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  • 2010-2014  (14)
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  • 1
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    PANGAEA
    In:  Supplement to: Croot, Peter L; Passow, Uta; Assmy, Philipp; Jansen, Sandra; Strass, Volker H (2007): Surface active substances in the upper water column during a Southern Ocean Iron Fertilization Experiment (EIFEX). Geophysical Research Letters, 34(3), L03612, https://doi.org/10.1029/2006GL028080
    Publication Date: 2023-10-28
    Description: Surface active substances (SAS) in the water column were measured by voltammetry using the electrochemical probe o-nitrophenol (ONP) during EIFEX, a mesoscale open ocean iron enrichment experiment in the Southern Ocean. SAS levels were low throughout the experiment (〈0.005 - 0.03 mg/L Triton X-100 equivalents). Initially SAS was extremely low in the photic zone, but as the phytoplankton bloom developed concentrations markedly increased throughout the upper 100 m (~0.02 mg/L Triton X-100 equivalents). Highest concentrations of SAS (〉0.02 mg/L Triton X-100 equivalents) were found at the end of the bloom particularly at density discontinuities where organic material may accumulate. Exudates from diatoms appeared to be the major source of SAS during EIFEX, either from direct extracellular release or in the action of being grazed upon by zooplankton.
    Keywords: ANT-XXI/3; Comment; Date/Time of event; DEPTH, water; Elevation of event; Event label; GOFLO; Go-Flo bottles; Latitude of event; Longitude of event; Polarstern; Priority Programme 1158 Antarctic Research with Comparable Investigations in Arctic Sea Ice Areas; PS65/508-1; PS65/514-1; PS65/543-9; PS65/570-1; PS65/580-1; PS65 EIFEX; South Atlantic Ocean; SPP1158; Surface active substances; Surface active substances, standard deviation; Voltammetry
    Type: Dataset
    Format: text/tab-separated-values, 144 data points
    Location Call Number Limitation Availability
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  • 2
    Publication Date: 2024-02-16
    Keywords: 06PO20050321; CTD; CTD/Rosette; CTD-RO; Date/Time of event; DEPTH, water; Elevation of event; Event label; Iron; Iron, dissolved; Iron, dissolved, standard deviation; Iron, standard deviation; Latitude of event; Longitude of event; Monosaccharides as glucose equivalent; Monosaccharides as glucose equivalent, standard deviation; Polysaccharides as glucose equivalent; Polysaccharides as glucose equivalent, standard deviation; POS320/1; POS320/1_36-1; POS320/1_37-1; POS320/1_40-1; POS320/1_42-1; POS320/1_43-1; POS320/1_46-1; POS320/1_47-1; POS320/1_49-1; POS320/1_50-1; POS320/1_51-1; POS320/1_52-1; POS320/1_52-2; POS320/1_55-2; POS320/1_56-1; POS320/1_58-2; POS320/1_61-2; POS320/1_62-1; POS320/1_63-1; POS320/1_64-1; POS320/1_65-2; POS320/1_68-1; Poseidon; Saccharides, total as glucose equivalent; Saccharides, total as glucose equivalent, standard deviation; Sample ID; SOPRAN; Surface Ocean Processes in the Anthropocene; Teflon pump; Transparent exopolymer particles as Gum Xanthan equivalents per volume; Transparent exopolymer particles as Gum Xanthan equivalents per volume, std dev; Tropical NE Atlantic
    Type: Dataset
    Format: text/tab-separated-values, 1411 data points
    Location Call Number Limitation Availability
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  • 3
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    PANGAEA
    In:  Supplement to: Arnosti, Carol; Grossart, Hans-Peter; Mühling, M; Joint, Ian; Passow, Uta (2011): Dynamics of extracellular enzyme activities in seawater under changed atmospheric pCO2: a mesocosm investigation. Aquatic Microbial Ecology, 64(3), 285-298, https://doi.org/10.3354/ame01522
    Publication Date: 2024-03-15
