feeding assay and the development of ookinetes by a 24 h ex vivo culture and the ookinete yield per 1000 erythrocytes were used to test transmission-blocking potential of the Malaria Box compounds in P. vivax. For P. berghei we used flow cytometry to evaluate male and female gametocyte time course and fluorescence microscopy to check the ookinete development. The two species used in this study showed similar results concerning the compounds' activity against gametocytes and ookinetes, which were different from those in P. falciparum. In addition, from the eight Malaria Box compounds tested in both species, compounds MMV665830, MMV665878 and MMV665941 were selected as a hit compounds due the high inhibition observed. CONCLUSION Our results showed that P. berghei is suitable as an initial screening system to test compounds against P. vivax.
Subject(s)
Animals , Plasmodium berghei/drug effects , Plasmodium vivax/drug effects , Malaria, Vivax/prevention & control , Mosquito Vectors/parasitology , Malaria, Vivax/drug therapy , Malaria, Vivax/transmissionABSTRACT
Abstract INTRODUCTION: The Culicoides transmit a variety of pathogens. Our aim was to survey the Culicoides species occurring in an Amazonian rural settlement, comparing abundance, richness, and diversity in different environments. METHODS: Culicoides were captured using CDC light traps. The Shannon-Wiener (H') and Rényi indices were used to compare species diversity and evenness between environments, the equitability (J') index was used to calculate the uniformity of distribution among species, and similarity was estimated using the Jaccard similarity index. A permutational multivariate analysis of variance was applied to assess the influence of environment on species composition. A non-metric dimensional scale was used to represent the diversity profiles of each environment in a multidimensional space. RESULTS: 6.078 Culicoides were captured, representing 84 species (45 valid species/39 morphotypes). H' values showed the following gradient: forest > capoeira > peridomicile > forest edge. The equitability J' was greater in capoeira and forests compared to peridomiciles and the forest edge. The population compositions of each environment differed statistically, but rarefaction estimates indicate that environments of the same type possessed similar levels of richness. Species of medical and veterinary importance were found primarily in peridomiciles: C. paraensis, vector of Oropouche virus; C. insignis and C. pusillus, vectors of Bluetongue virus; C. filariferus, C. flavivenula, C. foxi, and C. ignacioi, found carrying Leishmania DNA. CONCLUSIONS: This study indicates that diversity was higher in natural environments than in anthropized environments, while abundance and richness were highest in the most anthropized environment. These findings suggest that strictly wild Culicoides can adapt to anthropized environments.
Subject(s)
Animals , Male , Female , Ceratopogonidae/classification , Biodiversity , Insect Vectors/classification , Rural Population , Seasons , Brazil , Population DensityABSTRACT
Abstract INTRODUCTION: Malaria and leishmaniases are transmitted by vectors during blood-feeding. Vector-infected animals develop antibodies against the vector's saliva. This study evaluated IgY antibody detection in the chicken eggs exposed to bites from Migonemyia migonei, Lutzomyia longipalpis and Anopheles aquasalis. METHODS: We used ELISA to quantify the antibody levels in the sera and exposed chicken eggs. RESULTS: High IgY levels were observed following immunization; furthermore, higher reactivity was observed in the eggs and species-specific immune response was observed post final immunization. CONCLUSIONS: Chicken eggs can be used as sentinels to surveil vector saliva antibodies.
Subject(s)
Animals , Psychodidae/immunology , Saliva/immunology , Immunoglobulins/analysis , Chickens/parasitology , Eggs/parasitology , Insect Vectors/immunology , Anopheles/immunology , Time Factors , Enzyme-Linked Immunosorbent Assay , Leishmaniasis/transmission , Malaria/transmissionABSTRACT
BACKGROUND Lutzomyia umbratilis, the vector for Leishmania guyanensis in northern South America, has been found naturally infected with L. guyanensis only in areas north of the Negro and Amazon rivers. While populations of this sand fly species are also found in areas south of these rivers, these populations have never been reported to be infected and/or transmitting L. guyanensis. However, no studies on the corresponding host-parasite interactions are available. OBJECTIVES This study evaluated the interaction between Lu. guyanensis promastigotes and field-collected Lu. umbratilis sand flies from Rio Preto da Eva and Manacapuru, which are located to the north and south, respectively, of the Negro River. METHODS Procyclic and metacyclic attachment was quantified using an in vitro system. FINDINGS Low attachment of parasites to the midguts of insects collected from Manacapuru was detected. Conversely, greater binding of metacyclic parasites was observed in the midguts of insects collected from Rio Preto da Eva, and this attachment was more pronounced than that observed for procyclics (p < 0.03). MAIN CONCLUSIONS The Lu. umbratilis population from an area south of the Negro River has lower in vitro interaction with L. guyanensis. The higher attachment of L. guyanensis to midguts of insects from Rio Preto da Eva may suggest better vector competence. These findings are in accordance with previously reported epidemiological information of American cutaneous leishmaniasis (ACL) transmission in the Amazon.
