The SIOS Data Management Service (SDMS) integrates information from SIOS partner data repositories into a unified virtual data centre, the SIOS Data Access Portal, allowing users to search for and access data regardless of where they are archived. Providers and users have to commit to the SIOS data policy.
The current focus is on dataset discovery through standardised metadata, and retrieval, visualisation & transformation of data. Ultimately, the Data Management Service works towards integration of datasets which requires a high level of interoperability at the data level.
SDMS currently harvests information on SIOS relevant datasets from a number of data centres (see below), some hosted by SIOS partners and some not. Data centres hosted by SIOS partners work to harmonise access to the data allowing integrated visualisation etc for the relevant datasets.
Data centres SDMS is harvesting information from.
SIOS partner data centres
Other
AWI (DE)
British Antarctic Survey
CNR (IT) - temporarily disabled due to server issues
National Snow and Ice Data Center
IGPAS (PL)
IMR (NO)
IOPAN (PL)
MET (NO) - weather stations have not been updated for a while, update in progress
NERSC (NO)
NILU (NO)
NIPR (JP)
NPI (NO)
UiS (PL)
Citation of data and service
If you use data retrieved through this portal, please acknowledge our funding source: Research Council of Norway, project number 291644, Svalbard Integrated Arctic Earth Observing System – Knowledge Centre, operational phase.
Always remember to cite data when used!
Citation information for individual datasets is often provided in the metadata. However, not all datasets have this information embedded in the discovery metadata. On a general basis a citation of a dataset include the same components as any other citation:
author,
title,
year of publication,
publisher (for data this is often the archive where it is housed),
edition or version,
access information (a URL or persistent identifier, e.g. DOI if provided)
SIOS recommends all partner data repositories to mint Digital Object Identifiers (DOI) on all datasets. The information required to properly cite a dataset is normally provided in the discovery metadata the datasets.
SIOS Core Data
In order to find SIOS Core Data please use the searchable item marked "Collection" on the right hand side of the map and select "SIOSCD". Quick access to SIOS Core Data is provided here.
Nansen Legacy Data
The Nansen Legacy project is using the SIOS Data Management system as the data portal. Quick access to all Nansen Legacy related datasets is available here.
Brief user guide
The Data Access Portal has information in 3 columns. An outline of the content in these columns is provided above. When first entering the search interface, all potential datasets are listed. Datasets are indicated in the map and results tabulation elements which are located in the middle column. The order of results can be modified using the "Sort by" option in the left column. On top of this column is normally relevant guidance information to user presented as collapsible elements.
If the user want to refine the search, this can be done by constraining the bounding box search. This is done in the map - the listing of datasets is automatically updated. Date constraints can be added in the left column. For these to take effect, the user has to push the button marked search. In the left column it is also possible to specific text elements to search for in the datasets. Again pushing the button marked "Search" is necessary for these to take action. Complex search patterns can be constructed using logical operators from the drop down above the text field and prefixing words with '+' to require their presence and '-' to require their non presence.
Other elements indicated in the left and right columns are facet searches, i.e. these are keywords that are found in the datasets and all datasets that contain these specific keywords in the appropriate metadata elements are listed together. Further refinement can be done using full text, date or bounding box constraints. Individuals, organisations and data centres involved in generating or curating the datasets are listed in the facets in the right column.
The data has been collected during the Nansen Legacy Seasonal Study Q1 from 2 - 25 March 2021 on research vessel RV Kronprins Haakon (cruise number 2021703), along a transect in the northern Barents Sea from 76N to 82N. The dataset contains abundance of pelagic marine protists, including phytoplankton (autotrophic) and protozooplankton (heterotrophic). Protists were identified and counted with light microscopy using the Utermöhl method and the result are given as cells per liter (cells/L) called organismQuantity.
Quality
Sampling method:
The samples were collected with Niskin bottles attached to a CTD rosette at the following depths: 5, 10, 30, 60, 90 m and deep chlorophyll max (DCM). The samples were preserved using an aldehyde mixture of glutaraldehyde and hexamethylenetetramine-buffered formalin at final concentrations of 0.1% and 1% respectively.
