Issue 16, 2022
From the journal:

Lab on a Chip

Viable protoplast formation of the coral endosymbiont alga Symbiodinium spp. in a microfluidics platform

Faiza Bashir,ab   Sándor Kovács,a   Ágnes Ábrahám,cd   Krisztina Nagy,c   Ferhan Ayaydin, ORCID logo §e   Ildikó Valkony-Kelemen,e   Györgyi Ferenc, ORCID logo a   Péter Galajda, ORCID logo c   Szilvia Z. Tóth, ORCID logo a   László Sass,a   Péter B. Kós, ORCID logo af   Imre Vass ORCID logo *a  and  Milán Szabó ORCID logo *ag  

* Corresponding authors

a Institute of Plant Biology, Biological Research Centre, Eötvös Loránd Research Network, Szeged, Hungary
E-mail: vass.imre@brc.hu, szabo.milan@brc.hu

b Doctoral School of Biology, University of Szeged, Szeged, Hungary

c Institute of Biophysics, Biological Research Centre, Eötvös Loránd Research Network, Szeged, Hungary

d Doctoral School of Multidisciplinary Medical Sciences, University of Szeged, Szeged, Hungary

e Cellular Imaging Laboratory, Biological Research Centre, Eötvös Loránd Research Network, Szeged, Hungary

f Department of Biotechnology, Faculty of Science and Informatics, University of Szeged, Szeged, Hungary

g Climate Change Cluster, University of Technology Sydney, Australia

Abstract

Symbiodiniaceae is an important dinoflagellate family which lives in endosymbiosis with reef invertebrates, including coral polyps, making them central to the holobiont. With coral reefs currently under extreme threat from climate change, there is a pressing need to improve our understanding on the stress tolerance and stress avoidance mechanisms of Symbiodinium spp. Reactive oxygen species (ROS) such as singlet oxygen are central players in mediating various stress responses; however, the detection of ROS using specific dyes is still far from definitive in intact Symbiodinium cells due to the hindrance of uptake of certain fluorescent dyes because of the presence of the cell wall. Protoplast technology provides a promising platform for studying oxidative stress with the main advantage of removed cell wall, however the preparation of viable protoplasts remains a significant challenge. Previous studies have successfully applied cellulose-based protoplast preparation in Symbiodiniaceae; however, the protoplast formation and regeneration process was found to be suboptimal. Here, we present a microfluidics-based platform which allowed protoplast isolation from individually trapped Symbiodinium cells, by using a precisely adjusted flow of cell wall digestion enzymes (cellulase and macerozyme). Trapped single cells exhibited characteristic changes in their morphology, cessation of cell division and a slight decrease in photosynthetic activity during protoplast formation. Following digestion and transfer to regeneration medium, protoplasts remained photosynthetically active, regrew cell walls, regained motility, and entered exponential growth. Elevated flow rates in the microfluidic chambers resulted in somewhat faster protoplast formation; however, cell wall digestion at higher flow rates partially compromised photosynthetic activity. Physiologically competent protoplasts prepared from trapped cells in microfluidic chambers allowed for the first time the visualization of the intracellular localization of singlet oxygen (using Singlet Oxygen Sensor Green dye) in Symbiodiniaceae, potentially opening new avenues for studying oxidative stress.

Graphical abstract: Viable protoplast formation of the coral endosymbiont alga Symbiodinium spp. in a microfluidics platform

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Article information

DOI
https://doi.org/10.1039/D2LC00130F
Article type
Paper
Submitted
09 Feb 2022
Accepted
25 Apr 2022
First published
19 May 2022
This article is Open Access
Creative Commons BY-NC license

Lab Chip, 2022,22, 2986-2999

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Viable protoplast formation of the coral endosymbiont alga Symbiodinium spp. in a microfluidics platform

F. Bashir, S. Kovács, Á. Ábrahám, K. Nagy, F. Ayaydin, I. Valkony-Kelemen, G. Ferenc, P. Galajda, S. Z. Tóth, L. Sass, P. B. Kós, I. Vass and M. Szabó, Lab Chip, 2022, 22, 2986 DOI: 10.1039/D2LC00130F

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