Proficiency testing and cross-laboratory method comparison to support standardisation of diatom DNA metabarcoding for freshwater biomonitoring.

Valentin Vasselon, Sinziana F Rivera, Éva Ács, Salomé Baja Almeida, Karl B Andree, Laure Apothéloz-Perret-Gentil, Bonnie Bailet, Ana Baričević, Kevin K Beentjes, Juliane Bettig, Agnès Bouchez, Camilla Capelli, Cécile Chardon, Mónika Duleba, Tina Elersek, Clémence Genthon, Maša Jablonska, Louis Jacas, Maria Kahlert, Martyn G Kelly, Jan-Niklas Macher, Federica Mauri, Marina Moletta-Denat, Andreia Mortágua, Jan Pawlowski, Javier Pérez-Burillo, Martin Pfannkuchen, Erik Pilgrim, Panayiota Pissaridou, Frédéric Rimet, Karmen Stanic, Kálmán Tapolczai, Susanna Theroux, Rosa Trobajo, Berry Van der Hoorn, Marlen I Vasquez, Marie Vidal, David Wanless, Jonathan Warren, Jonas Zimmermann, Benoît Paix
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Abstract

DNA metabarcoding of benthic diatoms has been successfully applied for biomonitoring at the national scale and can now be considered technically ready for routine application. However, protocols and methods still vary between and within countries, limiting their transferability and the comparability of results. In order to overcome this, routine use of DNA metabarcoding for diatom biomonitoring requires knowledge of the sources of variability introduced by the different steps of the procedure. Here, we examine how elements of routine procedures contribute to variability between European laboratories. A set of four experiments were performed focusing on DNA extraction and PCR amplification steps to evaluate their reproducibility between different laboratories and the variability introduced by different protocols currently applied by the scientific community. Under the guidance of a reference laboratory, 17 participants from 14 countries performed DNA extraction and PCR amplification in parallel, using the same fixed protocol and their own choice of protocol. Experiments were performed by each participant on a set of standardised DNA and biofilm samples (river, lake and mock community) to investigate potential systematic and random errors. Our results revealed the successful transferability of a protocol amongst labs and a highly similar and consistent ecological assessment outcome obtained regardless of the protocols used by each participant. We propose an "all for one but prove them all" strategy, suggesting that distinct protocols can be used within the scientific community, as long as their consistency is be proven by following minimum standard requirements.

能力测试和跨实验室方法比较,以支持用于淡水生物监测的硅藻DNA元条形码标准化。
底栖硅藻的DNA元条形码已成功应用于全国范围的生物监测,现在可以认为技术上准备好常规应用。然而,议定书和方法在国家之间和国家内部仍然各不相同,限制了它们的可转移性和结果的可比性。为了克服这一点,常规使用DNA元条形码进行硅藻生物监测需要了解由程序的不同步骤引入的变异性来源。在这里,我们研究了常规程序的元素如何导致欧洲实验室之间的差异。本文对DNA提取和PCR扩增步骤进行了四组实验,以评估其在不同实验室之间的可重复性,以及目前科学界采用的不同方案所引入的可变性。在参比实验室的指导下,来自14个国家的17名参与者使用相同的固定方案和自己选择的方案,同时进行DNA提取和PCR扩增。每位参与者在一组标准化的DNA和生物膜样本(河流、湖泊和模拟群落)上进行实验,以调查潜在的系统和随机误差。我们的结果揭示了实验室之间协议的成功可转移性,并且无论每个参与者使用何种协议,都获得了高度相似和一致的生态评估结果。我们提出了一个“人人为一,但要证明所有”的策略,建议在科学界使用不同的协议,只要它们的一致性是通过遵循最低标准要求来证明的。
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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来源期刊
Metabarcoding and Metagenomics
Metabarcoding and Metagenomics Agricultural and Biological Sciences-Animal Science and Zoology
CiteScore
5.40
自引率
0.00%
发文量
25
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