Analyse method:
All samples have been analysed at Institute of Oceanology of the Polish Academy of Sciences (IOPAN). The organisms were identified and counted under an inverted microscope according to the Utermöhl method.
Header name index - events
- expedition: cruise number for R/V Kronprins Haakon
- eventID: UUID for the sample
- parentID: UUID for the gear deployment (each Niskin has a unique parentID)
- eventDate: the date-time when an event occurred, using ISO 8601-1:2019 format (2020-07-27T07:16:03.446Z).
- fieldNumber: human-readable sample ID (e.g. PHT-001)
- locationID: station name
- decimalLongitude: geographic latitude (in decimal degrees, using the spatial reference system given in geodetic datum)
- decimalLatitude: geographic longitude (in decimal degrees, using the spatial reference system given in geodeticDatum)
- bottomDepthInMeters: bottom depth in meters
- eventRemarks: comments or remarks about the event (free text field)
- gearType: the gear used to take the sample e.g. Niskin bottle
- samplingDepthInMeters: depth sampled
- sampleType: description of the sample type according to a standard list
- recordedBy: name of the person who took the samples
- principalInvestigatorName: name of the person in charge of the sample collection
- principalInvestigatorEmail: email address of the person in charge of the sample collection
- principalInvestigatorInstitution: affiliated institution of the person in charge of the sample collection
Header name index - occurrence
- scientificName: full scientific name of the identified organism at the lowest taxonomic level that can be ascertained. The scientificName should be selected from a drop-down menu linked to the list in taxonomy sheet. (e.g Thalassiosira hyalina).
- identificationQualifier: A standard term (sp., spp., and indet.) to express uncertainty in identification.
- lifeStage: the life stage (e.g. resting spore) of the organism.
- sizeGroupOperator: describes if the size group is less than or greater than a value (It = less than, gte = greater or equal to)
- sizeGroup: the size group in µm.
- organismRemark: indicates e.g. varieties, colony type
- identificationRemarks: a free text field for adding information relevant to the analysis
- identifiedBy: person who did the lab-analyse
- fieldsInCount: Number of fields counted in the microscope
- magnificationMicroscope: The magnification setting used during analysis. Selected from a drop-down menu linked to vocab-sheet
- maxFields: Number of fields in the entire sedimentation chamber (Related to magnification used)
- takenVolumeML: The volume taken for sedimentation in the Utermöhl chamber (the sub-sample taken for analysis)
- identifiedBy: Drop-down menu linked to list in people-sheet
- dateIdentified: Date for the analysis
- sampleSizeValue=(fieldsInCount/maxFields)*(takenVolumeML/convertionMLtoL)*dilutionFactorFormaldehyde), dilutionFactorFormaldehyde = 0.95
- sampleSizeUnit: liter (l)
- organismQuantity: the quantity of the organism per volume water in the environment (organismQuantity = individualCount/sampleSizeValue)
- organismQuantityType: cells/l
Funding:
The Nansen Legacy is funded by the Research Council of Norway and the Norwegian Ministry of Education and Research. They provide 50% of the budget while the participating institutions contribute 50% in-kind. The total budget for the Nansen Legacy project is 740 mill. NOK.
The data has been collected during the Nansen Legacy Seasonal Study Q2 from 27 April - 20 May 2021 on research vessel Kronprins Haakon (cruise number 2021704), along a transect in the northern Barents Sea from 76N to 82N. The dataset contains abundance of pelagic marine protists, including phytoplankton (autotrophic) and protozooplankton (heterotrophic). Protists were identified and counted with light microscopy using the Utermöhl method and the result are given as cells per liter (cells/L) called organismQuantity.
Quality
Sampling method:
The samples were collected with Niskin bottles attached to a CTD rosette at the following depths: 5, 10, 30, 60, 90 m and deep chlorophyll max (DCM). The samples were preserved using an aldehyde mixture of glutaraldehyde and hexamethylenetetramine-buffered formalin at final concentrations of 0.1% and 1% respectively.
