Please use this identifier to cite or link to this item: http://hdl.handle.net/1942/36908
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dc.contributor.authorHEMERYCK, Lara-
dc.contributor.authorHERMANS, Florian-
dc.contributor.authorChappell, Joel-
dc.contributor.authorKobayashi, Hiroto-
dc.contributor.authorLambrechts, Diether-
dc.contributor.authorLAMBRICHTS, Ivo-
dc.contributor.authorBRONCKAERS, Annelies-
dc.contributor.authorVankelecom, Hugo-
dc.date.accessioned2022-03-17T10:13:59Z-
dc.date.available2022-03-17T10:13:59Z-
dc.date.issued2022-
dc.date.submitted2022-03-02T10:52:12Z-
dc.identifier.citationCELLULAR AND MOLECULAR LIFE SCIENCES, 79 (3) (Art N° 153)-
dc.identifier.urihttp://hdl.handle.net/1942/36908-
dc.description.abstractInsight into human tooth epithelial stem cells and their biology is sparse. Tissue-derived organoid models typically replicate the tissue's epithelial stem cell compartment. Here, we developed a first-in-time epithelial organoid model starting from human tooth. Dental follicle (DF) tissue, isolated from unerupted wisdom teeth, efficiently generated epithelial organoids that were long-term expandable. The organoids displayed a tooth epithelial stemness phenotype similar to the DF's epithelial cell rests of Malassez (ERM), a compartment containing dental epithelial stem cells. Single-cell transcriptomics reinforced this organoid-ERM congruence, and uncovered novel, mouse-mirroring stem cell features. Exposure of the organoids to epidermal growth factor induced transient proliferation and eventual epithelial-mesenchymal transition, highly mimicking events taking place in the ERM in vivo. Moreover, the ERM stemness organoids were able to unfold an ameloblast differentiation process, further enhanced by transforming growth factor-beta (TGF beta) and abrogated by TGF beta receptor inhibition, thereby reproducing TGF beta's known key position in amelogenesis. Interestingly, by creating a mesenchymal-epithelial composite organoid (assembloid) model, we demonstrated that the presence of dental mesenchymal cells (i.e. pulp stem cells) triggered ameloblast differentiation in the epithelial stem cells, thus replicating the known importance of mesenchyme-epithelium interaction in tooth development and amelogenesis. Also here, differentiation was abrogated by TGF beta receptor inhibition. Together, we developed novel organoid models empowering the exploration of human tooth epithelial stem cell biology and function as well as their interplay with dental mesenchyme, all at present only poorly defined in humans. Moreover, the new models may pave the way to future tooth-regenerative perspectives.-
dc.description.sponsorshipThis work was supported by grants from KU Leuven (Research Fund) and Fund for Scientific Research (FWO) Flanders. L.H. is an FWO PhD Fellow (1S84718N). Acknowledgements We are grateful to all staff members of the Oral and Maxillofacial Surgery (MKA) of UZ Leuven, as well as the patients, for their invaluable help and contribution to collect freshly extracted third molars. We would also like to thank Dr. Reinhilde Jacobs and Dr. Elisabeth Tijskens for their help with sample collection. We thank Dr. Diether Lambrechts’ group for their technical assistance in 10× Genomics. Computational resources for scRNA-seq analysis were provided by ‘Vlaams Supercomputer Centrum’ (VSC), managed by the Fund for Scientific Research (FWO)—Flanders (Belgium). We acknowledge the use of the TEM platforms at VIB-KU Leuven, Biomedical Research Institute (BIOMED) UHasselt, and Institute of Development, Aging and Cancer, Tohoku University (Sendai, Japan). We would also like to thank Dr. Ronald Driesen (UHasselt) for help with CTOF analysis, and Dr. Marianne Carlon’s group (particularly Liesbeth De Keersmaecker; KU Leuven) for guiding and assisting in lentiviral transduction. We are grateful to Jeanine Santermans and Marc Jans (UHasselt) for their technical assistance in TEM and staining analyses. We also would like to thank Reena Chinnaraj and Vera Dermesrobian (FACS Core, KU Leuven) for their help with FACS experiments.-
dc.language.isoen-
dc.publisherSpringer-
dc.rightsThe Author(s) 2022-
dc.subject.otherTooth-
dc.subject.otherOrganoids-
dc.subject.otherStem cells-
dc.subject.otherAmeloblasts-
dc.subject.otherAssembloids-
dc.subject.otherTGF beta-
dc.titleOrganoids from human tooth showing epithelial stemness phenotype and differentiation potential-
dc.typeJournal Contribution-
dc.identifier.issue3-
dc.identifier.volume79-
local.bibliographicCitation.jcatA1-
local.publisher.placePICASSOPLATZ 4, BASEL, 4052, SWITZERLAND-
local.type.refereedRefereed-
local.type.specifiedArticle-
local.bibliographicCitation.artnr153-
dc.identifier.doi10.1007/s00018-022-04183-8-
dc.identifier.pmid35217915-
dc.identifier.isiWOS:000761959200003-
local.provider.typeCrossRef-
local.uhasselt.internationalyes-
item.fullcitationHEMERYCK, Lara; HERMANS, Florian; Chappell, Joel; Kobayashi, Hiroto; Lambrechts, Diether; LAMBRICHTS, Ivo; BRONCKAERS, Annelies & Vankelecom, Hugo (2022) Organoids from human tooth showing epithelial stemness phenotype and differentiation potential. In: CELLULAR AND MOLECULAR LIFE SCIENCES, 79 (3) (Art N° 153).-
item.fulltextWith Fulltext-
item.validationecoom 2023-
item.contributorHEMERYCK, Lara-
item.contributorHERMANS, Florian-
item.contributorChappell, Joel-
item.contributorKobayashi, Hiroto-
item.contributorLambrechts, Diether-
item.contributorLAMBRICHTS, Ivo-
item.contributorBRONCKAERS, Annelies-
item.contributorVankelecom, Hugo-
item.accessRightsOpen Access-
crisitem.journal.issn1420-682X-
crisitem.journal.eissn1420-9071-
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