說明
This resource documents fish species occurrences detected from environmental DNA (eDNA) collected in the core habitat of the Rice's whale (Balaenoptera ricei) in the northeastern Gulf of America. Seawater samples were collected from depths of 120-320 meters in July 2019 on board the NOAA Ship Gordan Gunter, concurrent with trawl surveys. Fish biodiversity was characterized using 12S rRNA metabarcoding (MiFish and Riaz markers) to identify potential prey available to this critically endangered cetacean.
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 912 筆紀錄。
亦存在 2 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。:
Wilcox Talbot L, Silliman K, Applegate M, Aichinger Dias L, Garrison L, Paterson C, Thompson L, Vollmer N, Rosel P (2025). Potential prey of Rice's whales based on seawater eDNA 2019. Version 1.2. NOAA Oceanic and Atmospheric Research. Occurrence dataset. https://ipt-obis.gbif.us/resource?r=rices-diet-edna&v=1.2
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 NOAA Oceanic and Atmospheric Research。 To the extent possible under law, the publisher has waived all rights to these data and has dedicated them to the Public Domain (CC0 1.0). Users may copy, modify, distribute and use the work, including for commercial purposes, without restriction.
GBIF 註冊
此資源已向GBIF註冊,並指定以下之GBIF UUID: 2fb7a0b9-1160-435e-bca9-82733c4df877。 NOAA Oceanic and Atmospheric Research 發佈此資源,並經由GBIF-US同意向GBIF註冊成為資料發佈者。
關鍵字
eDNA; metabarcoding; marine biodiversity; environmental DNA; Occurrence
外部資料
此資源尚有其他格式可用
| NCBI BioProject | https://www.ncbi.nlm.nih.gov/bioproject/?term=PRJNA1322479 UTF-8 BioSample, SRA, fastq.gz |
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聯絡資訊
- 元數據提供者 ●
- 出處 ●
- 連絡人
- Research Geneticist
https://orcid.org/0000-0001-9824-879X
- 元數據提供者 ●
- 出處 ●
- 連絡人
- Assistant Research Professor
- 4301 Rickenbacker Cswy
- 出處
- 出處
- 出處
- 出處
- 出處
- 出處
- 出處
- 作者
地理涵蓋範圍
USA: Gulf of Mexico
| 界定座標範圍 | 緯度南界 經度西界 [28.312, -86.858], 緯度北界 經度東界 [29.586, -85.325] |
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分類群涵蓋範圍
Marine vertebrates identified through eDNA metabarcoding
| Kingdom | Animalia, Bacteria |
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| Phylum | Chordata |
| Class | Mammalia, Teleostei |
| Order | Acanthuriformes, Acropomatiformes, Anguilliformes, Argentiniformes, Ateleopodiformes, Aulopiformes, Beloniformes, Callionymiformes, Carangiformes, Cetartiodactyla, Clupeiformes, Eupercaria incertae sedis, Gadiformes, Gobiiformes, Lampriformes, Lophiiformes, Myctophiformes, Ophidiiformes, Perciformes, Pleuronectiformes, Polymixiiformes, Scombriformes, Stomiiformes, Syngnathiformes, Tetraodontiformes |
時間涵蓋範圍
| 起始日期 / 結束日期 | 2019-07-06 / 2019-07-31 |
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計畫資料
Understanding the foraging ecology of endangered marine mammals is crucial for their conservation yet remains challenging due to the inaccessibility of their feeding habitats. This study used environmental DNA (eDNA) metabarcoding with two complementary 12S rRNA markers (MiFish and Riaz) to characterize potential fish prey communities available to the critically endangered Rice's whale (Balaenoptera ricei) in its core habitat in the northeastern Gulf of America. Water samples (N = 21) collected during a July 2019 survey detected 99 unique fish species across 62 families. The combined metabarcoding approach revealed 74 fish species not recorded in concurrent trawl surveys, while 16 trawl-caught species went undetected by eDNA. Notably, eDNA yielded higher detection rates for several potential prey taxa previously identified through stable isotope analysis, suggesting key prey species may be more prevalent than previously documented. This study demonstrates the value of eDNA as a complementary tool for monitoring the prey community of this critically endangered cetacean.