Analyse method:
All samples have been analysed at Institute of Oceanology of the Polish Academy of Sciences (IOPAN). The organisms were identified and counted under an inverted microscope according to the Utermöhl method.
Header name index - events
- expedition: cruise number for R/V Kronprins Haakon
- eventID: UUID for the sample
- parentID: UUID for the gear deployment (each Niskin has a unique parentID)
- eventDate: the date-time when an event occurred, using ISO 8601-1:2019 format (2020-07-27T07:16:03.446Z).
- fieldNumber: human-readable sample ID (e.g. PHT-001)
- locationID: station name
- decimalLongitude: geographic latitude (in decimal degrees, using the spatial reference system given in geodetic datum)
- decimalLatitude: geographic longitude (in decimal degrees, using the spatial reference system given in geodeticDatum)
- bottomDepthInMeters: bottom depth in meters
- eventRemarks: comments or remarks about the event (free text field)
- gearType: the gear used to take the sample e.g. Niskin bottle
- samplingDepthInMeters: depth sampled
- sampleType: description of the sample type according to a standard list
- recordedBy: name of the person who took the samples
- principalInvestigatorName: name of the person in charge of the sample collection
- principalInvestigatorEmail: email address of the person in charge of the sample collection
- principalInvestigatorInstitution: affiliated institution of the person in charge of the sample collection
Header name index - occurrence
- scientificName: full scientific name of the identified organism at the lowest taxonomic level that can be ascertained. The scientificName should be selected from a drop-down menu linked to the list in taxonomy sheet. (e.g Thalassiosira hyalina).
- identificationQualifier: A standard term (sp., spp., and indet.) to express uncertainty in identification.
- lifeStage: the life stage (e.g. resting spore) of the organism.
- sizeGroupOperator: describes if the size group is less than or greater than a value (It = less than, gte = greater or equal to)
- sizeGroup: the size group in µm.
- organismRemark: indicates e.g. varieties, colony type
- identificationRemarks: a free text field for adding information relevant to the analysis
- identifiedBy: person who did the lab-analyse
- fieldsInCount: Number of fields counted in the microscope
- magnificationMicroscope: The magnification setting used during analysis. Selected from a drop-down menu linked to vocab-sheet
- maxFields: Number of fields in the entire sedimentation chamber (Related to magnification used)
- takenVolumeML: The volume taken for sedimentation in the Utermöhl chamber (the sub-sample taken for analysis)
- identifiedBy: Drop-down menu linked to list in people-sheet
- dateIdentified: Date for the analysis
- sampleSizeValue=(fieldsInCount/maxFields)*(takenVolumeML/convertionMLtoL)*dilutionFactorFormaldehyde), dilutionFactorFormaldehyde = 0.95
- sampleSizeUnit: liter (l)
- organismQuantity: the quantity of the organism per volume water in the environment (organismQuantity = individualCount/sampleSizeValue)
- organismQuantityType: cells/l
Funding:
The Nansen Legacy is funded by the Research Council of Norway and the Norwegian Ministry of Education and Research. They provide 50% of the budget while the participating institutions contribute 50% in-kind. The total budget for the Nansen Legacy project is 740 mill. NOK.
M2 acoustic presence of marine mammals and anthropogenic noise manually counted for the period 2019-2020
Quality
Daily acoustic presence of the different sound sources (marine mammals, vessels and airguns) manually identified (except blue and fin whale, automatically detected using spectrogram correlation in Ishmael) during the manual inspection of spectrograms from each acoustic file (one file per hour) for the available data period 2019/2020 in M2, Svalbard. The M2 AURAL recorder sampled 12 min each hour during the given data period.