Subject(s)
Animals , Female , Psychodidae/parasitology , Leishmania guyanensis/physiology , Digestive System/parasitology , Host-Parasite Interactions/physiology , Psychodidae/classification , Brazil , Rivers , GeographyABSTRACT
BACKGROUND Aedes aegypti is considered the main Zika virus (ZIKV) vector, and is thought to be responsible for the 2015-2016 outbreak in Brazil. Zika positive Ae. aegypti males collected in the field suggest that vertical and/or venereal transmission of ZIKV may occur. OBJECTIVES In this study, we aimed to demonstrate that venereal transmission of ZIKV by Ae. aegypti can occur under laboratory conditions. METHODS Ae. aegypti collected in the city of Manaus, confirmed as negative for Zika, Dengue and Chikungunya virus by reverse transcription real-time polymerase chain reaction (RT-qPCR) (AaM3V- strain), were reared under laboratory conditions and used for the experiments. The ZIKV used in this study was isolated from a patient presenting with symptoms; ZIKV was confirmed by RT-qPCR. Experiment 1: virgin male mosquitoes of AaM3V- strain were intrathoracically inoculated with a ZIKV suspension; four days after injection, they were transferred to a cage containing virgin females of AaM3V- strain and left to copulate for five days. Experiment 2: virgin female mosquitoes of AaM3V- strain were orally infected with a ZIKV suspension by blood feeding membrane assay; nine days after blood feeding, they were placed in cages with Ae. aegypti AaM3V- virgin males and left to copulate for four days. After copulation, all mosquitoes were individually evaluated for viral infection by RT-qPCR. FINDINGS The mean infection rate in Experiment 1 and Experiment 2 was 45% and 35%, respectively. In both experiments, cycle threshold values ranged from 13 to 35, indicating the presence of viral genomes. MAIN CONCLUSION Ae. aegypti males intrathoracically inoculated with a ZIKV suspension are infected and can transmit the virus to uninfected females by mating. Moreover, Ae. aegypti females orally infected with a ZIKV suspension can transmit the virus to uninfected males by copulation. This study shows that ZIKV infection of Ae. aegypti mosquitoes occurs not only during blood feeding, but also during copulation.
Subject(s)
Animals , Sexually Transmitted Diseases/veterinary , Aedes/virology , Zika Virus/isolation & purification , Zika Virus/physiology , Copulation , Reverse Transcriptase Polymerase Chain ReactionABSTRACT
Phlebotomine sand flies are insects of medical importance. Species in the Neotropical region are highly diverse. Some of these species are considered cryptic species because of their morphological similarity between adult females of different species make identification especially difficult. The aim of this study was to analyze and describe the armature in the genital atrium (AGA) of some adult female sand flies, in order to discover new taxonomic characters that make it possible to distinguish between species that would otherwise be treated as cryptic by analysis of the AGA. The AGA of 16 Phlebotomine sand fly species are described. Distinct differences were found in relation to the shape and size of the armature, the presence or absence of spines on the armature, and the shape, size, and grouping patterns of the spines. These characters made it possible to distinguish between the species studied.
Os flebotomíneos são insetos de importância médica. Na região Neotropical existe grande diversidade de espécies. Algumas dessas espécies são consideradas espécies crípticas devido às semelhanças morfológicas entre fêmeas adultas de diferentes espécies, tornando a identificação especialmente difícil. O objetivo deste estudo foi analisar e descrever a armadura no átrio genital (AAG) de algumas fêmeas adultas de flebotomíneos, a fim de descobrir novos caracteres taxonômicos que tornem possível a distinção por análise da AAG entre as espécies que poderiam ser tratadas como espécies crípticas. Foram descritas a AAG de 16 espécies de flebotomíneos. Diferenças distintas foram encontradas em relação à forma e ao tamanho da armadura, a presença ou ausência de espinhos na armadura, e a forma, tamanho e padrões de agrupamento dos espinhos. Esses caracteres tornou possível a distinção entre as espécies estudadas.
Subject(s)
Female , Animals , Genitalia, Female/anatomy & histology , Psychodidae/anatomy & histology , Psychodidae/classificationABSTRACT
A malária é um problema de saúde pública. O Brasil é o país sul-americano que mais casos aporta todo ano, a maioria deles ocorridos na região Amazônica. Até o presente não há nenhuma vacina eficaz contra a malária. O controle dessa doença baseia-se principalmente no combate vetorial. Um dos desafios atuais é encontrar novas moléculas úteis para bloquear a transmissão da malária no vetor, sendo necessário para isso conhecer a biologia da interação entre os parasitos e seus hospedeiros. A maioria dos grupos de pesquisa utiliza como modelos de laboratórios combinações não naturais de Anopheles Plasmodium. Neste trabalho foi avaliada a suscetibilidade ao P. vivax em espécies Amazônicas de Anopheles, fêmeas de Anopheles darlingi, An. albitarsis s.l., An. nuneztovari s.l. e An. triannulatus s.l. e An.aquasalis foram infectadas com P. vivax utilizando um sistema de infecção experimental por membrana artificial...