| 計畫名稱 | Potential prey of Rice's whales based on seawater eDNA 2019 |
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| 經費來源 | This work was supported by the NOAA RESTORE Science Program, Trophic Dynamics of Gulf of Mexico Rice’s Whale Study, with award number NA16OAR4320199 to the Northern Gulf Institute from NOAA’s Office of Oceanic and Atmospheric Research (OAR) and National Marine Fisheries Service (NMFS), U.S. Department of Commerce. This research was carried out [in part] under the auspices of the Cooperative Institute for Marine and Atmospheric Studies (CIMAS), a Cooperative Institute of the University of Miami and the National Oceanic and Atmospheric Administration, cooperative agreement #NA20OAR4320472. |
| Project Award |
Trophic Dynamics of Gulf of Mexico Rice’s Whale Study https://ror.org/0042xzm63 National Oceanic and Atmospheric Administration RESTORE Science Program https://restoreactscienceprogram.noaa.gov/projects/rices-whales Northern Gulf Institute https://ror.org/018qsef31 National Oceanic and Atmospheric Administration RESTORE Science Program NA16OAR4320199 Cooperative Institute for Marine and Atmospheric Studies National Oceanic and Atmospheric Administration RESTORE Science Program NA20OAR4320472 |
參與計畫的人員:
取樣方法
During July 2019, a fish trawl (31.7 m footrope length, 0.6 cm sq codend mesh liner) was deployed from the NOAA Ship Gordon Gunter to collect potential Rice’s whale fish prey during daylight hours within Rice’s whale feeding areas in the northeastern Gulf of America (formerly known as the Gulf of Mexico). Trawl stations were selected by locating near-bottom aggregations of backscattering organisms (i.e., fishes) based on observations from a Simrad EK80 echosounder (transducer frequencies 18 kHz, 38 kHz and 120 kHz). Seawater samples (N = 21), collected between 120-320 m depth, were collected concurrently with the trawling using Niskin bottles (5 L total capacity) attached to a conductivity, temperature, and depth sensor (CTD) unit (Figure 1). Bottles were triggered to close via remote command at the desired sampling depth (Table S1). CTDs were deployed for seawater collection at one depth immediately after the trawl was retrieved at 18 stations, except for one trawl station where CTD sampling was repeated at two depths. Two additional CTD deployments collected seawater when no trawling was occurring while Rice’s whales were in the immediate vicinity and displaying feeding behavior. After each sample was collected, approximately 2 L of seawater was transferred from the Niskin bottle into a 2 L sterile Nalgene bottle (cleaned as described for the Niskin bottles prior to use) and placed into a cooler with ice until filtration. All samples were filtered within 35 minutes of collection. Filtration, cleaning, and sample storage followed that as described in (Wilcox Talbot et al., 2025), using a 47 mm diameter mixed cellulose ester (MCE) filter with a 0.45-µm pore size. Using sterile forceps, each MCE filter was placed in a 4 mL screw cap vial containing approximately 3 mL of sterile Longmire’s lysis buffer (Longmire et al., 1997). The preserved filters were stored at room temperature and in the dark until eDNA extraction.
