Methods

I. Study System Lake Mývatn, Iceland (65°36 N, 17°0′ W) is a large (38 km²) shallow (4 m max depth) lake divided into two large basins that function mostly as independent hydrologic bodies (Ólafsson 1979). The number of non-biting midge (Diptera: Chironomidae) larvae on the lake bottom is high, but variable: midge production between 1972-74 ranged from 14-100 g ash-free dw m^-2 yr^-1, averaging 28 g dw m^-2 yr^-1 (Lindegaard and Jónasson 1979). The midge assemblage is mostly comprised of two species (> 90% of total individuals), Chironomus islandicus (Kieffer) and Tanytarsus gracilentus (Holmgren) that feed as larvae in the sediment in silken tubes by scraping diatoms, algae, and detritus off the lake bottom (Lindegaard and Jónasson 1979). At maturity (May-August) midge pupae float to the lake surface, emerge as adults, and fly to land, forming large mating swarms around the lake (Einarsson et al. 2004, Gratton et al. 2008). On land, midges are consumed by terrestrial predators (Dreyer et al. 2012, Gratton et al. 2008), or enter the detrital pool upon death (Gratton et al. 2008, Hoekman et al. 2012). Midge populations naturally cycle with 5-8 year periodicity, with abundances fluctuating by 3-4 orders of magnitude (Einarsson et al. 2002, Ives et al. 2008). II. Midge Infall Measurement We deployed eleven transects of passive, lethal aerial infall traps arrayed at variable distances from Lake Mývatn to estimate relative midge abundance on shore during the summers 2008-2011. Each transect was perpendicular to the lake edge, with traps located at approximately 5, 50, 150, and 500 m (where possible) from shore for a total of 31 traps around the lake. Sampling locations were recorded using GPS and precise distances from the lake were calculated within a geographic information system. Traps consisted of a single 1000 mL clear plastic cup (0.0095 m² opening) affixed 1 m above the ground on a stake and filled with 300-500 mL of a 1:1 mixture of water and ethylene glycol and a trace amount of unscented detergent to capture, kill, and preserve insects landing on the surface of the liquid (Gratton et al. 2008, Dreyer et al. 2012). Midges and other insects were emptied from the traps weekly and the traps were reset immediately, thus collections span the entirety of each summer. III. Identification, Counts, and Conversions Midges were counted and identified to morphospecies, small and large. The midge (Diptera,Chrionomidae) assemblage at Mývatn is dominated by two species, Chironomus islandicus (Kieffer)(large, 1.1 mg dw) and Tanytarsus gracilentus (Holmgren)(small, 0.1 mg dw), together comprising 90 percent of total midge abundance (Lindegaard and Jonasson 1979). First, the midges collected in the infall traps were spread out in trays, and counted if there were only a few. Some midges were only identified to the family level of Simuliidae, and other arthropods were counted and categorized as the group, others. Arthropods only identified to the family level Simuliidae or classified as others were not dually counted as Chironomus islandicus or Tanytarsus gracilentus . If there were many midges, generally if there were hundreds to thousands, in an infall trap, subsamples were taken. Subsampling was done using plastic rings that were dropped into the tray. The rings were relatively small compared to the tray, about 2 percent of the area of a tray was represented in a ring. The area inside a ring and the total area of the trays were also measured. Note that different sized rings and trays were used in subsample analysis. These are as follows, trays, small (area of 731 square centimeters), “large1” (area of 1862.40 square centimeters), and large2 (area of 1247 square centimeters). Rings, standard ring (diameter of 7.30 centimeters, subsample area is 41.85 square centimeters) and small ring (diameter of 6.5 centimeters, subsample area is 33.18 square centimeters). A small ring was only used to subsample trays classified as type “large2.”The fraction subsampled was then calculated depending on the size of the tray and ring used for the subsample analysis. If the entire tray was counted and no subsampling was done then the fraction subsampled was assigned a value of 1.0. If subsampling was done the fraction subsampled was calculated as the number of subsamples taken multiplied by the fraction of the tray that a subsample ring area covers (number of subsamples multiplied by (ring area divided by tray area)). Note that this is dependent on the tray and ring used for subsample analysis. Finally, the number of midges in an infall trap accounting for subsampling was calculated as the raw count of midges divided by the fraction subsampled (raw count divided by fraction subsampled).Other metrics such as total insects in meters squared per day, and total insect biomass in grams per meter squared day can be calculated with these data. In addition to the estimated average individual midge masses in grams, For 2008 through 2010 average midge masses were calculated as, Tanytarsus equal to .0001104 grams, Chironomus equal to .0010837 grams. For 2011 average midge masses were, Tanytarsus equal to .000182 grams, Chironomus equal to .001268 grams.

