Nitrogen isotopic evidence for a shift from nitrate- to diazotroph-fueled export production in VAHINE mesocosm experiments
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Abstract. In a shallow, coastal lagoon off the southwest coast of New Caledonia, large-volume (~ 50 m3) mesocosm experiments were undertaken to track the fate of newly fixed nitrogen (N). The mesocosms were intentionally fertilized with 0.8 M dissolved inorganic phosphorus (DIP) to stimulate diazotrophy. N isotopic evidence indicates that the dominant source of N fueling export production shifted from subsurface nitrate (NO3) assimilated prior to the start of the 23 day experiments to N2 fixation by the end of the experiments. While the 15N of the sinking particulate N (PNsink) flux changed during the experiments, the 15N of the suspended PN (PNsusp) and dissolved organic N (DON) pools did not. This is consistent with previous observations that the 15N of surface ocean N pools is less responsive than that of PNsink to changes in the dominant source of new N to surface waters. In spite of the absence of detectable NO3 in the mesocosms, the 15N of PNsink indicated that NO3 continued to fuel a significant fraction of export production (20 to 60 %) throughout the 23 day experiments, with N2 fixation dominating export after about two weeks. The low rates of primary productivity and export production during the first 14 days were primarily supported by NO3, and phytoplankton abundance data suggest that export was driven by large diatoms sinking out of surface waters. Concurrent molecular and taxonomic studies indicate that the diazotroph community was dominated by diatom-diazotroph assemblages (DDAs) at this time. However, these DDAs represented a minor fraction (< 5 %) of the total diatom community and contributed very little new N via N2 fixation; they were thus not important for driving export production, either directly or indirectly. The unicellular cyanobacterial diazotroph, a Cyanothece-like UCYN-C, proliferated during the last phase of the experiments when N2 fixation, primary production, and the flux of PNsink increased significantly, and 15N budgets reflected a predominantly diazotrophic source of N fueling export production. At this time, the export flux itself was likely dominated by the non-diazotrophic diatom, Cylindrotheca closterium, along with a lesser contribution from other eukaryotic phytoplankton and a small contribution (< 10 %) from aggregated UCYN-C cells. Despite comprising a small fraction of the total biomass, UCYN-C was largely responsible for driving export production during the last ~ 10 days of the experiments through the rapid transfer of its newly fixed N to other phytoplankton; we infer that this newly fixed N was transferred through the DON and/or ammonium pools. This inference reconciles previous observations of invariant oligotrophic surface ocean DON concentrations and 15N with incubation studies showing that diazotrophs can release a significant fraction of their newly fixed N as some form of DON.
