Development of a loop-mediated isothermal amplification assay for detection of Austropeplea tomentosa from environmental water samples.

Lily Tran, Vignesh A Rathinasamy, Travis Beddoe
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引用次数: 1

Abstract

Lymnaeid snails are key intermediate hosts for the development and survival of Fasciola spp., the causative agent of Fascioliasis which are economically important parasites infecting humans and livestock globally. The current control method for treating Fascioliasis is heavily reliant on anthelmintic drugs, particularly Triclabendazole (TCBZ) which has resulted in drug-resistant parasites and poses significant risk as there are no long-term efficacious alternatives available. Sustainable control measures at the farm level could include both parasite and snail control will play an important role in Fasciola spp. control and reduce the reliance on anthelmintic drugs. Implementation of such sustainable control measures requires effective identification of snails on the property however Lymnaeid snails are small and difficult to physically locate. Snail identification using an environmental DNA approach is a recent approach in which physically locating snails are not required. Austropeplea tomentosa, is the primary intermediate snail host for F. hepatica transmission in South-East Australia and we present an in-field loop-mediated isothermal amplification and water filtering method for the detection of A. tomentosa eDNA from water samples to improve current surveillance methods. This methodology is highly sensitive with a detection limit of 5 × 10- 6 ng/μL, detected in < 20 minutes, with cumulative sample preparation and amplification time under 1 hour. This proposed workflow could assist in monitoring areas to determine the risk of Fascioliasis infection and implement strategies to manage snail populations to ultimately reduce the risk of infection for humans and livestock.

Supplementary information: The online version contains supplementary material available at 10.1186/s44149-022-00061-9.

Abstract Image

Abstract Image

建立环介导等温扩增法检测环境水样中绒毛南拟虫。
片形吸虫病是全球范围内重要的经济寄生虫,其病原是片形吸虫病,线虫螺是片形吸虫病发展和存活的关键中间宿主。目前治疗片形吸虫病的控制方法严重依赖驱虫药,特别是三氯苯达唑(TCBZ),这导致寄生虫产生耐药性,由于没有长期有效的替代品,因此具有重大风险。农场层面的可持续控制措施可包括寄生虫和蜗牛控制,这将在片形吸虫控制中发挥重要作用,并减少对驱虫药物的依赖。实施这种可持续的控制措施需要有效地识别该财产上的蜗牛,然而林奈蜗牛很小,难以物理定位。使用环境DNA方法鉴定蜗牛是最近的一种方法,在这种方法中不需要物理定位蜗牛。为了改进现有的监测方法,我们提出了一种现场环介导的等温扩增和水过滤方法,用于从水样中检测毛毛拟虫的eDNA。本方法灵敏度高,检出限为5 × 10 ~ 6 ng/μL,详见补充资料:在线补充资料:10.1186/s44149-022-00061-9。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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CiteScore
2.40
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