Methods

I. Study System Lake Mývatn, Iceland (65°36 N, 17°0′ W) is a large (38 km²) shallow (4 m max depth) lake divided into two large basins that function mostly as independent hydrologic bodies (Ólafsson 1979). The number of non-biting midge (Diptera: Chironomidae) larvae on the lake bottom is high, but variable: midge production between 1972-74 ranged from 14-100 g ash-free dw m^-2 yr^-1, averaging 28 g dw m^-2 yr^-1 (Lindegaard and Jónasson 1979). The midge assemblage is mostly comprised of two species (> 90% of total individuals), Chironomus islandicus (Kieffer) and Tanytarsus gracilentus (Holmgren) that feed as larvae in the sediment in silken tubes by scraping diatoms, algae, and detritus off the lake bottom (Lindegaard and Jónasson 1979). At maturity (May-August) midge pupae float to the lake surface, emerge as adults, and fly to land, forming large mating swarms around the lake (Einarsson et al. 2004, Gratton et al. 2008). On land, midges are consumed by terrestrial predators (Dreyer et al. 2012, Gratton et al. 2008), or enter the detrital pool upon death (Gratton et al. 2008, Hoekman et al. 2012). Midge populations naturally cycle with 5-8 year periodicity, with abundances fluctuating by 3-4 orders of magnitude (Einarsson et al. 2002, Ives et al. 2008). II. Midge Emergence Measurement We used submerged conical traps to estimate midge emergence from Lake Mývatn. Traps were constructed of 2 mm clear polycarbonate plastic (Laird Plastics, Madison, WI) formed into a cone with large-diameter opening of 46 cm (0.17 m²). The tops of the cones were open to a diameter of 10 cm, with a clear jar affixed at the apex. The trap was weighted to approximately neutral buoyancy, with the jar at the top containing air to allow mature midges to emerge. Traps were suspended with a nylon line ~1 m below the surface of the lake from an anchored buoy. For sampling, traps were raised to the surface and rapidly inverted, preventing midges from escaping. Jars and traps were thoroughly rinsed with lake water to collect all trapped midges, including unmetamorphosed larvae and pupae, and scrubbed before being returned to the lake to prevent growth of epiphytic algae and colonization by midges. We assume that the emergence traps collect all potentially emerging midges from the sampling area, though it is likely an underestimate, since some midges initially captured could fall out of the trap. Thus, our results should be considered a conservative estimate of potential midge emergence from the surface of the lake.We sampled midge emergence throughout the south basin of Lake Mývatn. Emergence was sampled at six sites in 2008 and 2011 and ten sites in 2009 and 2010, with locations relocated using GPS and natural sightlines. Each site had two traps within 5 m of each other that were monitored during midge activity, approximately from the last week of May to the first week of August. Midge emergence outside of this time frame is extremely low (Lindegaard & Jónasson 1979) and we assume it to be zero. Traps were checked weekly during periods of high emergence (initial and final 2-3 weeks of the study), and bi-weekly during low emergence periods in the middle of the study (July). III. Identification, Counts, and Conversions Midges were counted and identified to morphospecies, small and large. The midge (Diptera,Chrionomidae) assemblage at Mývatn is dominated by two species, Chironomus islandicus (Kieffer)(large, 1.1 mg dw) and Tanytarsus gracilentus (Holmgren)(small, 0.1 mg dw), together comprising 90 percent of total midge abundance (Lindegaard and Jonasson 1979). First, the midges collected in the infall traps were spread out in trays, and counted if there were only a few. Some midges were only identified to the family level of Simuliidae, and other arthropods were counted and categorized as the group, others. Arthropods only identified to the family level Simuliidae or classified as others were not dually counted as Chironomus islandicus or Tanytarsus gracilentus . If there were many midges, generally if there were hundreds to thousands, in an infall trap, subsamples were taken. Subsampling was done using plastic rings that were dropped into the tray. The rings were relatively small compared to the tray, about 2 percent of the area of a tray was represented in a ring. The area inside a ring and the total area of the trays were also measured. Note that different sized rings and trays were used in subsample analysis. These are as follows, trays, small (area of 731 square centimeters), “large1” (area of 1862.40 square centimeters), and large2 (area of 1247 square centimeters). Rings, standard ring (diameter of 7.30 centimeters, subsample area is 41.85 square centimeters) and small ring (diameter of 6.5 centimeters, subsample area is 33.18 square centimeters). A small ring was only used to subsample trays classified as type “large2.”The fraction subsampled was then calculated depending on the size of the tray and ring used for the subsample analysis. If the entire tray was counted and no subsampling was done then the fraction subsampled was assigned a value of 1.0. If subsampling was done the fraction subsampled was calculated as the number of subsamples taken multiplied by the fraction of the tray that a subsample ring area covers (number of subsamples multiplied by (ring area divided by tray area)). Note that this is dependent on the tray and ring used for subsample analysis. Finally, the number of midges in an infall trap accounting for subsampling was calculated as the raw count of midges divided by the fraction subsampled (raw count divided by fraction subsampled).Other metrics such as total insects in meters squared per day, and total insect biomass in grams per meter squared day can be calculated with these data. In addition to the estimated average individual midge masses in grams, For 2008 through 2010 average midge masses were calculated as, Tanytarsus equal to .0001104 grams, Chironomus equal to .0010837 grams. For 2011 average midge masses were, Tanytarsus equal to .000182 grams, Chironomus equal to .001268 grams.

