Methods

We collect zooplankton samples at the deepest part of the lake using two different gear types. We take one vertical tow with a Wisconsin Net (80um mesh), and a series of Schindler Patalas (53um mesh) samples spanning the water column. All samples are preserved in cold 95percent EtOH.
After collection we combine subsamples of the individual Schindler Patalas trap samples to create one hypsometrically pooled sample for each lakeordate. The individual depth samples are discarded after pooling except from one August sampling date per year. The Hypsometrically Pooled sample and the Wisconsin Net sample are archived in the UW Zoology museum.
We count zooplankton in one or two subsamples, each representing 1.8L of lake water, of the hypsometrically pooled samples to calculate zooplankton abundance. We count one sample date per month from the open water season, and the February ice cover sample. We identify individuals to genus or species, take length measurements, and count eggs and embryos.
Protocol log: 1981-May1984 -- a 0.5m high, 31L Schindler Patalas trap with 80um mesh net was used. Two Wisconsin Net tows were collected. Preservative was 12percent buffered formalin.
June1984 -- changed to 53um mesh net on Schindler trap.
July1986 -- began using the 2m high, 45L Schindler Patalas trap. Changed WI Net collection to take only one tow.
2001 -- changed zooplankton preservative from 12percent buffered formalin to 95percent EtOH.
The number of sample dates per year counted varies with lake and year, from 5 datesoryear to 17 datesoryear.
1981-1983 -- pooled samples are of several types: Total Pooled (TP) were created using equal volume subsamples of the Schindler samples. Epi, Meta, Hypo pooled used equal volume subsamples from the Schindler samples collected from each of the thermal strata. Strata Pooled used equal volume subsamples from the Epi, Meta, Hypo pooled samples to create an entire lake sample. Hypsometrically Pooled (HP) is our standard, which uses subsample volumes weighted to represent the hypsometry of the lake.

Methods

For detailed methods of data gathering, cleaning and compiling see attached pdf file.

Methods

Data were compiled from many sources, each was quality controlled and merged into this dataset. For detailed methods see attached PDF file.

Methods

Sampling:
Zooplankton were sampled approximately weekly with two net hauls through the water column (30 cm diameter net, 80 um mesh). Tows were taken at standard depths for almost all years. The standard depths are as follows: Peter, East Long, West Long, Crampton and Tuesday Lakes: 12m, Paul Lake: 8m, Ward Lake: 6m; exceptions are: for 2012 and beyond Tuesday Lake was sampled at 10m, Peter was sampled at 10m from 1984-1986, Paul was sampled at 7.5m in 1995. Samples were preserved with cold sugared formalin or Lugol's solution.

Methods

General: Bade, D., J. Houser, and S. Scanga (editors). 1998. Methods of the Cascading Trophic Interactions Project. 5th edition. Center for Limnology, University of Wisconsin-Madison, and Cary Institute of Ecosystem Studies, Millbrook, NY.

Methods

Samples counted prior to 1996 were assigned one taxon name with all taxonomic information. This taxon name was split into distinct columns of genus, species and description for archival as best possible. Samples from 2013-2015 were sent to Phycotech inc. (http://www.phycotech.com/) to be counted.

Methods

Methods for 1984-1990 were described by Carpenter and Kitchell (1993) and methods for 1991-1997 were described by Carpenter et al. (2001).

Methods

Methods for 1984-1990 were described by Carpenter and Kitchell (1993) and methods for 1991-1997 were described by Carpenter et al. (2001).

Methods

Detailed field and laboratory protocols can be found in the Cascade Methods Manual, found here: https://cascade.limnology.wisc.edu/public/public_files/methods/CascadeManual1998.pdf
POC, PON and DOC: 1. 100 - 300 ml (Typically ~200mL for PML, 150 metalimnion and 75 – 100 for the hypolimnion) of lake water from each depth was filtered through 153 um mesh to remove large zooplankton. Water was then filtered through a precombusted 25mm GF/F filter (0.7 um pore size) at less than 200 mm Hg pressure. Filters were placed in drying oven at 60 C to dry for at least 48 hours. 20mL of filtered water was stored in a scintillation vial and acidified with 200uL of 2N H2SO4 for DOC analysis. Blank samples for POC and DOC were prepared with deionized water to control for contamination. All samples were sent to the Cary Institute of Ecosystem Studies for analysis.

Methods

Protocol available in methods section of: http://msphere.asm.org/content/2/3/e00169-17
Prior to collection, water temperature and dissolved oxygen concentrations are measured using a YSI 550a. The ranges of the epilimnion and hypolimnion are determined based on the location of the thermocline (where temperature/oxygen is changing the fastest). The two layers are collected separately in 1 meter increments using an integrated water column sampler. Water samples are taken back to the lab, shaken thoroughly, and filtered via peristaltic pump through 0.22 micron filters (Pall Supor). Filters are temporarily stored at -20C after collection and then transferred to -80C after transport on dry ice from Trout Lake Station to UW-Madison. Nutrient samples are collected bi-weekly following standard LTER protocols. DNA is extracted from filters using a FASTDNA SpinKit for Soil with minor modifications. (In cases of low yield or specialized sequencing methods, a phenol-chloroform extraction is used instead). The protocol for sequencing and analysis of data varies by year and by sub-project.