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During the summer of 2018 and fall of 2019, six experiments were conducted to investigate the effect of phytoplankton growth phase on the ingestion rage of the copepod Calanus pacificus<\/em> on phytoplankton and marine snow aggregates (formed from the same phytoplankton). Each experiment consisted of three treatments: a control (in which copepods were placed in tanks with filtered seawater and no food source), an individual phytoplankton treatment (in which copepods were placed in tanks with individual phytoplankton as a food source), and an aggregate treatment (in which copepods were placed in tanks with aggregates as a food source). The six experiments were: Experiment 1 conducted in June of 2018, Experiment 2 in July of 2018, Experiment 3 in September of 2019, Experiment 4 in October of 2019, Experiment 5 in November of 2019, and Experiment 6 in December of 2019. Ingestion rate was quantified in these experiments using two methods: gut pigment analysis and stable isotope analysis.<\/p>\n C. pacificus<\/em> was collected using a small boat near Scripps Canyon in La Jolla, CA (32\u00b0 51.720\u2019 N, 117\u00b0 16.816\u2019 W) 5-20 days before each experiment with a 333 \u00b5m mesh plankton net (0.5 m diameter mouth). Samples were sorted in the lab to isolate individuals of the species C. pacificus<\/em>. Copepods were maintained with regular water changes in an incubator in the dark at 18\u00b0C until the experiment and fed a mixed diet of Thalassiosira weissflogii<\/em> and haptophytes (Tisochrysis sp. and Pavlova sp.<\/em>) for the 2018 experiments and Thalassiosira weissflogii<\/em> and Skeletonema marinoi<\/em> for the 2019 experiments. Copepods were starved for 24 hours prior to each experiment by transferring 30 C. pacificus<\/em> individuals (C5 copepodites and female adults) into a beaker corresponding to each treatment tank. Each beaker was wrapped in aluminum foil to maintain darkness, and was kept at room temperature.<\/p>\n Prior to each experiment, phytoplankton cultures of the species T. weissflogii<\/em> (Experiments 1, 2, 3, and 5) or S. marinoi<\/em> (Experiments 4 and 6) were started in 2L flasks. All cultures were grown in f\/2 media at room temperature under 12:12 hour LED light:dark cycle. In total, two culture flasks were started for each growth phase: one flask for the aggregate treatment and one flask for the phytoplankton treatment. The aggregate treatment culture flasks were started three days prior to the phytoplankton treatment culture flasks, to account for the fact that the aggregate treatment culture flasks were stopped three days earlier to allow for aggregate formation on a roller table (described below). Experiments 1 and 2 were carried out for three different growth phases phases (with the corresponding phytoplankton culturing time shown in parentheses): Early Exponential (5 days), Late Exponential (13 days), and Late Stationary (20 days). Experiments 3, 4, 5, and 6 were carried out for Early Exponential (5 days) and Late Exponential (12 days) growth phases. To carry out ingestion rate measurements using stable isotope analysis, 1.7 mL of an N-15 nitrate solution (7.5 g\/L N-15 potassium nitrate salt in DI water) was added to each phytoplankton culture 3 days before the culture was to be stopped (except for Experiment 1 where 12.75 mL of N-15 nitrate solution was added 2 days before each culture was stopped). Stable isotope analysis was not carried out for Experiment 2. Right before adding N-15 labeled nitrate to each culture, 25 mL of the culture was filtered onto a GF\/F to be used as initial measurements of naturally occurring N-15 concentrations in the phytoplankton cultures.<\/p>\n Three days before each experiment, after the aggregate treatment phytoplankton cultures had grown for the time specified above (depending on growth phase), these cultures were diluted (to 20,000 cell\/mL for T. weissflogii<\/em> and 39,000 cells\/mL for S. marinoi<\/em>) and added to two cylindrical acrylic tanks (each with a volume of 550 mL). These cylindrical tanks were allowed to rotate in the dark on roller table for 3 days at a rate of 4.6 rpm to form aggregates.<\/p>\n On the day of each experiment for each growth phase, two replicate cylindrical tanks (each with a volume of 2200 mL) were prepared per treatment (control, individual phytoplankton, and aggregate), thus resulting in 6 tanks per experiment per growth phase. The control tanks were filled completely with filtered seawater along with a small amount of N-15 nitrate solution such that the final concentration of N-15 in the tank was comparable to that in the phytoplankton and aggregate treatment tanks. The phytoplankton treatment tanks were filled with the phytoplankton culture that was diluted with filtered seawater (to final concentration of 5,000 cells\/mL for T. weissflogii<\/em> and 9,750 cells\/mL for S. marinoi<\/em>). For the aggregate treatments, aggregates formed in the smaller cylindrical tanks were transferred to the experimental tank (which had four times the volume) along with the associated seawater; the rest of the volume of the experimental tank was filled with filtered seawater, thus resulting in an equivalent phytoplankton concentration (in cells\/mL) between the phytoplankton and aggregate treatment tanks. For each treatment tank, 30 copepods were added and copepods were allowed to feed for an hour while the tank slowly rotating at ~1 rpm. Note that due to a lack of copepods, only one tank per treatment was run in the Late Stationary growth phase for Experiment 1 and only one control tank was run in the Late Stationary growth phase for Experiment 2.<\/p>\n Immediately after the one-hour incubation time had elapsed for each treatment, 40 mL of seltzer water was added to the tank to anesthetize the copepods. The copepods were removed from the cylindrical experimental tank with gentle suctioning of water onto a filter. For stable isotope analysis, immediately after the one-hour feeding experiment in each tank, five sets of two copepods were transferred by forceps into tin cups for each tank of each treatment (only 3 to 4 sets of two copepods were collected for Experiment 1, and no stable isotope analysis data was collected for Experiment 2 due to of lack of copepods). For each experiment, 5-6 sets of two unfed copepods (which were starved alongside experimental copepods but not used in any feeding tank) were transferred into tin cups to be used as initials, which were used to measure the natural concentration of N-15 in copepods before being exposed to phytoplankton grown in N-15 nitrate solution. Three replicates of 250 mL each of the remaining tank water for each treatment was filtered onto a GF\/F and packed into a tin cup for N-15 measurements of the food that was fed to the copepods in each treatment. All samples were sent off to be processed at UC Davis Stable Isotope Facility (with the exception of Experiment 1, in which samples were processed on an Isotope Ratio Mass Spectrometer at Scripps Institution of Oceanography).<\/p>\n