Methods

Water samples are taken along routine sampling and then prepared into permanent slides by the company Phyco Tech. Slides are available for all years, however, species may not have been determined for all available slides.
several taxonomic updates were implemented in February 2013, this includes simple name changes to currently accepted names, changes from genus level to species based on long term experience by Phyco Tech, and some slides were revisited to resolve taxonomic uncertainty.
1) Converted all Melosira entries to Aulacoseira. The species names have been changed appropriately. 2) Converted all Oscillatoria entries to Psuedanabaena. The species names have been changed appropriately. 3) Converted all Synedra tenera to Synedra filiformis. 4) Converted all Phacotus entries without a species name to Phacotus lendneri. 5) Converted all Phormidium mucicola to Psuedanabaena 6) Converted Glenodinium entries without a species name to Glenodinium quadridens 7) Assume that all other entries with genera names but not species names cannot be resolved to species. 8) Converted all Chrysococcus entries to Chrysocccus minutus 9) Changed some single-celled Microcystis entries so that they would match the format of the colonial entries (genus + species) 10) Resolved some entries to species that were previously coded incorrectly by genus. 11) Added in Cylindrospermopsis raciborskii entries that were recently recounted and changed from Anabaenopsis raciborskii. 12) Converted all entries of genus Erkenia to Erkenia subaequiciliata

Methods

Phytoplankton samples are collected using a peristaltic pump and tubing, collecting a separate sample from the epilimnion, metalimnion and hypolimnion for most of the lakes. For 27-2 Bog Lake, which is only 2m deep, we collect one 0-2m composite sample. The samples are preserved with Lugol's iodine solution. We create a single hypsometrically pooled composite sample per lake from subsamples of the epi, meta, and hypo samples. The pooled samples are sent to PhycoTech, Inc., a private lab specializing in plankton analysis, to be made into permanent slide mounts. The slides are archived, and no wet samples are saved.