An efficient and affordable laboratory method to produce and sustain high concentrations of microcystins by Microcystis aeruginosa

René S. Shahmohamadloo; Xavier Ortiz Almirall; Claire Holeton; Richard Chong-Kit; David G. Poirier; Satyendra P. Bhavsar; Paul K. Sibley

MethodsX (Jan 2019)

An efficient and affordable laboratory method to produce and sustain high concentrations of microcystins by Microcystis aeruginosa

René S. Shahmohamadloo,
Xavier Ortiz Almirall,
Claire Holeton,
Richard Chong-Kit,
David G. Poirier,
Satyendra P. Bhavsar,
Paul K. Sibley

Affiliations

René S. Shahmohamadloo: School of Environmental Sciences, University of Guelph, Guelph, Ontario, Canada; Corresponding author.
Xavier Ortiz Almirall: Ministry of the Environment, Conservation and Parks, Toronto, Ontario, Canada; School of Environmental Studies, Queen’s University, Kingston, Ontario, Canada
Claire Holeton: Ministry of the Environment, Conservation and Parks, Toronto, Ontario, Canada
Richard Chong-Kit: Ministry of the Environment, Conservation and Parks, Toronto, Ontario, Canada
David G. Poirier: Ministry of the Environment, Conservation and Parks, Toronto, Ontario, Canada
Satyendra P. Bhavsar: Ministry of the Environment, Conservation and Parks, Toronto, Ontario, Canada; Department of Physical & Environmental Sciences, University of Toronto, Toronto, Ontario, Canada
Paul K. Sibley: School of Environmental Sciences, University of Guelph, Guelph, Ontario, Canada

Journal volume & issue: Vol. 6
pp. 2521 – 2535

Abstract

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Microcystis aeruginosa is a cosmopolitan cyanobacteria that continues to jeopardize freshwater ecosystem services by releasing the hepatotoxin microcystin, which can, in some cases, cause death to aquatic fauna and even humans. Currently, our abilities to understand the mechanisms of microcystin toxicology are limited by the lack of a method for producing high concentrations, which are central to large-scale and long-term research in natural systems. Here we present an efficient and affordable laboratory method to produce high concentrations of microcystins by a toxigenic strain of M. aeruginosa. Through batch culture studies, we yielded microcystins at concentrations that are environmentally relevant to freshwaters around the world (1–300 μg L−1), maintained these concentrations without resupplying fresh medium (further reducing costs), and utilized rate equations to model the relationship between the environmental conditions in the cultures and changes occurring within the M. aeruginosa cells. Our assessment suggests that steady production of microcystins depends on the availability of carbon throughout the experiment. Hence, we recommend the use of tissue culture treated flasks with a vented cap to ensure the production of microcystins is uninterrupted. This method demonstrates that microcystins can be produced in the laboratory at concentrations relevant to freshwater ecosystems. • The method demonstrates M. aeruginosa CPCC 300 is a reliable strain of freshwater cyanobacteria that can yield microcystins at environmentally relevant concentrations. • Validation showed M. aeruginosa CPCC 300 is resilient in carbon-limited situations and may respond to stress by shifting the ratio of microcystin congeners. • Cell culture flasks with vented caps —filled no more than 50 % of the flask volume to allow for sufficient air exchange— are an excellent and cost-effective approach to maintaining cell growth and producing microcystins at a range between 300 to 1200 μg L−1. Method name: Method for production of microcystins in Blue-Green-11 (BG-11) medium, Keywords: Strain CPCC 300, Cyanobacteria, Cyanotoxins, Harmful algal blooms, Toxicology

Published in MethodsX

ISSN: 2215-0161 (Online)
Publisher: Elsevier
Country of publisher: Netherlands
LCC subjects: Science
Website: http://www.journals.elsevier.com/methodsx/

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