說明
This dataset contains eDNA metabarcoding data of fish species detected in 17 locations in the Belgian Part of the North Sea (BPNS). The seawater samples were collected during a field campaigns in 2022. The fish species were identified using 12S eDNA metabarcoding. The dataset includes amplicon sequence variants and their associated metadata.
[This dataset was processed using the GBIF eDNA converter tool.]
資料紀錄
此資源出現紀錄的資料已發佈為達爾文核心集檔案(DwC-A),其以一或多組資料表構成分享生物多樣性資料的標準格式。 核心資料表包含 94,281 筆紀錄。
亦存在 1 筆延伸集的資料表。延伸集中的紀錄補充核心集中紀錄的額外資訊。 每個延伸集資料表中資料筆數顯示如下。
此 IPT 存放資料以提供資料儲存庫服務。資料與資源的詮釋資料可由「下載」單元下載。「版本」表格列出此資源的其它公開版本,以便利追蹤其隨時間的變更。
版本
以下的表格只顯示可公開存取資源的已發布版本。
如何引用
研究者應依照以下指示引用此資源。:
Dukan N, Cornelis I, Brosens D, Derycke S (2024). Vertical and horizontal environmental DNA (eDNA) patterns of fish in a shallow and well-mixed North Sea area. Version 1.5. Flanders Research Institute for Agriculture, Fisheries and Food (ILVO). Occurrence dataset. https://ipt.inbo.be/resource?r=ilvo-metabarcoding-1&v=1.5
權利
研究者應尊重以下權利聲明。:
此資料的發布者及權利單位為 Flanders Research Institute for Agriculture, Fisheries and Food (ILVO)。 This work is licensed under a Creative Commons Attribution (CC-BY 4.0) License.
GBIF 註冊
此資源已向GBIF註冊,並指定以下之GBIF UUID: 8afcc57c-5d2b-4349-add6-29bfc33ed5cb。 Flanders Research Institute for Agriculture, Fisheries and Food (ILVO) 發佈此資源,並經由Ocean Biodiversity Information System同意向GBIF註冊成為資料發佈者。
關鍵字
Occurrence; eDNA; North Sea; trawl
聯絡資訊
- 出處
地理涵蓋範圍
Belgian part of the North Sea
界定座標範圍 | 緯度南界 經度西界 [-90, -180], 緯度北界 經度東界 [90, 180] |
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取樣方法
1.Sampling was carried out between September 26 and October 7, 2022 at the Belgium Part of the North Sea (BPNS) with the research vessel Belgica. Water samples were collected approximately 1 m above the seafloor at 17 locations covering the distribution of the three distinct fish communities (coastal, transition and offshore) (Figure 1). At twelve locations, water was sampled both at the surface and bottom to study the vertical distribution pattern of eDNA. A rosette equipped with 10 L Niskin bottles was deployed to collect the water samples: bottom samples were taken 1 meter above the seabed and surface samples 1 meter below the sea surface. Prior to deployment, the rosette was held below the surface for three minutes to allow the Niskin bottles and the CTD to equilibrate with the surrounding water mass. To minimize the potential disturbance of eDNA caused by the downward movement of the rosette, the surface samples were collected before the bottom samples. Five biological replicates were collected at each location and depth, with each replicate corresponding to a single Niskin bottle. From each Niskin bottle, 2 L seawater was pre-filtered through a 200 µm sterilized nylon mesh to remove bigger particles and organisms that can potentially cause clogging during the subsequent filtering process. Filtering of the samples was conducted onboard in a dedicated lab for eDNA analyses, right after the sample collection. The samples were filtered through a 0.45 µm Sterivex-HV filter (Millipore SterivexTM, PVDF, with Luer outlet) using a peristaltic pump (Masterflex L/S® Variable Speed Pump HV-77910-75) until the filter was close to clogging. 2. Quality control Negative control samples were collected in the field and laboratory environments. Negative field controls were taken by collecting commercial source water from the Niskin bottles after they were carefully rinsed using commercial source water, also using the prefilter. Negative filter controls were included by filtering source water over a blanco 0.45 µm Sterivex filter. Negative extraction controls were included by applying the extraction protocol on blanco 0.45 µM Sterivex filters. Negative PCR controls were included by replace the extracted eDNA with 3 µl of UltraPure™ water.
研究範圍 | The integration of eDNA metabarcoding into monitoring programs provides valuable information about fish community structures. Despite the growing body of evidence supporting the method's effectiveness in distinguishing fine-scale eDNA signals, there is a limited understanding of eDNA distribution in shallow, well-mixed environments, especially related to sampling depth. We analyzed 167 samples collected from the surface and bottom water at 17 locations of the Belgian Part of the North Sea (BPNS) and compared this to beam trawl catch data collected simultaneously at the same locations. |
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方法步驟描述:
- 1. eDNA extraction and Library preparation. After overnight incubation with the lysisbuffer at 56°C, the eDNA was extracted using the DNeasy Blood and Tissue kit (Qiagen). Library preparation The genetic analysis was based on 12S. A one-step amplification protocol was used in triplicate using fusion primers (Sigma Aldrich), which contained the template specific primer sequence and a unique barcode tag of 6 to 10 nucleotides. After amplification, the PCR replicates were pooled and purified using magnetic CleanNGS beads (CleanNA). After purification, the three 12S libraries were quality checked on the BioAnalyzer. The eDNA libraries were sequenced with Illumina MiSeq, 2 x 300 bp. 2. Bioinformatic processing The quality of the raw Illumina MiSeq sequencing reads was verified with FASTQC v0.11.9. The paired-end reads were then reorientated, demultiplexed and trimmed by using cutadapt. After demultiplexing, DADA2 was used for denoising, dereplication, merging, and removing of chimeric reads from the demultiplexed sequences. The taxonomic assignment of the resulting ASV sequences was performed against a custom made reference database using RDP classifier in DADA2 with a minimum bootstrapping support of 80. ASVs that remained unassigned at species level with RDP were successively run with BLASTn v2.12.0 against the custom made reference databases and the GenBank nucleotide database (from march 2023). After taxonomic assignment, the count table was cleaned by using MicroDecon using the field, filter, DNA extraction and PCR negative control samples.
額外的詮釋資料
替代的識別碼 | 8afcc57c-5d2b-4349-add6-29bfc33ed5cb |
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https://ipt.inbo.be/resource?r=ilvo-metabarcoding-1 |