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. 2020 Oct 14;14(10):e0008666.
doi: 10.1371/journal.pntd.0008666. eCollection 2020 Oct.

Tripartite interactions: Leishmania, microbiota and Lutzomyia longipalpis

Affiliations

Tripartite interactions: Leishmania, microbiota and Lutzomyia longipalpis

Thais Bonifácio Campolina et al. PLoS Negl Trop Dis. .

Abstract

The microbial consortium associated with sandflies has gained relevance, with its composition shifting throughout distinct developmental stages, being strongly influenced by the surroundings and food sources. The bacterial components of the microbiota can interfere with Leishmania development inside the sandfly vector. Microbiota diversity and host-microbiota-pathogen interactions regarding New World sandfly species have yet to be thoroughly studied, particularly in Lutzomyia longipalpis, the primary vector of visceral leishmaniasis in Brazil.The native microbiota of different developmental stages and physiological conditions of Lu. longipalpis (Lapinha Cave), was described by culturing and 16s rRNA gene sequencing. The 16s rRNA sequencing of culture-dependent revealed 13 distinct bacterial genera (Bacillus, Enterococcus, Erwinia, Enterobacter, Escherichia, Klebsiella, Lysinibacillus, Pseudocitrobacter, Providencia, Pseudomonas, Serratia, Staphylococcus and Solibacillus). The in vitro and in vivo effects of each one of the 13 native bacteria from the Lu. longipalpis were analyzed by co-cultivation with promastigotes of L.i. chagasi, L. major, L. amazonensis, and L. braziliensis. After 24 h of co-cultivation, a growth reduction observed in all parasite species. When the parasites were co-cultivated with Lysinibacillus, all parasites of L. infantum chagasi and L. amazonensis died within 24 hours. In the in vivo co-infection of L.chagasi, L. major and L. amazonensis with the genera Lysinibacillus, Pseudocitrobacter and Serratia it was possible to observe a significant difference between the groups co-infected with the bacterial genera and the control group.These findings suggest that symbiont bacteria (Lysinibacillus, Serratia, and Pseudocitrobacter) are potential candidates for paratransgenic or biological control. Further studies are needed to identify the nature of the effector molecules involved in reducing the vector competence for Leishmania.

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Conflict of interest statement

The authors have declared that no competing interests exist.

Figures

Fig 1
Fig 1. The short effect, in the parasite, when growth co-cultured with native bacteria.
A short temporal evaluation (0 to 120 minutes) showing the activity of each one of the ten native bacteria isolated from Lu. longipalpis when co-culture with four Leishmania species: (A) L.i. chagasi, (B) L. amazonensis, (C) L. braziliensis, and (D) L. major.
Fig 2
Fig 2. The long term mortality of Leishmania species when co-cultured with native bacteria.
Over a 120 hrs. evaluation showing a reduction in parasite growth exerted upon four Leishmania species when co-cultured with ten bacterial genera isolated from Lu. longipalpis. (A) L.i. chagasi, (B) L. amazonensis, (C) L. braziliensis, and (D) L. major.
Fig 3
Fig 3. The effect of co-infection of L. i. chagasi and native bacteria.
In vivo co-infection showing the result of the co-infection of L. i. chagasi (initial concentration 4x106 parasites/mL) with all ten bacterial taxa (initial concentration of 108 CFU/mL) isolated from Lu. longipalpis. The midguts individually macerated, and the number of parasites alive counted under a hemocytometer. The groups co-infected with Serratia and Lysinibacillus showed the lowest infection rate (statistically significant differences observed. α = 0.05). Six days post-infection, for all isolates, the number of parasites per midgut was lower than the pre-treated control.
Fig 4
Fig 4. Co-infection with the native bacteria and the effect in the live parasite.
In vivo co- infection of L. i. chagasi (A), L. amazonensis (B), and L. major (C) with the genera Lysinibacillus, Pseudocitrobacter, or Serratia affect live parasite counts. The sandflies were infected by artificial feeding with 4 × 106mL logarithmic phase promastigotes and bacterial isolates at 1 x 108 / mL. Three and six days post-infection the midguts were individually macerated Moreover, the number of parasites alive counted under a hemocytometer.

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