Variables: dt: date Month: Categorical variable with the name of the month Week: number of week since beginning of the study period Bowhead: acoustic presence of Balaena mysticetus Bowsong: acoustic presence of Balaena mysticetus songs Narwhal: acoustic presence of Monodon monoceros Narwhistle: acoustic presence of Monodon monoceros tonal sounds Walrus: acoustic presence of Odobenus rosmarus Bearded: acoustic presence of Erignathus barbatus Vessel: acoustic presence of vessel noise Odontocete: acoustic presence of odontocete-like whistle and tonal sounds non idetinfied to spp. level Airgun: acoustic presence of airgun blasts Harp: acoustic presence of Pagophilus groenlandicus Humpback: acoustic presence of Megaptera novaeangliae Blue: acoustic presence of Balaenoptera musculus Fin: acoustic presence of Balaenoptera physalus
The data set contains daily sea ice concentrations for each of the 42 Nansen Legacy stations for the period 2017-2021 derived from AMSR-2 and AMSR-E sea ice concentrations products. The data set is complemented with local sea ice concentration from visual bridge-based observations of the state of sea ice pack conducted following ASSIST Ice Watch protocol during some of the Nansen Legacy cruises to the study area.
This is a contribution to the Research Council of Norway project “Nansen Legacy” (https://arvenetternansen.com/), WP RF-1 “Physical drivers”.
Quality
For details on the data product see the attached file NL_stations_ice_concentration_2017-2021_metadata.pdf
Root Mean Squared (RMS) Sound Pressure Levels (SPL) were calculated for the one-Third Octave Level (TOL) bands centered at 63 Hz, 125 Hz and 250 Hz; and for the broadband 50-1000 Hz using PAMGuide package (Merchant et al. 2015) and custom-made MATLAB code. One RMS SPL value per file was obtained, averaging 12 min of recording in M2.
Variables: time: datetime TOL63HZ: Sound Pressure Level for the third-octave level band centered at 63 Hz TOL125HZ: Sound Pressure Level for the third-octave level band centered at 125 Hz TOL250HZ: Sound Pressure Level for the third-octave level band centered at 250 Hz BB501000: Sound Pressure Level for the broadband 50-1000 Hz
Sea ice-associated and pelagic highly branched isoprenoids (HBIs) and sterols in pelagic zooplankton (Calanus glacialis, Calanus hyperboreus, Calanus finmarchicus, Themisto libellula, Themisto abyssorum) collected during Nansen Legacy cruise Q4
Quality
Extraction of total lipids with chloroform/methanol, saponification with potassium hydroxide in water/methanol, purification via open column chromatography Analysis via gas chromatography-mass spectrometry
The data has been collected during the Nansen Legacy Seasonal Study Q3 from 5 - 27 August 2019 on research vessel RV Kronprins Haakon (cruise number 2019706), along a transect in the northern Barents Sea from 76N to 82N. The dataset contains abundance of ice algae marine protists, including ice algae (autotrophic) and protozoa (heterotrophic). Protists were identified and counted with light microscopy using the Utermöhl method and the result are given as cells per liter (cells/L) called organismQuantity
Quality
Sampling method:
The samples were collected with Kovacs ice corer 9 cm diameter (Kovacs Enterprise). The samples were collected from the bottom part of the ice core at the following dept layers: 0-3 cm, 3-10 cm, 10-20 cm & 20-30 cm. The ice cores were transferred to a clean bucket and 100mL filtered sea water were added per 1 cm of sea ice and melted at 4°C. When the ice core was melted, 95 mL of the sample was transferred into 100 ml brown glass bottle. The samples were preserved using an aldehyde mixture of glutaraldehyde and hexamethylenetetramine-buffered formalin at final concentrations of 0.1% and 1% respectively.
Analyse method:
All samples have been analysed at Institute of Oceanology of the Polish Academy of Sciences (IOPAN). The organisms were identified and counted under an inverted microscope according to the Utermöhl method.
Header name index - events
- expedition: cruise number for R/V Kronprins Haakon
- eventID: UUID for the sample
- parentID: UUID for the gear deployment (each ice core has a unique parentID)
- eventDate: the date-time when an event occurred, using ISO 8601-1:2019 format (2020-07-27T07:16:03.446Z).