Todas as espécies de Anopheles estudadas foram suscetíveis à infecção por P. vivax, porém a taxa de infecção e o numero de oocistos variaram significativamente entre elas. An. aquasalis (Spearman rho = 0.255, n = 386, p < 0.01) e An. darlingi (rho =0.518; n = 54, p < 0.01) mostraram uma correlação positiva entre o número de gametócitos e o número de oocistos formados. Também foi avaliada a via JAK/STAT de resposta imune em A. aquasalis, durante a fase tardia da infecção, e em A. darlingi, no início da infecção. A expressão dos genes STAT, PIAS e NOS foi avaliada por q-PCR. Em An. aquasalis a expressão dos genes estudados foi induzida a partir de 8 dPI (PIAS e NOS) e 12 dPI (STAT),e começou a diminuir aos 14dPI, provavelmente indicando a indução transitória desses genes na fase tardia da infecção. Em An. darlingi não foi observada a ativação dessa via imune durante a fase inicial da infecção com P. vivax. Estudos futuros devem ser realizados para saber de que forma os genes regulados pela via JAK/STAT podem modular o desenvolvimento do P. vivax em An. aquasalis, e outras vias de sinalização devem ser estudadas na resposta de An. darlingi à infecção pelo Plasmodium...
Subject(s)
Animals , Anopheles/parasitology , Host-Parasite Interactions/immunology , Malaria/prevention & control , Plasmodium vivax/pathogenicityABSTRACT
A malária é um problema de saúde pública. O Brasil é o país sul-americano que mais casos aporta todo ano, a maioria deles ocorridos na região Amazônica. Até o presente não há nenhuma vacina eficaz contra a malária. O controle dessa doença baseia-se principalmente no combate vetorial. Um dos desafios atuais é encontrar novas moléculas úteis para bloquear a transmissão da malária no vetor, sendo necessário para isso conhecer a biologia da interação entre os parasitos e seus hospedeiros. A maioria dos grupos de pesquisa utiliza como modelos de laboratórios combinações não naturais de Anopheles Plasmodium. Neste trabalho foi avaliada a suscetibilidade ao P. vivax em espécies Amazônicas de Anopheles, fêmeas de Anopheles darlingi, An. albitarsis s.l., An. nuneztovari s.l. e An. triannulatus s.l. e An.aquasalis foram infectadas com P. vivax utilizando um sistema de infecção experimental por membrana artificial.
Todas as espécies de Anopheles estudadas foram suscetíveis à infecção por P. vivax, porém a taxa de infecção e o numero de oocistos variaram significativamente entre elas. An. aquasalis (Spearman rho = 0.255, n = 386, p < 0.01) e An. darlingi (rho =0.518; n = 54, p < 0.01) mostraram uma correlação positiva entre o número de gametócitos e o número de oocistos formados. Também foi avaliada a via JAK/STAT de resposta imune em A. aquasalis, durante a fase tardia da infecção, e em A. darlingi, no início da infecção. A expressão dos genes STAT, PIAS e NOS foi avaliada por q-PCR. Em An. aquasalis a expressão dos genes estudados foi induzida a partir de 8 dPI (PIAS e NOS) e 12 dPI (STAT),e começou a diminuir aos 14dPI, provavelmente indicando a indução transitória desses genes na fase tardia da infecção. Em An. darlingi não foi observada a ativação dessa via imune durante a fase inicial da infecção com P. vivax. Estudos futuros devem ser realizados para saber de que forma os genes regulados pela via JAK/STAT podem modular o desenvolvimento do P. vivax em An. aquasalis, e outras vias de sinalização devem ser estudadas na resposta de An. darlingi à infecção pelo Plasmodium.
Subject(s)
Animals , Anopheles/parasitology , Host-Parasite Interactions/immunology , Malaria/prevention & control , Plasmodium vivax/pathogenicityABSTRACT
Aedes albopictus é registrado pela primeira vez no estado de Roraima, Brasil. Entre junho de 2006 e maio de 2007 foram coletadas três pupas e dez larvas, duas das quais chegaram à fase adulta, durante atividades de vigilância rotineiras em três bairros urbanos da cidade de Boa Vista. Embora essa espécie não seja incriminada como vetor primário do dengue, a sua presença pode favorecer a ligação entre os ciclos silvestre e urbano da febre amarela e de outras arboviroses no Brasil.
Aedes albopictus is registered for the first time in Roraima, Brazil. From June 2006 to May 2007, three pupae and ten larvae of Ae. albopictus were collected, during routine surveillance work in three urban neighborhoods in the city of Boa Vista. Two larvae reached adulthood as females. Although Ae. albopictus is not presently considered of primary importance in dengue transmission, its occurrence could favor a linkage between urban and forest cycles of yellow fever and other arboviruses in Brazil.