| 研究範圍 | Within Rice’s whale feeding areas in the northeastern Gulf of America (also known as the Gulf of Mexico). |
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| 品質控管 | All Niskin bottles were sterilized before use by thoroughly rinsing several times with ~500 mL of 20% bleach for 10 minutes, followed by multiple rinses with tap water, and allowed to air dry. The outside of each bottle was wiped with a Clorox® Disinfecting Wipe and allowed to air dry. For negative field controls, Nalgene bottles were used to collect 2–2.8 L of ship’s water, and filtered using the same process as completed for a Niskin seawater sample. To avoid cross-contamination, all eDNA sampling preparation and processing were conducted isolated from trawling activities and specimens; i.e.; staff who processed the eDNA samples did not assist in sorting trawl specimens and vice-versa. In addition, eDNA processing was performed in locations on the ship where no tissue samples were handled. |
方法步驟描述:
- Sample Collection Method Seawater was collected using 5 L Niskin bottles attached to a conductivity, temperature, and depth (CTD) sensor unit. Bottles were triggered remotely at depths between 120 and 320 meters. Approximately 2 L of seawater from each Niskin bottle was transferred to a sterile 2 L Nalgene bottle, placed in a cooler with ice, and filtered within 35 minutes of collection
- Sample Processing Filtration was conducted using a 47 mm diameter mixed cellulose ester (MCE) filter with a 0.45-µm pore size. Using sterile forceps, each filter was placed in a 4 mL screw cap vial containing approximately 3 mL of sterile Longmire’s lysis buffer. Preserved filters were stored at room temperature in the dark until extraction.
- Molecular Methods - eDNA Extraction: eDNA was extracted from the filters using a phenol:chloroform (1:1) method, followed by DNA precipitation using 5M NaCl and ice-cold 100% ethanol . - Metabarcoding: The 12S rRNA gene was amplified using two different fish-specific primer sets: modified MiFish-U-F/R2 primers and the Riaz primers. - Sequencing: Library pools were sequenced on an Illumina MiSeq in a 2x250 bp paired-end format using a MiSeq v2 500 cycle reagent cartridge. - Bioinformatics: Raw reads were processed using cutadapt v4.4 and Tourmaline v1.1.1 (which implements QIIME2 and DADA2) to infer amplicon sequence variants (ASVs). - Taxonomic Assignment: Taxonomy was assigned using Naïve Bayes classifiers trained on custom 12S reference sequence databases for each marker. To support this, 12S rRNA gene sequences from 15 regional fish species collected in the trawls were generated for this study and added to the reference databases
額外的詮釋資料
| 致謝 | This work was supported by the NOAA RESTORE Science Program, Trophic Dynamics of Gulf of Mexico Rice’s Whale Study, with award number NA16OAR4320199 to the Northern Gulf Institute from NOAA’s Office of Oceanic and Atmospheric Research (OAR) and National Marine Fisheries Service (NMFS), U.S. Department of Commerce. This research was carried out [in part] under the auspices of the Cooperative Institute for Marine and Atmospheric Studies (CIMAS), a Cooperative Institute of the University of Miami and the National Oceanic and Atmospheric Administration, cooperative agreement #NA20OAR4320472. We thank the crew and scientific personnel onboard the NOAA Ship Gordon Gunter, in particular Michael Hendon, Kendall Falana, Taniya Wallace, and Warren Brown for their technical expertise in trawl operations. |
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| 目的 | The primary purpose of this dataset is to characterize the potential fish prey community available to the critically endangered Rice's whale (Balaenoptera ricei) within its core habitat in the northeastern Gulf of America. Understanding the foraging ecology of this species is a critical conservation priority, but it is exceptionally difficult to study using traditional methods. This dataset provides species occurrence data generated using a non-invasive environmental DNA (eDNA) metabarcoding approach to fill this knowledge gap. The data were generated by sequencing two 12S rRNA gene markers (MiFish and Riaz) from 21 deep-water (120–320 m) samples collected in July 2019. The dataset documents 99 unique fish species, providing a comprehensive baseline of fish biodiversity in the whale's deep-water feeding habitat. A key finding demonstrated by this data is the enhanced sensitivity of eDNA compared to concurrent physical trawl surveys. The eDNA dataset includes 74 fish species that were not captured by the trawls, indicating that the available prey community is more diverse than previously documented. Furthermore, this dataset shows higher detection rates for several fish taxa previously identified as potential Rice's whale prey through stable isotope analysis. This suggests these key prey items may be more prevalent in the habitat than was previously understood. |
| 替代的識別碼 | https://ipt-obis.gbif.us/resource?r=rices-diet-edna |