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首页> 外文期刊>International Journal for Parasitology: Parasites and Wildlife >Utilising a novel surveillance system to investigate species of Forcipomyia (Lasiohelea) (Diptera: Ceratopogonidae) as the suspected vectors of Leishmania macropodum (Kinetoplastida: Trypanosomatidae) in the Darwin region of Australia
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Utilising a novel surveillance system to investigate species of Forcipomyia (Lasiohelea) (Diptera: Ceratopogonidae) as the suspected vectors of Leishmania macropodum (Kinetoplastida: Trypanosomatidae) in the Darwin region of Australia

机译:利用新型监测系统来调查澳大利亚达尔文地区的Leishmania Macropodum(Kinetoplastida:Trypanosomatidaidae)的疑似载体

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摘要

Up until recently, Australia was considered free of Leishmania due to the absence of phlebotomine sandfly species (Diptera: Phlebotominae) known to transmit Leishmania parasites in other parts of the world. The discovery of Leishmania ( Mundinia ) macropodum (Kinetoplastida: Trypanosomatidae) in Northern Australia sparked questions as to the existence of alternative vectors of Leishmania . This has added to the complexity of fully understanding the parasite's interaction with its vector, which is known to be very specific. Previous findings demonstrated L. macropodum infection beyond the blood meal stage in the day-biting midges Forcipomyia ( Lasiohelea ) Kieffer (Diptera: Ceratopogonidae) implicating them in the parasite's life cycle. Currently, there is no conclusive evidence demonstrating this suspected vector to transmit L . macropodum to a na?ve host. Therefore, this research aimed to investigate the vector competency of day-biting midge F. ( Lasiohelea ) to transmit L . macropodum utilising a novel technology that preserves nucleic acids. Honey-soaked Flinders Technology Associates (FTA?) filter-paper cards were used to obtain saliva expectorated from biting midges while sugar-feeding. F . ( Lasiohelea ) were aspirated directly off macropods from a known Leishmania -transmission site and were kept in a waxed-paper container holding a honey-coated FTA? card for feeding. Insect identification and Taqman quantitative real-time PCR (qPCR) screening assays revealed L. macropodum DNA in F. ( Lasiohelea ) up to 7 days post field-collection, and in an unidentified biting midge, previously known as F. (Lasiohelea ) sp.1. Moreover, 7/145 (4.83%) of FTA? cards were confirmed positive with L . macropodum DNA after exposure to field-collected F. (Lasiohelea ). Additionally, FTA? cards were found to be a valuable surveillance tool, given the ease of use in the field and laboratory. Overall, our findings support previous reports on L . macropodum transmission by an alternative vector to phlebotomine sandflies. Further studies identifying and isolating infective L. macropodum promastigotes is necessary to resolve questions on the L. macropodum vector.
机译:直到近期,由于没有含有痰含沙蝇物种(Diptera:Phlebotominae)在世界其他地区传播Leishmania寄生虫的嗜血麦芽肿种(Diptera:Phlebotominae),澳大利亚被认为是免费的。澳大利亚北部的Leishmania(Mundinia)Macropodum(Kinetoplastida:Trypanosomatidae)的发现引发了Leishmania替代载体的问题。这增加了完全了解寄生虫与其向量的互动的复杂性,这已知是非常具体的。以前的研究结果显示,超越血液膳食阶段的L. macropodum感染在咬血症的中午(Lasiohelea)Kieffer(Diptera:Ceratopogonidae)在寄生虫的生命周期中暗示它们。目前,没有确凿的证据证明这种疑似载体传输L. macropodum到na ve宿主。因此,这项研究旨在研究咬壁的载体能力(Lasiohelea)传递l。利用一种保留核酸的新技术的巨大技术。蜂蜜浸泡的剥落技术伙伴(FTA?)滤纸卡用于从喂食时从咬咬时从咬中的中间时咳出唾液。 F 。 (Lasiohelea)直接从已知的Leishmania-Tlearsmission部位脱掉大鼠的宏od,并保存在持有蜂蜜涂层的FTA的蜡纸容器中?喂养卡。昆虫鉴定和Taqman定量实时PCR(QPCR)筛选测定揭示了F.(Lasiohelea)的L.Macropodum DNA,最多7天柱收集,并且在以前称为F.(LasioHelea)SP的未识别的咬合的中途.1。此外,7/145(4.83%)的FTA?卡被L阳性与L确认。在暴露于田间收集的F.(Lasiohelea)后Macropodum DNA。另外,FTA?鉴于该领域和实验室的易用性,发现卡片是一个有价值的监视工具。总体而言,我们的调查结果支持之前的L.通过替代载体的麦克脂传播到痰麦芽肿粉。在解决L.Macropodum载体上的问题是必要的鉴定和分离感染性L. macropodum癌症的进一步研究。

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