    Description: As part of the PeECE II mesocosm project, we investigated the effects of pCO2 levels on the initial step of heterotrophic carbon cycling in the surface ocean. The activities of microbial extracellular enzymes hydrolyzing 4 polysaccharides were measured during the development of a natural phytoplankton bloom under pCO2 conditions representing glacial (190 µatm) and future (750 µatm) atmospheric pCO2. We observed that (1) chondroitin hydrolysis was variable throughout the pre-, early- and late-bloom phases, (2) fucoidanase activity was measurable only in the glacial mesocosm as the bloom developed, (3) laminarinase activity was low and constant, and (4) xylanase activity declined as the bloom progressed. Concurrent measurements of microbial community composition, using denaturing-gradient gel electrophoresis (DGGE), showed that the 2 mesocosms diverged temporally, and from one another, especially in the late-bloom phase. Enzyme activities correlated with bloom phase and pCO2, suggesting functional as well as compositional changes in microbial communities in the different pCO2 environments. These changes, however, may be a response to temporal changes in the development of phytoplankton communities that differed with the pCO2 environment. We hypothesize that the phytoplankton communities produced dissolved organic carbon (DOC) differing in composition, a hypothesis supported by changing amino acid composition of the DOC, and that enzyme activities responded to changes in substrates. Enzyme activities observed under different pCO2 conditions likely reflect both genetic and population-level responses to changes occurring among multiple components of the microbial loop.
    Keywords: 14C-leucine incorporation; Alkalinity, total; Aragonite saturation state; Bacteria, production as carbon; Bacterial cell multiplication; Bicarbonate ion; BIOACID; Biological Impacts of Ocean Acidification; Biomass/Abundance/Elemental composition; Calcite saturation state; Calculated using seacarb after Nisumaa et al. (2010); Carbon, inorganic, dissolved; Carbonate ion; Carbonate system computation flag; Carbon dioxide; Cell density; Cell density, standard deviation; Chondroitin sulfate hydrolysis; Coast and continental shelf; EPOCA; EUR-OCEANS; European network of excellence for Ocean Ecosystems Analysis; European Project on Ocean Acidification; Experimental treatment; Experiment day; Field experiment; Fucoidan hydrolysis; Fugacity of carbon dioxide (water) at sea surface temperature (wet air); Identification; Laminarin hydrolysis; Measured; Mesocosm or benthocosm; North Atlantic; OA-ICC; Ocean Acidification International Coordination Centre; Other metabolic rates; Partial pressure of carbon dioxide (water) at sea surface temperature (wet air); Pelagos; pH; Proportion of total bacteria attached to particles; Salinity; Sample ID; see reference(s); Temperate; Temperature, water; Thymidine incorporation; Time, incubation; Xylan hydrolysis
    Type: Dataset
    Format: text/tab-separated-values, 664 data points
    Location Call Number Limitation Availability
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  • 4
    Publication Date: 2015-09-21
    Description: As part of the PeECE II mesocosm project, we investigated the effects of pCO2 levels on the initial step of heterotrophic carbon cycling in the surface ocean. The activities of microbial extracellular enzymes hydrolyzing 4 polysaccharides were measured during the development of a natural phytoplankton bloom under pCO2 conditions representing glacial (190 µatm) and future (750 µatm) atmospheric pCO2. We observed that (1) chondroitin hydrolysis was variable throughout the pre-, early- and late-bloom phases, (2) fucoidanase activity was measurable only in the glacial mesocosm as the bloom developed, (3) laminarinase activity was low and constant, and (4) xylanase activity declined as the bloom progressed. Concurrent measurements of microbial community composition, using denaturing-gradient gel electrophoresis (DGGE), showed that the 2 mesocosms diverged temporally, and from one another, especially in the late-bloom phase. Enzyme activities correlated with bloom phase and pCO2, suggesting functional as well as compositional changes in microbial communities in the different pCO2 environments. These changes, however, may be a response to temporal changes in the development of phytoplankton communities that differed with the pCO2 environment. We hypothesize that the phytoplankton communities produced dissolved organic carbon (DOC) differing in composition, a hypothesis supported by changing amino acid composition of the DOC, and that enzyme activities responded to changes in substrates. Enzyme activities observed under different pCO2 conditions likely reflect both genetic and population-level responses to changes occurring among multiple components of the microbial loop.
