Publication:
Taurine Augments Telomerase Activity and Promotes Chondrogenesis in Dental Pulp Stem Cells

dc.contributor.authorJamal, Mohamed
dc.date.accessioned2022-03-15T10:06:19Z
dc.date.available2022-03-15T10:06:19Z
dc.date.issued2021
dc.description.abstractBackground: Stem cell therapy has become an advanced and state-of-the-art procedure to regenerate lost tissues of the human body. Cartilage repair is a challenging task in which stem cells find potential application. One of the important biologic modifiers that can cause chondrogenic differentiation of stem cells is taurine. However, taurine has not been investigated for its effects on dental pulp derived stem cell (DPSC) chondrogenic differentiation. Objective: The objective of the study was to investigate if taurine administration to DPSCs heralds chondrogenic differentiation as ascertained by expression of SOX9, COL2A1, ACAN, ELN, and COMP. The study also investigated if the differentiated cells synthesized glycosaminoglycans, a marker of cartilage formation. The study also aimed to assess proliferative activity of the cells after taurine administration by measuring the hTERT gene and protein expression. Materials and methods: DPSCs were obtained from a molecular biology laboratory and characterization of stem cell markers was done by flow cytometry. The cells were subjected to a MTT assay using various concentrations of taurine. Following this, hTERT gene and protein estimation was done in the control, telomerase inhibitor treated DPSC (TI-III), 10 µM taurine treated DPSC, and TI-III + 10 µM taurine treated DPSCs. A polymerase chain reaction was done to assess gene expression of SOX9, COL2A1, ACAN, ELN, and COMP genes and glycosaminoglycans were estimated in control cells, Induced DPSCs, induced and TI-III treated DPSCs, and 10 µM taurine treated DPSCs. Results: DPSCs expressed CD73, CD90, and CD105 and did not express CD34, CD45, and HLA-DR, which demonstrated that they were mesenchymal stem cells. The MTT assay revealed that various concentrations of taurine did not affect the cell viability of DPSCs. A concentration of 10 µM of taurine was used for further assays. With regard to the hTERT gene and protein expression, the taurine treated cells expressed the highest levels that were statistically significant compared to the other groups. Taurine was also found to restore hTERT expression in telomerase inhibitor treated cells. With regard to chondrogenesis related genes, taurine administration significantly increased the expression of SOX9, COL2A1, ACAN, and ELN genes in DPSCs and caused a significant increase in glycosaminoglycan production by the cells. Conclusions: Taurine can be regarded a biologic modifier that can significantly augment chondrogenic differentiation of DPSCs and can find potential applications in regenerative medicine in the area of cartilage regeneration.en_US
dc.identifier.other304-2021.45
dc.identifier.urihttps://repository.mbru.ac.ae/handle/1/910
dc.language.isoenen_US
dc.subjectMesenchymal stem cellsen_US
dc.subjectChondrogenesisen_US
dc.subjectTelomeraseen_US
dc.subjectTaurineen_US
dc.subjectDental pulpen_US
dc.subjectRegenerative medicineen_US
dc.titleTaurine Augments Telomerase Activity and Promotes Chondrogenesis in Dental Pulp Stem Cellsen_US
dc.typeArticleen_US
dspace.entity.typePublicationen_US

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