Abstract:
List of fish species identified and cross-referenced by an integrative taxonomy analysis. Specimens were identified to the lowest taxonomic level using morphological features. A sub-sample of small muscle tissue from each individual was taken for DNA extraction and amplification of two mitochondrial genes, cox1 and the non-coding control region (CR).
Special attention was given to larval and juvenile specimens. Samples were collected by fishery observers on board krill fishing vessels for the winter seasons between 2019 and 2024. Extra samples collected before 2019 were obtained from the biological archives at BAS including muscle and fin tissue as well as otolith samples spanning from 1988 through 2022. All samples were measured and photographed prior to be subsampled for DNA. Most samples were blast-freeze and stored at -20 degrees C or fixed in 90% ethanol. Tissue samples were stored in 90-95% ethanol and kept at -20 degrees C. Data resources from this project were used to developed enhanced identification guides for larval and adult fish species caught as bycatch within the Antarctic krill fishery.
This is a Darwin plus initiative awarded to Philip, R. Hollyman under round 10 funding scheme, project reference DPLUS166.
Keywords:
Antarctic Peninsula, Area 48, Fish, Krill bycatch, South Georgia
Romero Martinez, M., Hollyman, P., & Collins, M. (2025). Fish bycatch diversity within the Antarctic krill fishery, CCAMLR sub-areas 48.1 to 48.3, 2019-2024 (Version 1.0) [Data set]. NERC EDS UK Polar Data Centre. https://doi.org/10.5285/9c459656-5fe4-44f7-860f-da287111016c
| Access Constraints: | Data is under embargo until the publication of an associated paper. |
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| Use Constraints: | This data is governed by the NERC data policy (http://www.nerc.ac.uk/research/sites/data/policy/) and supplied under Open Government Licence v.3 (http://www.nationalarchives.gov.uk/doc/open-government-licence/version/3/). |
| Creation Date: | 2025-05-13 |
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| Dataset Progress: | Planned |
| Dataset Language: | English |
| ISO Topic Categories: |
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| Parameters: |
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| Personnel: | |
| Name | UK Polar Data Centre |
| Role(s) | Metadata Author |
| Organisation | British Antarctic Survey |
| Name | Maria Lorena Romero Martinez |
| Role(s) | Investigator, Technical Contact |
| Organisation | British Antarctic Survey |
| Name | Philip Hollyman |
| Role(s) | Investigator |
| Organisation | Bangor University |
| Name | Dr Martin A Collins |
| Role(s) | Investigator |
| Organisation | British Antarctic Survey |
| Parent Dataset: | N/A |
| Reference: | Collins M.A. and Xavier J. (2022). Field guide to the macro-plankton and nekton of the Scotia Sea. Efremenko, F.N. (1983). Atlas of Fish Larvae of the Southern Ocean. Cybium, 7, 1 - 74. Scott Polar Research Institute, Cambridge. Gon, O and Heemstra, P.C. (eds). (1990). Fishes of the Southern Ocean. J.L.B. Smith Institute of Ichthyology, Grahamstown, 462 pp. 12 pls. Romero Martínez, M.L., Hollyman, P.R., Reid, W.D.K., Goodall-Copestake, W.P., Moir Clark, J., Collins, M.A. (2023). Improving identification of fish bycatch in the Antarctic Krill fishery. CCAMLR, WG-FSA-2023/04. Romero Martínez, M.L., Reid, W.D.K., Collins, M.A., Goodall-Copestake, W.P., Moir Clark, J., Viney, B., Hollyman, P.R. (2024). CCAMLR, WG-FSA-2024/13. |
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| Lineage/Methodology: | Samples were collected by fishery observers as part of the 25kg per trawl collected for the reporting of fish bycatch with the Antarctic krill fishery. The spatial distribution for the collection of samples covered the three subareas of Area 48 delimited by CCAMLR, subarea 48.1 (Antarctic Peninsula), 48.2 (Southern Scotia Sea) and 48.3 (Northern Scotia Sea including South Georgia Island). To process the samples an integrative taxonomy approached taken, whereby each specimen was identified to the lowest taxonomic level following the morphological keys provided in Efremenko (1983) and Kellermann (1989) for larval fish, while for juvenile and adult fish the morphological keys in Gon and Heemstra (1990) and Collins and Xavier (2022) were used. Total and standard length were measured and a photographed from the left side of the fish was taken. Photographic material was produced by mounting a Nikon Z camera fitted with a macro lens on a Kaiser copy stand. Each specimen was subsampled for DNA by making a small incision on the right side of the fish above the lateral line to take a small