- fieldNumber: human-readable sample ID (e.g. IAT-001)
- locationID: station name
- decimalLongitude: geographic latitude (in decimal degrees, using the spatial reference system given in geodetic datum)
- decimalLatitude: geographic longitude (in decimal degrees, using the spatial reference system given in geodeticDatum)
- maximumDepthInCentimeters: bottom depth of the core section in cm
- minimumDepthInCentimeters: upper depth of the core section in cm
- eventRemarks: comments or remarks about the event (free text field)
- gearType: the gear used to take the sample e.g. Ice corer 9 cm
- samplingDepthInMeters: depth sampled
- sampleType: description of the sample type according to a standard list
- recordedBy: name of the person who took the samples
- principalInvestigatorName: name of the person in charge of the sample collection
- principalInvestigatorEmail: email address of the person in charge of the sample collection
- principalInvestigatorInstitution: affiliated institution of the person in charge of the sample collection
Header name index - occurrence
- scientificName: full scientific name of the identified organism at the lowest taxonomic level that can be ascertained. The scientificName should be selected from a drop-down menu linked to the list in taxonomy sheet. (e.g Nitzschia frigida).
- identificationQualifier: A standard term (sp., spp., and indet.) to express the determiner’s doubts about the Identification.
- lifeStage: the life stage (e.g. resting spore) of the organism
- sizeGroupOperator: describes if the size group is less than or greater than a value (It = less than, gte = greater or equal to)
- sizeGroup: the size group in µm.
- organismRemark: indicates e.g. varieties, colony type
- identificationRemarks: a free text field for adding information relevant to the analysis
- identifiedBy: person who did the lab-analyse
- identifiedBy: Drop-down menu linked to list in people-sheet
- dateIdentified: Date for the analysis
- fieldsInCount: Number of fields counted in the microscope
- magnificationMicroscope: The magnification setting used during analysis. Selected from a drop-down menu linked to vocab-sheet
- maxFields: Number of fields in the entire sedimentation chamber (Related to magnification used)
- takenVolumeML: The volume taken for sedimentation in the Utermöhl chamber (the sub-sample taken for analysis)
- totalMeltedVolumeL: The total melted volume in L recorded during sampling.
- addedFSWvolumeL: Volume in L of filtered sea water added to the sample during melting.
- initialVolumeL: The total volume in L of the melted core, measured during sampling. If it wasn’t measured one can use the theoretical calculated core volume based on diameter of the core. initialVolumeL=(totalMeltedVolumeL-addedFSWvolumeL)) or teoreticalCoreVolumeL = coreAreM*(maxDepthCM-minDepthCM)
- sampleSizeValue=((fieldsInCount/maxFields)(takenVolumeML/conversionMLtoL))(dilutionFactorFormaldehyde*dilutionFactorFSW)), dilutionFactorFormaldehyde = 0.95, dilutionFactorFSW=
- sampleSizeUnit: liter (l)
- organismQuantity: the quantity of the organism per volume water in the environment (organismQuantity = individualCount/sampleSizeValue)
- organismQuantityType: cells/l
- cellsPerM2: The quantity (number of cells) of the organism per area (m2). cellsPerM2 = ((individualCount/(sampleSizeValue/initialVolumeL))/coreAreaM
Funding:
The Nansen Legacy is funded by the Research Council of Norway and the Norwegian Ministry of Education and Research. They provide 50% of the budget while the participating institutions contribute 50% in-kind. The total budget for the Nansen Legacy project is 740 mill. NOK.
The dataset includes spectral absorption coefficients of colored dissolved organic matter (CDOM), ’particulate matter and non-algal particles in seawater. Samples were collected in May 2021 as part of cruise 2021704, Q2, in the northern Barents Sea as part of the Nansen Legacy project. Sea water was sampled using Niskin bottles attached to a rosette onboard R/V Kronprins Haakon. CDOM samples were filtered through a 0.22 μm cartridge filter, and measured on a 1 m liquid waveguide capillary cell (LWCC). Particulate absorption measured on 0.7 μm pore size GFF filters (25 mm diameter, nominally 1 liter filtered volume), and measured on a Lambda 950 UV-Vis-NIR spectrophotometer and QFT-ICAM absorption meter. Non-algal particle absorption is measured after bleaching the filters using H2O2.
