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Development and application of an eDNA method to detect and quantify a pathogenic parasite in aquatic ecosystems

机译:开发和应用eDNA方法检测和定量水生生态系统中的致病性寄生虫

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Approaches based on organismal DNA found in the environment (eDNA) have become increasingly utilized for ecological studies and biodiversity inventories as an alternative to traditional field survey methods. Such DNA-based techniques have largely been used to establish the presence of free-living organisms, but have much potential for detecting and quantifying infectious agents in the environment, which is necessary to evaluate disease risk. We developed an eDNA method to examine the distribution and abundance of the trematode Ribeiroia ondatrae, a pathogenic parasite known to cause malformations in North American amphibians. In addition to comparing this eDNA approach to classical host necropsy, we examined the detectability of R. ondatrae in water samples subject to different degradation conditions (time and temperature). Our test exhibited high specificity and sensitivity to R. ondatrae, capable of detecting as little as 14 fg (femtograms) of this parasite's DNA (1/2500th of a single infectious stage) from field water samples. Compared to our results from amphibian host necropsy, quantitative PCR was similar to 90% concordant with respect to R. ondatrae detection from 15 field sites and was also a significant predictor of host infection abundance. DNA was still detectable in lab samples after 21 days at 25 degrees C, indicating that our method is robust to field conditions. By comparing the advantages and disadvantages of eDNA vs. traditional survey methods for determining pathogen presence and abundance in the field, we found that the lower cost and effort associated with eDNA approaches provide many advantages. The development of alternative tools is critical for disease ecology, as wildlife management and conservation efforts require reliable establishment and monitoring of pathogens.
机译:环境中发现的基于有机体DNA(eDNA)的方法已越来越多地用于生态研究和生物多样性清单,以替代传统的田间调查方法。这种基于DNA的技术已广泛用于建立自由生物的存在,但在检测和量化环境中的传染原方面具有很大的潜力,这是评估疾病风险的必要条件。我们开发了一种eDNA方法来检查吸虫吸虫Ribeiroia ondatrae的分布和丰度,该病原体是已知会导致北美两栖动物畸形的致病性寄生虫。除了将这种eDNA方法与经典的尸体尸检进行比较之外,我们还研究了在不同降解条件(时间和温度)下水样中黄花菜的可检测性。我们的测试对R. ondatrae表现出高度的特异性和敏感性,能够从田间水样中检测出这种寄生虫的DNA低至14 fg(飞克)(单个感染阶段的1/2500)。与我们从两栖动物尸体尸检中得到的结果相比,定量PCR与从15个野外站点检测到的金黄色花念珠菌相似,达到90%一致,并且也是宿主感染丰度的重要预测指标。在25摄氏度下21天后,仍可在实验室样品中检测到DNA,这表明我们的方法对田间条件具有鲁棒性。通过比较eDNA与传统调查方法在现场确定病原体存在和丰度的优缺点,我们发现与eDNA方法相关的较低成本和工作量具有许多优点。替代工具的开发对于疾病生态至关重要,因为野生动植物的管理和保护工作需要可靠地建立和监测病原体。

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