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首页> 外文期刊>Molecular ecology resources >Evaluating environmental DNA-based quantification of ranavirus infection in wood frog populations
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Evaluating environmental DNA-based quantification of ranavirus infection in wood frog populations

机译:评估蛙蛙种群中基于环境DNA的蛙病毒感染的定量分析

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摘要

A variety of challenges arise when monitoring wildlife populations for disease. Sampling tissues can be invasive to hosts, and obtaining sufficient sample sizes can be expensive and time-consuming, particularly for rare species and when pathogen prevalence is low. Environmental DNA (eDNA)-based detection of pathogens is an alternative approach to surveillance for aquatic communities that circumvents many of these issues. Ranaviruses are emerging pathogens of ectothermic vertebrates linked to die-offs of amphibian populations. Detecting ranavirus infections is critical, but nonlethal methods have the above issues and are prone to false negatives. We report on the feasibility and effectiveness of eDNA-based ranavirus detection in the field. We compared ranavirus titres in eDNA samples collected from pond water to titres in wood frog (Lithobates sylvaticus; n=5) tadpoles in sites dominated by this one species (n=20 pond visits). We examined whether ranavirus DNA can be detected in eDNA from pond water when infections are present in the pond and if viral titres detected in eDNA samples correlate with the prevalence or intensity of ranavirus infections in tadpoles. With three 250mL water samples, we were able to detect the virus in all visits with infected larvae (0.92 diagnostic sensitivity). Also, we found a strong relationship between the viral eDNA titres and titres in larval tissues. eDNA titres increased prior to observed die-offs and declined afterwards, and were two orders of magnitude higher in ponds with a die-off. Our results suggest that eDNA is useful for detecting ranavirus infections in wildlife and aquaculture.
机译:监测野生动植物种群的疾病时会遇到各种挑战。采样组织可能会侵入宿主,获取足够的样本量可能既昂贵又耗时,特别是对于稀有物种以及病原体流行率较低的情况。基于环境DNA(eDNA)的病原体检测是对水生生物进行监视的另一种方法,可以规避许多这些问题。鼻病毒是与两栖动物种群死亡相关的外热脊椎动物的病原体。检测鼻病毒感染至关重要,但是非致命方法存在上述问题,并且容易出现假阴性。我们报告在现场基于eDNA的鼻病毒检测的可行性和有效性。我们比较了从池塘水中收集的eDNA样品中的蛙病毒滴度与该物种占主导地位的地点的蛙(Lithobates sylvaticus; n = 5)tit的滴度(n = 20)。我们检查了池塘中是否存在感染时,是否可以在池塘水中的eDNA中检测到蛙病毒DNA,以及在eDNA样品中检测到的病毒滴度是否与ra中的蛙病毒感染的发生率或强度相关。使用三个250mL的水样本,我们能够在所有被感染的幼虫中进行检测(诊断灵敏度为0.92)。此外,我们发现病毒eDNA滴度与幼虫组织的滴度之间有很强的关系。 eDNA滴度在观察到死亡之前先升高,然后下降,在死亡的池塘中升高了两个数量级。我们的结果表明,eDNA可用于检测野生动植物和水产养殖中的鼻病毒感染。

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