Carbon-concentrating mechanisms and beta-carboxylation: their potential contribution to marine photosynthetic carbon isotope fractionation

• Main Author: Cassar, Nicolas
• Other Authors: Laws, Edward A
• Published: University of Hawaii at Manoa 2009
• Online Access: http://hdl.handle.net/10125/6884

The ability of the ocean to buffer the concentration of CO2 in the atmosphere through the so-called biological pump depends on the extent to which the photosynthetic rate of marine phytoplankton is limited by the concentration of CO2 in the water. If CO2 becomes available to phytoplankton by passive diffusion through the boundary layer around the cell, then the growth of large cells, which are believed to contribute disproportionately to the biological pump, could be limited by CO2 availability. However, many species appear to have the ability to circumvent diffusion control through the use of carbon-concentrating mechanisms (CCMs) such as active CO2 uptake, bicarbonate (HCO3-) transport, and carbonic anhydrase activity. These mechanisms are likely adaptations to the fact that the main carbon fixing enzyme, ribulose-1,5-bisphosphate carboxylase-oxygenase (Rubisco), is less than half saturated at normal seawater CO2 concentrations. Using short-term 14CO2-disequilibrium experiments, a clone of the marine diatom Phaeodactylum tricornutum was shown to take up little or no HCO3- even under conditions of severe CO2 limitation. These results agree with predictions based on stable carbon isotopic fractionation data and demonstrate that combining isotopic disequilibrium experiments with continuous growth cultures and stable isotope fractionation experiments is a powerful tool for understanding the response of oceanic primary producers to anthropogenic CO2 emissions as well as for interpreting paleoceanographic carbon isotope data. Isotopic disequilibrium experiments were also performed in the field to estimate the extent of photosynthetic bicarbonate (HCO3-) uptake in the oceans. The experiments were conducted in the Southern Ocean during the Southern Ocean Iron Experiment (SOFeX). In contrast to the results with P. tricornutum, approximately half of the photosynthetic inorganic carbon uptake was direct HCO3- uptake, the other half being direct CO2 uptake (passive and/or active uptake). A low-CO2 treatment induced an increase in uptake of CO2 through increased enzymatically mediated extracellular dehydration of HCO3- (carbonic anhydrase activity), which was at the expense of direct HCO3- transport across the plasmalemma. Because of the presence of CCMs, biological productivity in the Southern Ocean is unlikely to be directly regulated by natural or anthropogenic variations in atmospheric CO2 concentration. These results are consistent with stable isotope fractionation models and could have important implications for the global biogeochemical cycle of carbon. It is generally believed that most of the variations in stable isotope fractionation are associated with changes in CCM activity. A review and experimental study of the various factors that influence CCM activity and therefore photosynthetic carbon isotope fractionation revealed that, other than CCMs, several factors that have been essentially ignored in the scientific literature may also contribute to the isotopic signature of photosynthetic organic matter. In this study, photorespiration appeared to be of greater magnitude than commonly reported in marine diatoms, although its contribution to isotopic fractionation was negligible. Isotopic fractionation during photosynthesis in P. tricornutum was found to be well correlated to changes in Rubisco enzyme kinetics and to the molar organic carbon to nitrogen ratio (C/N). Contrary to the general scientific belief, the C/N proved to be dependent on the CO2 concentration, with the greatest dependency at lower growth rates, presumably because of luxury carbon uptake at lower growth rates. At higher growth rates, a tighter coupling of the organic nitrogen and carbon cycles may explain the lower responsiveness of C/N to changes in CO2 concentration. The contribution of carboxylases other than Rubisco to photosynthetic stable carbon isotope fractionation was also examined. Some f3-carboxylation enzymes, such as phosphoenolpyruvate carboxylase (PEPC), have a carbon isotope discrimination factor different from Rubisco and may significantly contribute to carbon fixation. Changes in PEPC/Rubisco activity under various growth conditions may explain some of the variations in stable isotope fractionation. The f3-carboxylase activity in P. tricornutum increased with decreasing growth rates and increasing CO2 concentrations. PEPC activities larger than generally reported in the literature were observed. This difference may be attributable to variations in methodological approaches. A multitude of factors may influence overall photosynthetic carbon isotope fractionation. Understanding these factors will be crucial to the use of isotopic analyses for paleo-CO2 reconstruction. === xiv, 222 leaves