The data has been collected during the Nansen Legacy Seasonal Study Q4 from 28 November - 17 December 2019 on research vessel RV Kronprins Haakon (cruise number 201971), along a transect in the northern Barents Sea from 76N to 82N. The dataset contains abundance of ice algae marine protists, including ice algae (autotrophic) and protozoa (heterotrophic). Protists were identified and counted with light microscopy using the Utermöhl method and the result are given as cells per liter (cells/L) called organismQuantity.
Quality
Sampling method:
The samples were collected with Kovacs ice corer 9 cm diameter (Kovacs Enterprise). The samples were collected from the bottom part of the ice core at the following dept layers: 0-3 cm, 3-10 cm, 10-20 cm & 20-30 cm. The ice cores were transferred to a clean bucket and 100mL filtered sea water were added per 1 cm of sea ice and melted at 4°C. When the ice core was melted, 95 mL of the sample was transferred into 100 ml brown glass bottle. The samples were preserved using an aldehyde mixture of glutaraldehyde and hexamethylenetetramine-buffered formalin at final concentrations of 0.1% and 1% respectively.
Analyse method:
All samples have been analysed at Institute of Oceanology of the Polish Academy of Sciences (IOPAN). The organisms were identified and counted under an inverted microscope according to the Utermöhl method.
Header name index - events
- expedition: cruise number for R/V Kronprins Haakon
- eventID: UUID for the sample
- parentID: UUID for the gear deployment (each ice core has a unique parentID)
- eventDate: the date-time when an event occurred, using ISO 8601-1:2019 format (2020-07-27T07:16:03.446Z).
- fieldNumber: human-readable sample ID (e.g. IAT-001)
- locationID: station name
- decimalLongitude: geographic latitude (in decimal degrees, using the spatial reference system given in geodetic datum)
- decimalLatitude: geographic longitude (in decimal degrees, using the spatial reference system given in geodeticDatum)
- maximumDepthInCentimeters: bottom depth of the core section in cm
- minimumDepthInCentimeters: upper depth of the core section in cm
- eventRemarks: comments or remarks about the event (free text field)
- gearType: the gear used to take the sample e.g. Ice corer 9 cm
- samplingDepthInMeters: depth sampled
- sampleType: description of the sample type according to a standard list
- recordedBy: name of the person who took the samples
- principalInvestigatorName: name of the person in charge of the sample collection
- principalInvestigatorEmail: email address of the person in charge of the sample collection
- principalInvestigatorInstitution: affiliated institution of the person in charge of the sample collection
Header name index - occurrence
- scientificName: full scientific name of the identified organism at the lowest taxonomic level that can be ascertained. The scientificName should be selected from a drop-down menu linked to the list in taxonomy sheet. (e.g Nitzschia frigida).
- identificationQualifier: A standard term (sp., spp., and indet.) to express the determiner’s doubts about the Identification.
- lifeStage: the life stage (e.g. resting spore) of the organism
- sizeGroupOperator: describes if the size group is less than or greater than a value (It = less than, gte = greater or equal to)
- sizeGroup: the size group in µm.
- organismRemark: indicates e.g. varieties, colony type
- identificationRemarks: a free text field for adding information relevant to the analysis
- identifiedBy: person who did the lab-analyse
- identifiedBy: Drop-down menu linked to list in people-sheet
- dateIdentified: Date for the analysis
- fieldsInCount: Number of fields counted in the microscope
- magnificationMicroscope: The magnification setting used during analysis. Selected from a drop-down menu linked to vocab-sheet
- maxFields: Number of fields in the entire sedimentation chamber (Related to magnification used)
- takenVolumeML: The volume taken for sedimentation in the Utermöhl chamber (the sub-sample taken for analysis)
- totalMeltedVolumeL: The total melted volume in L recorded during sampling.
- addedFSWvolumeL: Volume in L of filtered sea water added to the sample during melting.
