2024-03-29T15:43:21Zhttp://repisalud.isciii.es/oai/requestoai:repisalud.isciii.es:20.500.12105/94222023-09-28T07:16:05Zcom_20.500.12105_2060com_20.500.12105_2052com_20.500.12105_2051col_20.500.12105_2061
Repisalud
author
Remadi, Latifa
author
Chargui, Najla
author
Jimenez, Maribel
author
Molina, Ricardo
author
Haouas, Najoua
author
Gonzalez, Estela
author
Chaabane-Banaouas, Raja
author
Ben Salah, Eya
author
Haddaji, Mohsen
author
Chaabouni, Yassine
author
Babba, Hamouda
2020-04-03T07:38:24Z
2020-04-03T07:38:24Z
2020-03
PLoS Negl Trop Dis. 2020 Mar 26;14(3):e0008077.
1935-2735
http://hdl.handle.net/20.500.12105/9422
32214313
10.1371/journal.pntd.0008077
1935-2735
PLoS neglected tropical diseases
BACKGROUND: Phlebotomus (Larroussius) perniciosus and Canis familiaris are respectively the only confirmed vector and reservoir for the transmission of Leishmania (L.) infantum MON-1 in Tunisia. However, the vector and reservoir hosts of the two other zymodemes, MON-24 and MON-80, are still unknown. The aim of this study was to analyze the L. infantum life cycle in a Tunisian leishmaniasis focus. For this purpose, we have focused on: i) the detection, quantification and identification of Leishmania among this sand fly population, and ii) the analysis of the blood meal preferences of Larroussius (Lar.) subgenus sand flies to identify the potential reservoirs. METHODOLOGY AND FINDINGS: A total of 3,831 sand flies were collected in seven locations from the center of Tunisia affected by human visceral leishmaniasis. The collected sand flies belonged to two genus Phlebotomus (Ph.) (five species) and Sergentomyia (four species). From the collected 1,029 Lar. subgenus female sand flies, 8.26% was positive to Leishmania by ITS1 nested PCR. Three Leishmania spp. were identified: L. infantum 28% (24/85), L. killicki 13% (11/85), and L. major 22% (19/85). To identify the blood meal sources in Ph. Lar. subgenus sand flies, engorged females were analyzed by PCR-sequencing targeting the vertebrate cytochrome b gene. Among the 177 analyzed blood-fed females, 169 samples were positive. Sequencing results showed seven blood sources: cattle, human, sheep, chicken, goat, donkey, and turkey. In addition, mixed blood meals were detected in twelve cases. Leishmania DNA was found in 21 engorged females, with a wide range of blood meal sources: cattle, chicken, goat, chicken/cattle, chicken/sheep, chicken/turkey and human/cattle. The parasite load was quantified in fed and unfed infected sand flies using a real time PCR targeting kinetoplast DNA. The average parasite load was 1,174 parasites/reaction and 90 parasites/reaction in unfed and fed flies, respectively. CONCLUSION: Our results support the role of Ph. longicuspis, Ph. perfiliewi, and Ph. perniciosus in L. infantum transmission. Furthermore, these species could be involved in L. major and L. killicki life cycles. The combination of the parasite detection and the blood meal analysis in this study highlights the incrimination of the identified vertebrate in Leishmania transmission. In addition, we quantify for the first time the parasite load in naturally infected sand flies caught in Tunisia. These findings are relevant for a better understanding of L. infantum transmission cycle in the country. Further investigations and control measures are needed to manage L. infantum transmission and its spreading.
eng
Molecular detection and identification of Leishmania DNA and blood meal analysis in Phlebotomus (Larroussius) species
journal article
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URL
https://repisalud.isciii.es/bitstream/20.500.12105/9422/1/MolecularDetectionAndIdentification_2020.pdf
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MolecularDetectionAndIdentification_2020.pdf
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https://repisalud.isciii.es/bitstream/20.500.12105/9422/5/MolecularDetectionAndIdentification_2020.pdf.txt
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MolecularDetectionAndIdentification_2020.pdf.txt