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来自水生生物膜样本的鱼类环境DNA宏条形码分析:方法学方面

Fish eDNA metabarcoding from aquatic biofilm samples: Methodological aspects.

作者信息

Rivera Sinziana F, Rimet Frédéric, Vasselon Valentin, Vautier Marine, Domaizon Isabelle, Bouchez Agnès

机构信息

INRA, UMR CARRTEL, Université Savoie Mont-Blanc, Thonon-les-Bains, France.

Scimabio-Interface, Thonon les Bains, France.

出版信息

Mol Ecol Resour. 2022 May;22(4):1440-1453. doi: 10.1111/1755-0998.13568. Epub 2021 Dec 14.

DOI:10.1111/1755-0998.13568
PMID:34863036
Abstract

Fish eDNA metabarcoding is usually performed from filtered water samples. The volume of filtered water depends on the study scope and can rapidly become time consuming according to the number of samples that have to be processed. To avoid time allocated to filtration, passive DNA samplers have been used to recover fish eDNA from marine environments faster. In freshwater ecosystems, aquatic biofilms were used to catch eDNA from macroinvertebrates. Here, we test the capacity of aquatic biofilms to entrap fish eDNA in a large lake and, therefore, the possibility to perform fish eDNA metabarcoding from this matrix compared to the traditional fish eDNA approach from filtered water samples. Methodological aspects of the use of aquatic biofilms for fish eDNA metabarcoding (e.g. PCR replicates, biological replicates, bioinformatics pipeline, reference database and taxonomic assignment) were validated against a mock community. When using biofilms from habitats sheltered from wind and waves, biofilm and water approach provided similar inventories. Richness and diversity were comparable between both approaches. Approaches differed only for rare taxa. Our results illustrate the capacity of aquatic biofilms to act as passive eDNA samplers of fish eDNA and, therefore, the possibility to use biofilms to monitor fish communities efficiently from biofilms. Furthermore, our results open up avenues of research to study a diversity of biological groups (among which bioindicators as diatoms, macroinvertebrates and fish) from eDNA isolated from a single environmental matrix reducing sampling efforts, analysis time and costs.

摘要

鱼类环境DNA宏条形码分析通常从过滤后的水样中进行。过滤水的体积取决于研究范围,并且根据需要处理的样本数量,很快就会变得耗时。为了避免分配给过滤的时间,已使用被动式DNA采样器从海洋环境中更快地回收鱼类环境DNA。在淡水生态系统中,水生生物膜被用于捕获大型无脊椎动物的环境DNA。在此,我们测试了水生生物膜在大型湖泊中捕获鱼类环境DNA的能力,因此,与从过滤水样中提取鱼类环境DNA的传统方法相比,测试了从这种基质中进行鱼类环境DNA宏条形码分析的可能性。针对模拟群落验证了将水生生物膜用于鱼类环境DNA宏条形码分析的方法学方面(例如PCR重复、生物学重复、生物信息学流程、参考数据库和分类学归属)。当使用来自避风浪栖息地的生物膜时,生物膜和水样方法提供了相似的物种清单。两种方法的丰富度和多样性相当。两种方法仅在稀有分类群上有所不同。我们的结果说明了水生生物膜作为鱼类环境DNA被动式环境DNA采样器的能力,因此,说明了利用生物膜有效监测鱼类群落的可能性。此外,我们的结果开辟了研究途径,可从单一环境基质中分离的环境DNA研究多种生物类群(其中包括作为生物指示物的硅藻、大型无脊椎动物和鱼类),从而减少采样工作量、分析时间和成本。

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