- initialVolumeL: The total volume in L of the melted core, measured during sampling. If it wasn’t measured one can use the theoretical calculated core volume based on diameter of the core. initialVolumeL=(totalMeltedVolumeL-addedFSWvolumeL)) or teoreticalCoreVolumeL = coreAreM*(maxDepthCM-minDepthCM)
- sampleSizeValue=((fieldsInCount/maxFields)(takenVolumeML/conversionMLtoL))(dilutionFactorFormaldehyde*dilutionFactorFSW)), dilutionFactorFormaldehyde = 0.95, dilutionFactorFSW=
- sampleSizeUnit: liter (l)
- organismQuantity: the quantity of the organism per volume water in the environment (organismQuantity = individualCount/sampleSizeValue)
- organismQuantityType: cells/l
- cellsPerM2: The quantity (number of cells) of the organism per area (m2). cellsPerM2 = ((individualCount/(sampleSizeValue/initialVolumeL))/coreAreaM
Funding:
The Nansen Legacy is funded by the Research Council of Norway and the Norwegian Ministry of Education and Research. They provide 50% of the budget while the participating institutions contribute 50% in-kind. The total budget for the Nansen Legacy project is 740 mill. NOK.
Fatty acid-specific stable isotopes of the fatty acids 16:1(n-7), 20:5(n-3) and 22:6(n-3) in pelagic particulate organic matter (PPOM), ice-associated particulate organic matter (IPOM) and pelagic zooplankton species (copepods, krill, amphipods, chaetognaths, appendicularians) collected from the Barents Sea during Nansen Legacy seasonal cruise Q3 in August 2019
The data has been collected during the Nansen Legacy Seasonal Study Q4 from 28 November - 17 December 2019 on research vessel RV Kronprins Haakon (cruise number 201971), along a transect in the northern Barents Sea from 76N to 82N. The dataset contains abundance of pelagic marine protists, including phytoplankton (autotrophic) and protozooplankton (heterotrophic). Protists were identified and counted with light microscopy using the Utermöhl method and the result are given as cells per liter (cells/L) called organismQuantity.
Quality
Sampling method:
The samples were collected with Niskin bottles attached to a CTD rosette at the following depths: 5, 10, 30, 60, 90 m and deep chlorophyll max (DCM). The samples were preserved using an aldehyde mixture of glutaraldehyde and hexamethylenetetramine-buffered formalin at final concentrations of 0.1% and 1% respectively.
Analyse method:
All samples have been analysed at Institute of Oceanology of the Polish Academy of Sciences (IOPAN). The organisms were identified and counted under an inverted microscope according to the Utermöhl method.
Header name index - events
- expedition: cruise number for R/V Kronprins Haakon
- eventID: UUID for the sample
- parentID: UUID for the gear deployment (each Niskin has a unique parentID)
- eventDate: the date-time when an event occurred, using ISO 8601-1:2019 format (2020-07-27T07:16:03.446Z).
- fieldNumber: human-readable sample ID (e.g. PHT-001)
- locationID: station name
- decimalLongitude: geographic latitude (in decimal degrees, using the spatial reference system given in geodetic datum)
- decimalLatitude: geographic longitude (in decimal degrees, using the spatial reference system given in geodeticDatum)
- bottomDepthInMeters: bottom depth in meters
- eventRemarks: comments or remarks about the event (free text field)
- gearType: the gear used to take the sample e.g. Niskin bottle
- samplingDepthInMeters: depth sampled
- sampleType: description of the sample type according to a standard list
- recordedBy: name of the person who took the samples
- principalInvestigatorName: name of the person in charge of the sample collection
- principalInvestigatorEmail: email address of the person in charge of the sample collection
- principalInvestigatorInstitution: affiliated institution of the person in charge of the sample collection
Header name index - occurrence
- scientificName: full scientific name of the identified organism at the lowest taxonomic level that can be ascertained. The scientificName should be selected from a drop-down menu linked to the list in taxonomy sheet. (e.g Thalassiosira hyalina).
- identificationQualifier: A standard term (sp., spp., and indet.) to express uncertainty in identification.
- lifeStage: the life stage (e.g. resting spore) of the organism.
- sizeGroupOperator: describes if the size group is less than or greater than a value (It = less than, gte = greater or equal to)
- sizeGroup: the size group in µm.
