Sca1+ Progenitor Cells (Ex vivo) Exhibits Differential Proteomic Signatures From the Culture Adapted Sca1+ Cells (In vitro), Both Isolated From Murine Skeletal Muscle Tissue

Sca1+ Progenitor Cells (Ex vivo) Exhibits Differential Proteomic Signatures From the Culture Adapted Sca1+ Cells (In vitro), Both Isolated From Murine Skeletal Muscle Tissue

Stem cell antigen-1 (Sca-1) is a glycosyl-phosphatidylinositol-anchored membrane protein that is expressed in a sub-population of muscle stem and progenitor cell types. Reportedly, Sca-1 regulates the myogenic property of myoblasts and Sca-1 −/− mice exhibited defective muscle regeneration. Although...

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Veröffentlicht in:Stem cell reviews and reports 2021-10, Vol.17 (5), p.1754-1767
Hauptverfasser: Kapoor, Saketh, Subba, Pratigya, Shenoy P, Sudheer, Bose, Bipasha
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Ataxin
Biomedical and Life Sciences
Biomedical Engineering and Bioengineering
Cell Biology
Cell culture
Cell differentiation
Cell fusion
Cell surface
Comparative analysis
Life Sciences
Mass spectroscopy
Membrane proteins
Mice
Microenvironments
Muscle, Skeletal
Musculoskeletal system
Myoblasts
Myotubes
Phosphatidylinositol
Progenitor cells
Protein biosynthesis
Proteins
Proteome
Proteomes
Proteomics
Regenerative Medicine/Tissue Engineering
Skeletal muscle
Stem Cells
Surface markers
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Zusammenfassung:Stem cell antigen-1 (Sca-1) is a glycosyl-phosphatidylinositol-anchored membrane protein that is expressed in a sub-population of muscle stem and progenitor cell types. Reportedly, Sca-1 regulates the myogenic property of myoblasts and Sca-1 −/− mice exhibited defective muscle regeneration. Although the role of Sca-1 in muscle development and maintenance is well-acknowledged, molecular composition of muscle derived Sca-1 + cells is not characterized. Here, we applied a high-resolution mass spectrometry-based workflow to characterize the proteomic landscape of mouse hindlimb skeletal muscle derived Sca-1 + cells. Furthermore, we characterized the impact of the cellular microenvironments on the proteomes of Sca-1 + cells. The proteome component of freshly isolated Sca-1 + cells ( ex vivo ) was compared with that of Sca-1 + cells expanded in cell culture ( in vitro ). The analysis revealed significant differences in the protein abundances in the two conditions reflective of their functional variations. The identified proteins were enriched in various biological pathways. Notably, we identified proteins related to myotube differentiation, myotube cell development and myoblast fusion. We also identified a panel of cell surface marker proteins that can be leveraged in future to enrich Sca-1 + cells using combinatorial strategies. Comparative analysis implicated the activation of various pathways leading to increased protein synthesis under in vitro condition. We report here the most comprehensive proteome map of Sca-1 + cells that provides insights into the molecular networks operative in Sca-1 + cells. Importantly, through our work we generated the proteomic blueprint of protein abundances significantly altered in Sca-1 + cells under ex vivo and in vitro conditions. The curated data can also be visualized at https://yenepoya.res.in/database/Sca-1-Proteomics . Graphical Abstract
ISSN:2629-3269
2629-3277
DOI:10.1007/s12015-021-10134-w