Identifying differentiation markers between dermal fibroblasts and adipose-derived mesenchymal stromal cells (AD-MSCs) in human visceral and subcutaneous tissues using single-cell transcriptomics

被引:0
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作者
Koczkowska, Magdalena [1 ]
Kostecka, Anna [1 ,2 ]
Zawrzykraj, Malgorzata [3 ]
Myszczynski, Kamil [4 ]
Skoniecka, Aneta [5 ]
Deptula, Milena [5 ]
Tyminska, Agata [5 ]
Czerwiec, Katarzyna [3 ]
Jakalski, Marcin [1 ]
Zielinski, Jacek [6 ]
Crossman, David K. [7 ]
Crowley, Michael R. [7 ]
Cichorek, Miroslawa [5 ]
Skowron, Piotr M. [8 ]
Pikula, Michal [5 ]
Piotrowski, Arkadiusz [1 ,2 ]
机构
[1] Med Univ Gdansk, 3P Med Lab, Gdansk, Poland
[2] Med Univ Gdansk, Dept Biol & Pharmaceut Bot, Gdansk, Poland
[3] Med Univ Gdansk, Dept Anat, Div Clin Anat, Gdansk, Poland
[4] Med Univ Gdansk, Ctr Biostat & Bioinformat Anal, Gdansk, Poland
[5] Med Univ Gdansk, Dept Anat, Div Embryol, Gdansk, Poland
[6] Med Univ Gdansk, Dept Surg Oncol Transplant Surg & Gen Surg, Gdansk, Poland
[7] Univ Alabama Birmingham, Genom Core Facil, Birmingham, AL USA
[8] Univ Gdansk, Fac Chem, Dept Mol Biotechnol, Gdansk, Poland
关键词
Single-cell RNA sequencing; scRNA-seq; Human adipose-derived mesenchymal stromal cells; AD-MSCs; Dermal fibroblasts; Visceral AD-MSCs; Subcutaneous AD-MSCs; Regenerative medicine; Heterogeneity; STEM-CELLS; INTERNATIONAL-SOCIETY; EXTRACELLULAR-MATRIX; EXPRESSION; GROWTH;
D O I
10.1186/s13287-025-04185-w
中图分类号
Q813 [细胞工程];
学科分类号
摘要
BackgroundAdipose-derived mesenchymal stromal cells (AD-MSCs) and fibroblasts are both widely used in regenerative medicine, demonstrating significant potential for personalized cell therapy. A major challenge in their use lies in their high biological similarity, encompassing morphology, differentiation capabilities, and flow cytometric markers, making their distinction difficult.MethodsIn our study, we aimed to compare AD-MSCs obtained from two types of adipose tissue, subcutaneous and visceral, alongside skin fibroblasts. Notably, all tissue samples were sourced from the same donors. We analyzed the cells for surface antigens via flow cytometry and conducted single-cell RNA sequencing, followed by verification with quantitative PCR (qPCR).ResultsOur results revealed phenotypic similarities between the isolated AD-MSCs and dermal fibroblasts, particularly in the expression of markers characteristic of AD-MSCs. However, through in-depth analyses, we identified distinct differences between these cell types. Specifically, we pinpointed 30 genes exhibiting the most significant variations in expression between AD-MSCs and fibroblasts. These genes are associated with biological processes such as tissue remodeling, cell movement, and activation in response to external stimuli. Among them, MMP1, MMP3, S100A4, CXCL1, PI16, IGFBP5, COMP were further validated using qPCR, clearly demonstrating their potential to differentiate between AD-MSCs and fibroblasts.ConclusionsOur scRNA-seq analysis elucidates the transcriptional landscape of AD-MSCs and fibroblasts with unprecedented resolution, highlighting both the population-specific markers and the intrapopulation heterogeneity. Our findings underscore the importance of employing high-resolution techniques for cell identification. Created with BioRender.co.
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页数:12
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