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距离、流速和 PCR 抑制:两种源头溪流中的 eDNA 动态。

Distance, flow and PCR inhibition: eDNA dynamics in two headwater streams.

机构信息

Department of Environmental Conservation, University of Massachusetts, Amherst, MA, 01003, USA.

出版信息

Mol Ecol Resour. 2015 Jan;15(1):216-27. doi: 10.1111/1755-0998.12285. Epub 2014 Jun 13.

DOI:10.1111/1755-0998.12285
PMID:24890199
Abstract

Environmental DNA (eDNA) detection has emerged as a powerful tool for monitoring aquatic organisms, but much remains unknown about the dynamics of aquatic eDNA over a range of environmental conditions. DNA concentrations in streams and rivers will depend not only on the equilibrium between DNA entering the water and DNA leaving the system through degradation, but also on downstream transport. To improve understanding of the dynamics of eDNA concentration in lotic systems, we introduced caged trout into two fishless headwater streams and took eDNA samples at evenly spaced downstream intervals. This was repeated 18 times from mid-summer through autumn, over flows ranging from approximately 1-96 L/s. We used quantitative PCR to relate DNA copy number to distance from source. We found that regardless of flow, there were detectable levels of DNA at 239.5 m. The main effect of flow on eDNA counts was in opposite directions in the two streams. At the lowest flows, eDNA counts were highest close to the source and quickly trailed off over distance. At the highest flows, DNA counts were relatively low both near and far from the source. Biomass was positively related to eDNA copy number in both streams. A combination of cell settling, turbulence and dilution effects is probably responsible for our observations. Additionally, during high leaf deposition periods, the presence of inhibitors resulted in no amplification for high copy number samples in the absence of an inhibition-releasing strategy, demonstrating the necessity to carefully consider inhibition in eDNA analysis.

摘要

环境 DNA(eDNA)检测已成为监测水生生物的有力工具,但在各种环境条件下,水生 eDNA 的动态仍知之甚少。溪流和河流中的 DNA 浓度不仅取决于 DNA 进入水体的平衡,还取决于通过降解离开系统的 DNA,还取决于下游运输。为了提高对流水系统中 eDNA 浓度动态的理解,我们将笼养鳟鱼引入两条无鱼的源头溪流,并在均匀间隔的下游间隔处采集 eDNA 样本。从仲夏到秋季,在大约 1-96 L/s 的流量范围内重复了 18 次。我们使用定量 PCR 将 DNA 拷贝数与距离源的关系。我们发现,无论流量如何,在 239.5 m 处都可以检测到 DNA 水平。流量对 eDNA 计数的主要影响在两条溪流中方向相反。在最低流量下,靠近源的 eDNA 计数最高,并迅速随距离衰减。在最高流量下,靠近和远离源的 DNA 计数都相对较低。生物量与两条溪流中的 eDNA 拷贝数呈正相关。细胞沉降、湍流和稀释效应的组合可能是造成我们观察结果的原因。此外,在高叶片沉积期,由于缺乏抑制物释放策略,抑制剂的存在导致高拷贝数样本无法扩增,这表明在 eDNA 分析中必须仔细考虑抑制作用。

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