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Quantitative polymerase chain reaction (qPCR) cyanotoxin data for eight mesocosm experiments in the Caloosahatchee River, Florida from May 2019 through August 2021

Metadata Updated: October 30, 2025

An interdisciplinary and multiagency study was conducted in southern Florida to examine harmful algal bloom (HAB) dynamics on the Caloosahatchee River, which drains from Lake Okeechobee to the west into the Gulf of Mexico. Using in-situ mesocosm experiments, ammonium, nitrate, phosphate, and urea were altered from ambient conditions to determine the effects on cyanotoxin biosynthesis gene presence and quantity as measured via quantitative polymerase chain reaction (qPCR). Eight experiments were conducted seasonally from May 2019 through July 2021 at the W.P. Franklin Lock and Dam. The experimental installations consisted of three floating metal cradles each containing four opaque fiberglass chambers filled with local river water. Each chamber was open at the top to allow free flow of air and light but closed off at every other part. This ensured the chambers were in the river but not getting cross-contaminated by exchange with the river water. The twelve chambers were each enriched using one of five treatments depending on the experiment: phosphate (P), nitrate (N), ammonium (A), urea (U) or control (C) – with only four of the five treatments selected, each with three replicates, for every experiment. The P, N, A, and U treatment chambers were enriched by applying a concentrated dosing solution of either dibasic dodecahydrate sodium phosphate, anhydrous sodium nitrate, liquid ammonium hydroxide, or urea, respectively to elevate concentrations above ambient levels. The control chambers were left unenriched. The mesocosms were treated and sampled in approximately 24-hour intervals over a 72-hour period (Time 0, Time 24, Time 48, Time 72). May and July 2021 mesocosms were additionally sampled one week from the initiation of the experiment (T240). Deoxyribonucleic acid (DNA) was extracted from these samples and tested via six qPCR assays to determine the presence and quantity of different cyanotoxin biosynthesis genes. Each qPCR assay tests for a different cyanotoxin biosynthesis gene with one assay testing for cyanobacterial 16S DNA as an internal control. The five toxin biosynthesis genes tested were microcystin (mcyE), nodularin (ndaF), saxitoxin (sxtA), anatoxin (anaC), and cylindrospermopsin (cyrA).

Access & Use Information

Public: This dataset is intended for public access and use. License: No license information was provided. If this work was prepared by an officer or employee of the United States government as part of that person's official duties it is considered a U.S. Government Work.

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Dates

Metadata Created Date September 13, 2025
Metadata Updated Date October 30, 2025

Metadata Source

Harvested from DOI USGS DCAT-US

Additional Metadata

Resource Type Dataset
Metadata Created Date September 13, 2025
Metadata Updated Date October 30, 2025
Publisher U.S. Geological Survey
Maintainer
Identifier http://datainventory.doi.gov/id/dataset/usgs-632c61aad34e900e86c5103b
Data Last Modified 2022-10-03T00:00:00Z
Category geospatial
Public Access Level public
Bureau Code 010:12
Metadata Context https://project-open-data.cio.gov/v1.1/schema/catalog.jsonld
Metadata Catalog ID https://ddi.doi.gov/usgs-data.json
Schema Version https://project-open-data.cio.gov/v1.1/schema
Catalog Describedby https://project-open-data.cio.gov/v1.1/schema/catalog.json
Harvest Object Id 6aa1df65-c4b7-4901-a430-c398279bc1ae
Harvest Source Id 2b80d118-ab3a-48ba-bd93-996bbacefac2
Harvest Source Title DOI USGS DCAT-US
Metadata Type geospatial
Old Spatial -82.0300, 26.5000, -81.2400, 26.7900
Source Datajson Identifier True
Source Hash 5e910fe8b3462fa3fb4c47772eae73f35081072f22cf8f3bc3051df977fa04cc
Source Schema Version 1.1
Spatial {"type": "Polygon", "coordinates": -82.0300, 26.5000, -82.0300, 26.7900, -81.2400, 26.7900, -81.2400, 26.5000, -82.0300, 26.5000}

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