- organismRemark: indicates e.g. varieties, colony type
- identificationRemarks: a free text field for adding information relevant to the analysis
- identifiedBy: person who did the lab-analyse
- fieldsInCount: Number of fields counted in the microscope
- magnificationMicroscope: The magnification setting used during analysis. Selected from a drop-down menu linked to vocab-sheet
- maxFields: Number of fields in the entire sedimentation chamber (Related to magnification used)
- takenVolumeML: The volume taken for sedimentation in the Utermöhl chamber (the sub-sample taken for analysis)
- identifiedBy: Drop-down menu linked to list in people-sheet
- dateIdentified: Date for the analysis
- sampleSizeValue=(fieldsInCount/maxFields)*(takenVolumeML/convertionMLtoL)*dilutionFactorFormaldehyde), dilutionFactorFormaldehyde = 0.95
- sampleSizeUnit: liter (l)
- organismQuantity: the quantity of the organism per volume water in the environment (organismQuantity = individualCount/sampleSizeValue)
- organismQuantityType: cells/l
Funding:
The Nansen Legacy is funded by the Research Council of Norway and the Norwegian Ministry of Education and Research. They provide 50% of the budget while the participating institutions contribute 50% in-kind. The total budget for the Nansen Legacy project is 740 mill. NOK.
Time-series data from moorings covering the Svalbard Branch of the Atlantic Water inflow over the upper continental slope north of Svalbard, Sep 2015 to Sep 2017. The data comprise temperature, salinity and other parameters from CTDs, and water currents from ADCPs.
Data are published as individual time-series files from the different instruments. Both raw and processed ADCP data are published.
Quality
Data processed with standard software from the instrument manufacturers plus additional quality controls to remove bad data points. Details of ADCP processing and quality control are described in the documentation PDF.
Dissolved inorganic nutrients (nitrate, phosphate and silicic acid) from the combined Nansen Legacy and A-TWAIN cruise Mooring service cruise 2021 (cruise 2021713).
The cruise 2021713 in November 2021 aboard the Research Vessel Kronprins Haakon is part of the projects A-TWAIN and the Nansen LEGACY. The A-TWAIN project is focusing on monitoring of the Atlantic Water boundary current north of Svalbard. The Nansen LEGACY is the Norwegian Arctic research community’s joint effort to establish a holistic understanding of a changing marine Arctic climate and ecosystem.
Water column temperature and salinity profiles were obtained with a conductivity-temperature-depth (CTD) sensor system Sea-Bird SBE 911+ mounted on a General Oceanics rosette sampler equipped with 24 Niskin bottles used for seawater sampling of chemical variables in the water column. Samples for the determination of dissolved inorganic nutrients were collected from full water column at a total of six stations starting from the shelf northern Barents Sea to the Nansen Basin along the moored A-TWAIN line. The seawater samples were collected from Niskin bottles in 20 ml plastic HDPE vials (rinsed three times) and preserved with 250 µL chloroform and stored +4C and dark until post-cruise analysis of nitrite (NO2), nitrate (NO3-), phosphate (PO43-), and silicate (Si(OH)4), using spectrophotometry according to standard protocols (Grasshoff et al., 2009; Gundersen et al., 2022) at the chemical laboratory at Institute of Marine Research, Bergen, Norway. Three replicates were analyzed for each sample. The detection limits based on QUASIMEME ring-test are 0.06 µmol/L, 0.5 µmol/L, 0.06 µmol/L and 0.7 µmol/L for NO2, NO3-, PO43-, and Si(OH)4, respectively. The sampling and sample analysis were supported by the Research Council of Norway through the projects The Nansen LEGACY (RCN #276730) and SIOS-InfraNor (RCN #269927).
The data set present the calculated sea ice back-trajectories of 30 sea ice stations conducted in the northern Barents Sea and in western Arctic Basin north of Svalbard between August 2018 to March 2022. The sea ice stations were made during eight research cruises to the area with R/V Kronprins Haakon in the framework of the Nansen Legacy project. For details on the back-tracking methodology and data structure please see the attached metadata file NansenLegacy_sea_ice_stations_back-trajectories.pdf