AI Article Synopsis

  • Decellularized tissues can be used in regenerative medicine and disease modeling by removing cells from tissues while preserving their structure.
  • Recent techniques using apoptosis for decellularization have shown to better maintain the extracellular matrix compared to traditional detergent methods, especially in murine sciatic nerves.
  • A new apoptosis-assisted method for lung tissue decellularization was developed using camptothecin and sulfobetaine-10, resulting in more effective cell removal and ECM preservation, and supporting healthy cell growth in culture.

Article Abstract

Decellularized tissues hold great potential for both regenerative medicine and disease modeling applications. The acellular extracellular matrix (ECM)-enriched scaffolds can be recellularized with patient-derived cells prior to transplantation, or digested to create thermally-gelling ECM hydrogels for 3D cell culture. Current methods of decellularization clear cellular components using detergents, which can result in loss of ECM proteins and tissue architectural integrity. Recently, an alternative approach utilizing apoptosis to decellularize excised murine sciatic nerves resulted in superior ECM preservation, cell removal, and immune tolerance in vivo. However, this apoptosis-assisted decellularization approach has not been optimized for other tissues with a more complex geometry, such as lungs. To this end, we developed an apoptosis-assisted lung tissue decellularization method using a combination of camptothecin and sulfobetaine-10 (SB-10) to induce apoptosis and facilitate gentle and effective removal of cell debris, respectively. Importantly, combination of the two agents resulted in superior cell removal and ECM preservation compared to either of the treatments alone, presumably because of pulmonary surfactants. In addition, our method was superior in cell removal compared to a previously established detergent-based decellularization protocol. Furthermore, thermally-gelling lung ECM hydrogels supported high viability of rat lung epithelial cells for up to 2 weeks in culture. This work demonstrates that apoptosis-based lung tissue decellularization is a superior technique that warrants further utilization for both regenerative medicine and disease modeling purposes.

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Source
http://dx.doi.org/10.1039/d1bm00032bDOI Listing

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