High-glutathione mesenchymal stem cells isolated using the FreSHtracer probe enhance cartilage regeneration in a rabbit chondral defect model

被引:3
|
作者
Cho, Gun Hee [1 ,2 ]
Bae, Hyun Cheol [2 ]
Cho, Won Young [2 ]
Jeong, Eui Man [3 ]
Park, Hee Jung [2 ]
Yang, Ha Ru [2 ]
Wang, Sun Young [2 ]
Kim, You Jung [2 ]
Shin, Dong Myung [4 ]
Chung, Hyung Min [5 ]
Kim, In Gyu [6 ]
Han, Hyuk-Soo [1 ,2 ]
机构
[1] Seoul Natl Univ, Coll Med, Dept Orthoped Surg, 101 Daehak Ro, Seoul 03080, South Korea
[2] Seoul Natl Univ Hosp, Dept Orthoped Surg, Seoul 110744, South Korea
[3] Jeju Natl Univ, Coll Pharm, Dept Pharm, Jeju Special Self Governi, Jeju Do, South Korea
[4] Univ Ulsan, Asan Med Ctr, Dept Biomed Sci, Coll Med, 88 Olym Ro 43 Gil, Seoul 05505, South Korea
[5] Konkuk Univ, Sch Med, Dept Stem Cell Biol, Seoul 05029, South Korea
[6] Cell2in Inc, Lab Cellular Response Oxidat Stress, Seoul 03127, South Korea
关键词
FreSHtracer; Glutathione; Mesenchymal stem cells; Cartilage regeneration; Chondral defect; DIFFERENTIATION; OXYGEN; IMPAIRMENT; BIOLOGY; SOX9; ROS;
D O I
10.1186/s40824-023-00398-3
中图分类号
R318 [生物医学工程];
学科分类号
0831 ;
摘要
Background Mesenchymal stem cells (MSCs) are a promising cell source for cartilage regeneration. However, the function of MSC can vary according to cell culture conditions, donor age, and heterogeneity of the MSC population, resulting in unregulated MSC quality control. To overcome these limitations, we previously developed a fluorescent real-time thiol tracer (FreSHtracer) that monitors cellular levels of glutathione (GSH), which are known to be closely associated with stem cell function. In this study, we investigated whether using FreSHtracer could selectively separate high-functioning MSCs based on GSH levels and evaluated the chondrogenic potential of MSCs with high GSH levels to repair cartilage defects in vivo.Methods Flow cytometry was conducted on FreSHtracer-loaded MSCs to select cells according to their GSH levels. To determine the function of FreSHtracer-isolated MSCs, mRNA expression, migration, and CFU assays were conducted. The MSCs underwent chondrogenic differentiation, followed by analysis of chondrogenic-related gene expression. For in vivo assessment, MSCs with different cellular GSH levels or cell culture densities were injected in a rabbit chondral defect model, followed by histological analysis of cartilage-regenerated defect sites.Results FreSHtracer successfully isolated MSCs according to GSH levels. MSCs with high cellular GSH levels showed enhanced MSC function, including stem cell marker mRNA expression, migration, CFU, and oxidant resistance. Regardless of the stem cell tissue source, FreSHtracer selectively isolated MSCs with high GSH levels and high functionality. The in vitro chondrogenic potential was the highest in pellets generated by MSCs with high GSH levels, with increased ECM formation and chondrogenic marker expression. Furthermore, the MSCs' function was dependent on cell culture conditions, with relatively higher cell culture densities resulting in higher GSH levels. In vivo, improved cartilage repair was achieved by articular injection of MSCs with high levels of cellular GSH and MSCs cultured under high-density conditions, as confirmed by Collagen type 2 IHC, Safranin-O staining and O'Driscoll scores showing that more hyaline cartilage was formed on the defects.Conclusion FreSHtracer selectively isolates highly functional MSCs that have enhanced in vitro chondrogenesis and in vivo hyaline cartilage regeneration, which can ultimately overcome the current limitations of MSC therapy.
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页数:14
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