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OAS accession Detail for 0278152
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| accessions_id: | 0278152 | archive |
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| Title: | Element quotas of individual plankton cells collected during IRNBRU (MV1405) and June 2015 Line P cruises (NCEI Accession 0278152) |
| Abstract: | This dataset contains chemical and physical data collected on CCGS John P. Tully and R/V Melville during cruises 2015-009 and MV1405 in the North Pacific Ocean on 2021-02-24. These data include Carbon, Iron, Manganese, Silicon, and depth. The instruments used to collect these data include Pump, Trace Metal Bottle, and X-ray fluorescence analyzer. These data were collected by Benjamin Twining of Bigelow Laboratory for Ocean Sciences as part of the "Collaborative Research: Investigating the Ecological Importance of Iron Storage in Diatoms (Diatom Iron Storage)" project. The Biological and Chemical Oceanography Data Management Office (BCO-DMO) submitted these data to NCEI on 2021-05-18. The following is the text of the dataset description provided by BCO-DMO: Cellular trace elements from IRNBRU and Line P cruises Dataset Description: Acquisition Description: R/V Melville 1405 took place in the North Pacific Ocean along the California coast from 32°S to 43°N and extending from -117°E to -127°E. The Line P cruise on CCGS John P. Tully was in the North Pacific Ocean off the coast British Columbia from Vancouver (48°N, 123°W) to Ocean Station Papa (50°N, 145°W). Samples were collected with trace-metal clean bottles or trace-metal clean pump. A small aliquot of unfiltered seawater was collected following protocols described in Twining et al. (2015). Cellular metals were analyzed with the 2-ID-E microprobe beamline at the Advanced Photon Source, Argonne National Laboratory. Incident beam energy was 10 keV to enable the excitation of K α fluorescence for elements ranging in atomic number from Si (14) to Zn (30). Element quantification was performed by averaging the spectra from pixels representing the cells of interest. Spectra were also extracted from a background area close to each cell. The spectra were then fit with MAPS, a custom fitting software package (Vogt, 2003). Concentrations were calculated based on conversion factors obtained by running the thin-film standards NBS 1832, NBS 1833, and custom Si, P, and Fe standards made by Micromatter XRF. Cell volume was calculated based on measurements taken from bright field images of the cells and using the equations of Hillebrand et al. (1999). Cellular C was then calculated from the volumes using the equations described in Menden-Deuer and Lessard (2000). Complete methodology is published in Twining et al. (2020). |
| Date received: | 20210518 |
| Start date: | 20210224 |
| End date: | 20210224 |
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| West boundary: | -145 |
| East boundary: | -123.66 |
| North boundary: | 50 |
| South boundary: | 38.66 |
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| Submitting institution: | Biological and Chemical Oceanography Data Management Office |
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| Metadata version: | 1 |
| Keydate: | 2023-05-13 04:44:15+00 |
| Editdate: | 2023-05-13 04:45:11+00 |