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水生环境 DNA 的样本保存和 PCR 前处理实用指南。

A practical guide to sample preservation and pre-PCR processing of aquatic environmental DNA.

机构信息

Department of Biology, University of Central Florida, Genomics and Bioinformatics Cluster, Orlando, FL, USA.

Department of Ocean Engineering and Marine Sciences, Florida Institute of Technology, Melbourne, FL, USA.

出版信息

Mol Ecol Resour. 2020 Jan;20(1):29-39. doi: 10.1111/1755-0998.13107. Epub 2019 Nov 12.

DOI:10.1111/1755-0998.13107
PMID:31633859
Abstract

Environmental DNA (eDNA) is rapidly growing in popularity as a tool for community assessments and species detection. While eDNA approaches are now widely applied, there is not yet agreement on best practices for sample collection and processing. Investigators looking to integrate eDNA approaches into their research programme are required to examine a growing collection of disparate studies to make an often uncertain decision about which protocols best fit their needs. To promote the application of eDNA approaches and to encourage the generation of high-quality data, here we review the most common techniques for the collection, preservation and extraction of metazoan eDNA from water samples. Specifically, we focus on experimental studies that compare various methods and outline the numerous challenges associated with eDNA. While the diverse applications of eDNA do not lend themselves to a one-size-fits-all recommendation, in most cases, capture/concentration of eDNA on cellulose nitrate filters (with pore size determined by water turbidity), followed by storage of filters in Longmire's buffer and extraction with a DNeasy Blood & Tissue Kit (or similar) has been shown to provide sufficient, high-quality DNA. However, we also emphasize the importance of testing and optimizing protocols for the system of interest.

摘要

环境 DNA(eDNA)作为群落评估和物种检测工具越来越受欢迎。虽然 eDNA 方法现在已经广泛应用,但对于样本采集和处理的最佳实践仍未达成共识。希望将 eDNA 方法纳入其研究计划的研究人员需要研究越来越多的不同研究,以便对哪些协议最符合其需求做出不确定的决定。为了促进 eDNA 方法的应用,并鼓励生成高质量的数据,我们在这里回顾了从水样中收集、保存和提取后生动物 eDNA 的最常见技术。具体来说,我们专注于比较各种方法的实验研究,并概述了与 eDNA 相关的许多挑战。虽然 eDNA 的多种应用不能一概而论,但在大多数情况下,使用纤维素硝酸酯滤器(根据水浊度确定孔径)来捕获/浓缩 eDNA,然后将滤器储存在 Longmire 的缓冲液中,并使用 DNeasy Blood & Tissue Kit(或类似的试剂盒)进行提取,已被证明可以提供足够的高质量 DNA。然而,我们还强调了针对感兴趣的系统测试和优化协议的重要性。

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