Chemical reprogramming culture for the expansion of salivary gland epithelial basal progenitor cells

Ye Jin Jeong; Yongpyo Hong; Yeo-Jun Yoon; Nam Suk Sim; Seung-Min Hong; Jae-Yol Lim

doi:10.1186/s13287-025-04295-5

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Chemical reprogramming culture for the expansion of salivary gland epithelial basal progenitor cells

Authors: Ye Jin Jeong ; Yongpyo Hong ; Yeo-Jun Yoon ; Nam Suk Sim ; Seung-Min Hong ; Jae-Yol Lim

Citation: STEM CELL RESEARCH & THERAPY, Vol.16(1) : 187, 2025-04

Journal Title: STEM CELL RESEARCH & THERAPY

Issue Date: 2025-04

MeSH: Animals ; Cell Differentiation / drug effects ; Cell Proliferation ; Cells, Cultured ; Cellular Reprogramming* ; Epithelial Cells* / cytology ; Epithelial Cells* / drug effects ; Epithelial Cells* / metabolism ; Humans ; Mice ; Organoids ; Salivary Glands* / cytology ; Salivary Glands* / metabolism ; Stem Cells* / cytology ; Stem Cells* / drug effects ; Stem Cells* / metabolism

Keywords: Basal progenitor cell ; Cell therapy ; Chemical reprogramming culture ; Epithelial stem cell ; Salivary gland

Abstract: Background: Salivary gland (SG) hypofunction presents a significant clinical challenge with limited treatment options. SG epithelial cells offer a promising approach due to their intrinsic tissue specificity and regenerative potential. However, the lack of efficient culture methods has hindered their clinical use.

Methods: This study presents a chemical reprogramming culture (CRC) system that utilizes a combination of three small molecules for the long-term two-dimensional culture of human SG epithelial progenitor cells. We characterized the cultured cells, measured their organoid-forming efficiencies, and assessed their differentiation potential. To evaluate the therapeutic efficacy of the SG basal progenitor cells (SG-BPCs), we administered them into a mouse model with radiation-induced SG hypofunction and assessed the functional recovery.

Results: By utilizing optimal concentrations of the small molecules Y-27632, A83-01, and LDN193189, the SG epithelial cells achieved over 50 population doubling levels (PD) within 80 d, surpassing the Hayflick limit. β-galactosidase and Terminal deoxynucleotidyl transferase dUTP nick end labeling staining confirmed that these small molecules inhibited cellular senescence and apoptosis, respectively. The cells expressed SG basal ductal cell markers KRT5, KRT19, and SOX9, with increased expression levels observed from PD5 to PD40. Notably, these expanded cells were able to differentiate into various SG cell types, including acinar and myoepithelial cells, indicating that SG-basal progenitor cells (SG-BPCs) were selectively proliferated using our CRC method. To assess the therapeutic potential of the expanded SG-BPCs, they were administered to mice with radiation-induced SG hypofunction. The treatment successfully restored SG function.

Conclusion: Our findings demonstrate that our CRC system is an effective method for the long-term culture of SG-BPCs. This advancement holds significant promise for the development of SG epithelial progenitor-based therapies to treat SG hypofunction.