    Type: Article , PeerReviewed
    Format: text
    Location Call Number Limitation Availability
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  • 5
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    In:  [Poster] In: 3. International Symposium on The Ocean in a high-CO2 World, 24.-27.09.2012, Monterey, USA .
    Publication Date: 2014-11-25
    Type: Conference or Workshop Item , NonPeerReviewed
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  • 6
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    COPERNICUS GESELLSCHAFT MBH
    In:  EPIC3Biogeosciences, COPERNICUS GESELLSCHAFT MBH, 11(15), pp. 4173-4190, ISSN: 1726-4170
    Publication Date: 2014-08-25
    Description: The degradation of marine dissolved organic matter (DOM) is an important control variable in the global carbon cycle. For our understanding of the kinetics of organic matter cycling in the ocean, it is crucial to achieve a mechanistic and molecular understanding of its transformation processes. A long-term microbial experiment was performed to follow the production of non-labile DOM by marine bacteria. Two different glucose concentrations and dissolved algal exudates were used as substrates. We monitored the bacterial abundance, concentrations of dissolved and particulate organic carbon (DOC, POC), nutrients, amino acids, and transparent exopolymer particles (TEP) for two years. The molecular characterization of extracted DOM was performed by ultrahigh resolution Fourier Transform Ion Cyclotron Resonance Mass Spectrometry (FT-ICR MS) after 70 days and after ~2 years of incubation. Although glucose was quickly degraded, a non-labile DOC background (5-9% of the initial DOC) was generated in the glucose incubations. Only 20% of the organic carbon from the algal exudate was degraded within the 2 years of incubation. The degradation rates for the non-labile DOC background in the different treatments varied between 1 and 11 µmol DOC L-1 yr-1. TEP, which are released by microorganisms, were produced during glucose degradation but decreased back to half of the maximum concentration within less than three weeks (degradation rate: 25 µg xanthan gum equivalents L-1 d-1) and were below detection in all treatments after 2 years. Additional glucose was added after two years to test whether labile substrate can promote the degradation of background DOC (co-metabolism; priming effect). A priming effect was not observed but the glucose addition led to a slight increase of background DOC. The molecular analysis demonstrated that DOM generated during glucose degradation differed appreciably from DOM transformed during the degradation of the algal exudates. Our results led to several conclusions: (i) Based on our experimental setup, higher substrate concentration resulted in a higher concentration of non-labile DOC; (ii) TEP, generated by bacteria, are degraded rapidly, thus limiting their potential contribution to carbon sequestration; (iii) The molecular signatures of DOM derived from algal exudates or glucose after 70 days of incubation differed strongly from refractory DOM. After 2 years, however, the molecular patterns of DOM in glucose incubations were more similar to deep ocean DOM whereas the degraded exudate was still different.
    Repository Name: EPIC Alfred Wegener Institut
    Type: Article , isiRev
    Format: application/pdf
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  • 7
    Publication Date: 2019-07-17
    Repository Name: EPIC Alfred Wegener Institut
    Type: Article , isiRev
    Format: application/pdf
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  • 8
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    In:  EPIC3Marine Ecology Progress Series 404, pp. 21-29
    Publication Date: 2019-07-17
    Repository Name: EPIC Alfred Wegener Institut
    Type: Article , isiRev
    Format: application/pdf
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  • 9
    Publication Date: 2019-07-17
    Repository Name: EPIC Alfred Wegener Institut
    Type: Article , isiRev
    Format: application/pdf
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  • 10
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    In:  EPIC3Biologie in unserer Zeit, 40(5), pp. 304-313
    Publication Date: 2019-07-17
    Repository Name: EPIC Alfred Wegener Institut
    Type: Article , peerRev
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