Comparison of techniques used to count single-celled viable phytoplankton

dc.contributor.author Steinberg, Mia K.
dc.contributor.author First, Matthew R.
dc.contributor.author Lemieux, Edward J.
dc.contributor.author Drake, Lisa A.
dc.contributor.author Nelson, Bruce N.
dc.contributor.author Kulis, David M.
dc.contributor.author Anderson, Donald M.
dc.contributor.author Welschmeyer, Nicholas A.
dc.contributor.author Herring, Penny R.
dc.date.accessioned 2012-09-26T18:03:41Z
dc.date.available 2012-09-26T18:03:41Z
dc.date.issued 2010-10-14
dc.description Author Posting. © The Author(s), 2010. This is the author's version of the work. It is posted here by permission of Springer for personal use, not for redistribution. The definitive version was published in Journal of Applied Phycology 24 (2012): 751-758, doi:10.1007/s10811-011-9694-z. en_US
dc.description.abstract Four methods commonly used to count phytoplankton were evaluated based upon the precision of concentration estimates: Sedgewick Rafter and membrane filter direct counts, flow cytometry, and flow-based imaging cytometry (FlowCAM). Counting methods were all able to estimate the cell concentrations, categorize cells into size classes, and determine cell viability using fluorescent probes. These criteria are essential to determine whether discharged ballast water complies with international standards that limit the concentration of viable planktonic organisms based on size class. Samples containing unknown concentrations of live and UV-inactivated phytoflagellates (Tetraselmis impellucida) were formulated to have low concentrations (<100 ml-1) of viable phytoplankton. All count methods used chlorophyll a fluorescence to detect cells and SYTOX fluorescence to detect non-viable cells. With the exception of one sample, the methods generated live and non-viable cell counts that were significantly different from each other, although estimates were generally within 100% of the ensemble mean of all subsamples from all methods. Overall, percent coefficient of variation (CV) among sample replicates was lowest in membrane filtration sample replicates, and CVs for all four counting methods were usually lower than 30% (although instances of ~60% were observed). Since all four methods were generally appropriate for monitoring discharged ballast water, ancillary considerations (e.g., ease of analysis, sample processing rate, sample size, etc.) become critical factors for choosing the optimal phytoplankton counting method. en_US
dc.description.sponsorship This study was supported by the U.S. Coast Guard Research and Development Center under contract HSCG32-07- X-R00018. Partial research support to DMA and DMK was provided through NSF International Contract 03/06/394, and Environmental Protection Agency Grant RD-83382801-0. en_US
dc.format.mimetype application/pdf
dc.identifier.uri https://hdl.handle.net/1912/5388
dc.language.iso en_US en_US
dc.relation.uri https://doi.org/10.1007/s10811-011-9694-z
dc.subject Phytoplankton en_US
dc.subject Enumeration en_US
dc.subject FlowCAM en_US
dc.subject Flow cytometry en_US
dc.subject Sedgewick Rafter en_US
dc.subject Ballast water en_US
dc.subject SYTOX Green en_US
dc.subject CellTracker Green en_US
dc.title Comparison of techniques used to count single-celled viable phytoplankton en_US
dc.type Preprint en_US
dspace.entity.type Publication
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