piece of tissue (25mg) as well as a fin clip (whenever possible). Tissue samples were then stored in 90% ETOH at -20°C before the DNA extraction and PCR amplification of cox1 gen and control region with species-specific primers. DNA was extracted from 25mg of muscle tissue using two types of kit and following manufactures instructions. The extracted gDNA was resuspended in 50 to 70 micro l eluent and stored at -20 degrees °C before amplification of targeted genes by polymerase chain reaction (PCR). Species specific primers were designed for the PCR amplification of cox1 and control region (Romero Martínez et al., 2023 and 2024). PCR amplification was performer on a thermocycle, PCR reactions mix consisted of 3-5 ng of DNA template, 7.5 micro l of master mix, 0.3-0.5 micro M of each forward and reverse primer to make a 15 micro l reaction. The thermocycling profile was 2 min at 95°C inital denaturation followed by 38 cycles at 95°C for 20 s, 50°C for 30 s, 72°C for 1:30 min and a final extension at 72°C for 1 min for cox1 and inital denaturation at 95°C for 5 min, 38 cycles at 95°C for 20 s, 50-55°C for 30 s, 72°C for 2 min, and final extension at 72°C for 1 min for control region. Amplicons for cox1 were Sanger sequenced using sequencing primers that were attached to species-specific primers to serve as a priming site for Sanger sequencing. Forward (ACTGCCATCTTGGAGGAC) and reverse (CCCAGGATTATGGAACGG) nondegenerate adapter tails. Sequencing was performed by Eurofins Genomics UK (Wolverhampton, UK). Amplicons for control region were sequenced in-house using the Oxford Nanopore Technology (ONT) MinIon and the associated sequencing platform MinKnow v23.07.15. CR amplicons were used to prepare sequencing libraries with the ONT Native Barcoding Kit following the manufactures instructions. The default experimental set up was used for all sequencing runs. Basecalling and demultiplexing were performed in real time using the High accuracy (HAC) basecalling model and minimum read length set to 200 bp. The GenBank BioProject ID for the project is PRJNA1270765. |
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| Temporal Coverage: | |
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| Start Date | 2022-11-01 |
| End Date | 2024-10-31 |
| Spatial Coverage: | |
| Latitude | |
| Southernmost | -73.22 |
| Northernmost | -60 |
| Longitude | |
| Westernmost | -70 |
| Easternmost | -50 |
| Altitude | |
| Min Altitude | N/A |
| Max Altitude | N/A |
| Depth | |
| Min Depth | N/A |
| Max Depth | N/A |
| Latitude | |
| Southernmost | -57 |
| Northernmost | -50 |
| Longitude | |
| Westernmost | -50 |
| Easternmost | -30 |
| Altitude | |
| Min Altitude | N/A |
| Max Altitude | N/A |
| Depth | |
| Min Depth | N/A |
| Max Depth | N/A |
| Latitude | |
| Southernmost | -64 |
| Northernmost | -57 |
| Longitude | |
| Westernmost | -50 |
| Easternmost | -30 |
| Altitude | |
| Min Altitude | N/A |
| Max Altitude | N/A |
| Depth | |
| Min Depth | N/A |
| Max Depth | N/A |
| Location: | |
| Location | South Georgia Island |
| Detailed Location | N/A |
| Location | South Orkney Islands |
| Detailed Location | N/A |
| Location | South Shetland Islands |
| Detailed Location | N/A |
| Location | Antarctica |
| Detailed Location | Antarctic Peninsula |
| Data Collection: | Morphology laboratory Camera: Nikon Z camera (Model N1929) Macro lens (Nikkor Z mount MC 50mm f/2.8 or a Laowa 25mm f2.8 2.5-5x ultra). Kaiser copy stand (RS10) with a Copy Arm RTP- 100cm. Molecular laboratory DNA extraction kits: PureLink(TM) Genomic DNA Mini Kit (Invitrogen, Carlsbad, USA) and DNeasy(R) Blood and Tissue Kit (Qiagen Ltd., West Sussex, UK) Thermocycler: PCRmax Alpha Cycler version 2.41. (Antylia Scientific, AXT PTY LTD, Australia). PCR master mix: 2x MyTaq HS master mix and (Meridian Bioscience, Bioline Reagents Ltd, UK), ONT MinIon Mk1B (MIN-101B) ONT Native barcoding kit 96 V14 (SQK-NBD114.96) |
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| Data Storage: | 752 JPG files. Specimen images. The images are in sub-folders named after each of the samples available in the "Sample_metadata" .csv. 3 CSV files containing the following information: "Species_list", contains a summary of fish species that were identified by the amplification and sequencing of cox1 and control region (CR). "Sample_metadata", contains the metadata for individual sample identified to the species level by morphology and genetic identification with either cox1, control region or both mitochondrial regions. "Primers", contains the list of primers that were developed for the amplification of both mitochondrial regions. |
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