Culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers
Abstract Organoids emulate many aspects of their parental tissue and are therefore used to study pathogen-host interactions and other complex biological processes. Here, we report a robust protocol for the isolation, maintenance and differentiation of rabbit small intestinal organoids and organoid-d...
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2021-03-01
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Online Access: | https://doi.org/10.1038/s41598-021-84774-w |
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doaj-43223eede3be437581dc9245543fa6372021-03-11T12:24:14ZengNature Publishing GroupScientific Reports2045-23222021-03-0111111210.1038/s41598-021-84774-wCulture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayersEgi Kardia0Michael Frese1Elena Smertina2Tanja Strive3Xi-Lei Zeng4Mary Estes5Robyn N. Hall6Health and Biosecurity, Commonwealth Scientific and Industrial Research OrganisationHealth and Biosecurity, Commonwealth Scientific and Industrial Research OrganisationHealth and Biosecurity, Commonwealth Scientific and Industrial Research OrganisationHealth and Biosecurity, Commonwealth Scientific and Industrial Research OrganisationDepartment of Molecular Virology and Microbiology, Baylor College of MedicineDepartment of Molecular Virology and Microbiology, Baylor College of MedicineHealth and Biosecurity, Commonwealth Scientific and Industrial Research OrganisationAbstract Organoids emulate many aspects of their parental tissue and are therefore used to study pathogen-host interactions and other complex biological processes. Here, we report a robust protocol for the isolation, maintenance and differentiation of rabbit small intestinal organoids and organoid-derived cell monolayers. Our rabbit intestinal spheroid and monolayer cultures grew most efficiently in L-WRN-conditioned medium that contained Wnt, R-spondin and Noggin, and that had been supplemented with ROCK and TGF-β inhibitors. Organoid and monolayer differentiation was initiated by reducing the concentration of the L-WRN-conditioned medium and by adding ROCK and Notch signalling inhibitors. Immunofluorescence staining and RT-qPCR demonstrated that our organoids contained enterocytes, enteroendocrine cells, goblet cells and Paneth cells. Finally, we infected rabbit organoids with Rabbit calicivirus Australia-1, an enterotropic lagovirus that—like many other caliciviruses—does not grow in conventional cell culture. Despite testing various conditions for inoculation, we did not detect any evidence of virus replication, suggesting either that our organoids do not contain suitable host cell types or that additional co-factors are required for a productive infection of rabbit organoids with Rabbit calicivirus Australia-1.https://doi.org/10.1038/s41598-021-84774-w |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Egi Kardia Michael Frese Elena Smertina Tanja Strive Xi-Lei Zeng Mary Estes Robyn N. Hall |
spellingShingle |
Egi Kardia Michael Frese Elena Smertina Tanja Strive Xi-Lei Zeng Mary Estes Robyn N. Hall Culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers Scientific Reports |
author_facet |
Egi Kardia Michael Frese Elena Smertina Tanja Strive Xi-Lei Zeng Mary Estes Robyn N. Hall |
author_sort |
Egi Kardia |
title |
Culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers |
title_short |
Culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers |
title_full |
Culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers |
title_fullStr |
Culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers |
title_full_unstemmed |
Culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers |
title_sort |
culture and differentiation of rabbit intestinal organoids and organoid-derived cell monolayers |
publisher |
Nature Publishing Group |
series |
Scientific Reports |
issn |
2045-2322 |
publishDate |
2021-03-01 |
description |
Abstract Organoids emulate many aspects of their parental tissue and are therefore used to study pathogen-host interactions and other complex biological processes. Here, we report a robust protocol for the isolation, maintenance and differentiation of rabbit small intestinal organoids and organoid-derived cell monolayers. Our rabbit intestinal spheroid and monolayer cultures grew most efficiently in L-WRN-conditioned medium that contained Wnt, R-spondin and Noggin, and that had been supplemented with ROCK and TGF-β inhibitors. Organoid and monolayer differentiation was initiated by reducing the concentration of the L-WRN-conditioned medium and by adding ROCK and Notch signalling inhibitors. Immunofluorescence staining and RT-qPCR demonstrated that our organoids contained enterocytes, enteroendocrine cells, goblet cells and Paneth cells. Finally, we infected rabbit organoids with Rabbit calicivirus Australia-1, an enterotropic lagovirus that—like many other caliciviruses—does not grow in conventional cell culture. Despite testing various conditions for inoculation, we did not detect any evidence of virus replication, suggesting either that our organoids do not contain suitable host cell types or that additional co-factors are required for a productive infection of rabbit organoids with Rabbit calicivirus Australia-1. |
url |
https://doi.org/10.1038/s41598-021-84774-w |
work_keys_str_mv |
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