An optimised method for intact nuclei isolation from diatoms

Due to their abundance in the oceans, their extraordinary biodiversity and the increasing use for biotech applications, the study of diatom biology is receiving more and more attention in the recent years. One of the limitations in developing molecular tools for diatoms lies in the peculiar nature o...

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Bibliographic Details
Published in:Scientific reports 2021-01, Vol.11 (1), p.1681-1681, Article 1681
Main Authors: Annunziata, Rossella, Balestra, Cecilia, Marotta, Pina, Ruggiero, Antonella, Manfellotto, Francesco, Benvenuto, Giovanna, Biffali, Elio, Ferrante, Maria Immacolata
Format: Article
Language:English
Subjects:
631/208/191
704/829/826
Bacillariophyceae
Biodiversity
Cell Fractionation - methods
Cell Fractionation - standards
Cell Nucleus - chemistry
Cell Nucleus - genetics
Cell Nucleus - metabolism
Cell walls
Deoxyribonucleic acid
Diatoms - cytology
Diatoms - genetics
Diatoms - metabolism
DNA
DNA - genetics
DNA - metabolism
Epigenetics
Humanities and Social Sciences
Lysis
Marine microorganisms
Microscopy, Confocal
multidisciplinary
Nuclei
Oceans
Organelles
Plankton
Proteomics
Science
Science (multidisciplinary)
Silica
Sonication
Species
Subcellular Fractions - metabolism
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Summary:Due to their abundance in the oceans, their extraordinary biodiversity and the increasing use for biotech applications, the study of diatom biology is receiving more and more attention in the recent years. One of the limitations in developing molecular tools for diatoms lies in the peculiar nature of their cell wall, that is made of silica and organic molecules and that hinders the application of standard methods for cell lysis required, for example, to extract organelles. In this study we present a protocol for intact nuclei isolation from diatoms that was successfully applied to three different species: two pennates, Pseudo-nitzschia multistriata and Phaeodactylum tricornutum, and one centric diatom species, Chaetoceros diadema . Intact nuclei were extracted by treatment with acidified NH 4 F solution combined to low intensity sonication pulses and separated from cell debris via FAC-sorting upon incubation with SYBR Green. Microscopy observations confirmed the integrity of isolated nuclei and high sensitivity DNA electrophoresis showed that genomic DNA extracted from isolated nuclei has low degree of fragmentation. This protocol has proved to be a flexible and versatile method to obtain intact nuclei preparations from different diatom species and it has the potential to speed up applications such as epigenetic explorations as well as single cell (“single nuclei”) genomics, transcriptomics and proteomics in different diatom species.
ISSN:2045-2322
2045-2322
DOI:10.1038/s41598-021-81238-z