Calanoid copepod abundances in the northern Benguela Current System from 2009 and 2010

Abundance data of copepods were derived from vertical Multinet hauls at 10 stations, carried out in the northern Benguela upwelling system in December 2009 (FRS Africana) and September/October 2010 (RRS Discovery). Three transects along ~ 17°S, 19°S and 23°S with three stations each (neritic, shelf break, oceanic) and one station at 21°S were analysed for copepod abundance. Maximum sampling depth was either close to the seafloor (neritic and shelf break stations) or 700 m (2009) and 1000 m (2010) for the oceanic stations. Calanoid copepod species and stages were identified and enumerated separately. Adult females, males and copepodite stage 5 (C5) (in case of C. carinatus and N. minor) were included in the abundance calculations. Abundance is expressed as number of individuals per m**3, calculated from the volume of water filtered (calibrated flowmeter, Hydro-Bios) and the maximum sampling depth at each station.

Feeding parameters of copepods from upwelling areas

Feeding patterns of mass herbivorous copepods in upwelling areas are investigated. Daily rations and aspects of their formation are examined in Calanoides carinatus (Benguela upwelling), Calanus pacificus (off the California coast), and Calanus australis (Peru upwelling). Rations were calculated based on gut plant pigment contents obtained at daily stations using laser spectrofluorometry, experimental data on the rate of gut evacuation and data on the carbon/chlorophyll ratio in phytoplankton and particulate matter at the respective stations. When phytoplankton was abundant, diel feeding rhythms were not pronounced and gut pigment level was high during the entire 24-h period. When phytoplankton biomass was low, distinct feeding rhythms were pronounced with a nocturnal maximum. During active upwelling intensive feeding on phytoplankton supports energy (respiration) and plastic (growth, development, reproduction, accumulation of reserves) metabolism of copepods. When upwelling was inactive, the surface part of the population feeds less actively and is able only partially to cover its energy expenditures. The actively growing and reproducing populations of C. pacificus and C. carinatus may consume close to 20% of primary production, whereas the inactive population of C. australis consumed only 0.2% of primary production when upwelling weakened.

Planktonic foraminiferas in bottom sediments and paleotemperatures in the areas of the Benguela and Canary upwellings

Distribution of planktonic foraminiferal tests was studied in four drill cores of Upper Quaternary sediments from the zone of influence of the Canary upwelling and in nine sediment cores from the zone of the Benguela upwelling. Paleotemperatures were reconstructed from these data. It was established that under conditions during stadials, interstadials, and interglacials of Quaternary time, the upwelling existed continuously, intensifying and expanding during colder epochs and weakening and contracting in the warmer intervals. During the last stadial (about 18000 yrs ago), relative cooling of sea waters as compared to central regions of the ocean in the zone of the Canary upwelling was not lower than 9°C (4.5°C higher than at present time), and in the zone of the Benguela upwelling it was not lower than 15°C (8.5°C higher than at present time).

Respiration and ingestion rates of calanoid copepod in the northern Benguela Current System measured ex situ during the RSS Discovery D356 cruise in 2010

Respiration rates of 16 calanoid copepod species from the northern Benguela upwelling system were measured on board RRS Discovery in September/October 2010 to determine their energy requirements and assess their significance in the carbon cycle. Copepod species were sampled by different net types. Immediately after the hauls, samples were sorted to species and stages (16 species; females, males and C5 copepodids) according to Bradford-Grieve et al. (1999). Specimens were kept in temperature-controlled refrigerators for at least 12 h before they were used in experiments. Respiration rates of different copepod species were measured onboard by optode respirometry (for details see Köster et al., 2008) with a 10-channel optode respirometer (PreSens Precision Sensing Oxy-10 Mini, Regensburg, Germany) under simulated in situ conditions in temperature-controlled refrigerators. Experiments were run in gas-tight glass bottles (12-13 ml). For each set of experiments, two controls without animals were measured under exactly the same conditions to compensate for potential bias. The number of animals per bottle depended on the copepods size, stage and metabolic activity. Animals were not fed during the experiments but they showed natural species-specific movements. Immediately after the experiments, all specimens were deep-frozen at - 80 °C for later dry mass determination (after lyophilisation for 48 h) in the home lab. The carbon content (% of dry mass) of each species was measured by mass-spectrometry in association with stable isotope analysis and body dry mass was converted to units of carbon. For species without available carbon data, the mean value of all copepod species (44% dry mass) was applied. For the estimation of carbon requirements of copepod species, individual oxygen consumption rates were converted to carbon units, assuming that the expiration of 1 ml oxygen mobilises 0.44 mg of organic carbon by using a respiratory quotient (RQ) of 0.82 for a mixed diet consisting of proteins (RQ = 0.8-1.0), lipids (RQ = 0.7) and carbohydrates (RQ = 1.0) (Auel and Werner, 2003). The carbon ingestion rates were calculated using the energy budget and the potential maximum ingestion rate approach. To allow for physiological comparisons of respiration rates of deep- and shallow-living copepod species without the effects of ambient temperature and different individual body mass, individual respiration rates were temperature- (15°C, Q10=2) and size-adjusted. The scaling coefficient of 0.76 (R2=0.556) is used for the standardisation of body dry mass to 0.3 mg (mean dry mass of all analysed copepods), applying the allometric equation R= (R15°C/M0.76)×0.30.76, where R is respiration and M is individual dry mass in mg.