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新型凋亡辅助肺组织脱细胞方法的开发。

Development of novel apoptosis-assisted lung tissue decellularization methods.

机构信息

J. Crayton Pruitt Family Department of Biomedical Engineering, University of Florida, Gainesville, FL, USA.

出版信息

Biomater Sci. 2021 May 4;9(9):3485-3498. doi: 10.1039/d1bm00032b.

DOI:10.1039/d1bm00032b
PMID:33949462
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.

摘要

去细胞组织在再生医学和疾病建模应用中具有巨大的潜力。无细胞细胞外基质 (ECM) 丰富的支架可以在移植前用患者来源的细胞再细胞化,也可以消化以创建用于 3D 细胞培养的热凝胶 ECM 水凝胶。目前使用去污剂清除细胞成分的去细胞化方法会导致 ECM 蛋白和组织结构完整性的丧失。最近,一种利用细胞凋亡来去除切除的鼠坐骨神经的替代方法导致 ECM 保存、细胞去除和体内免疫耐受效果更好。然而,这种凋亡辅助的去细胞化方法尚未针对具有更复杂几何形状的其他组织(如肺)进行优化。为此,我们开发了一种使用喜树碱和磺基甜菜碱-10 (SB-10) 的组合来诱导细胞凋亡并分别促进温和有效地去除细胞碎片的凋亡辅助肺组织去细胞化方法。重要的是,与单独使用任一种药物相比,两种药物的组合导致细胞去除和 ECM 保存效果更好,这可能是由于肺表面活性剂的存在。此外,与以前建立的基于去污剂的去细胞化方案相比,我们的方法在细胞去除方面更具优势。此外,热凝胶肺 ECM 水凝胶在培养中支持大鼠肺上皮细胞长达 2 周的高活力。这项工作表明,基于细胞凋亡的肺组织去细胞化是一种优越的技术,值得进一步用于再生医学和疾病建模目的。

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