Scarritt Michelle E, Bonvillain Ryan W, Burkett Brian J, Wang Guangdi, Glotser Elana Y, Zhang Qiang, Sammarco Mimi C, Betancourt Aline M, Sullivan Deborah E, Bunnell Bruce A
1 Center for Stem Cell Research and Regenerative Medicine, Tulane University School of Medicine , New Orleans, Louisiana.
Tissue Eng Part A. 2014 May;20(9-10):1426-43. doi: 10.1089/ten.TEA.2013.0438. Epub 2014 Feb 28.
There are an insufficient number of donor organs available to meet the demand for lung transplantation. This issue could be addressed by regenerating functional tissue from diseased or damaged lungs that would otherwise be deemed unsuitable for transplant. Detergent-mediated whole-lung decellularization produces a three-dimensional natural scaffold that can be repopulated with various cell types. In this study, we investigated the decellularization and initial recellularization of diseased lungs using a rat model of monocrotaline-induced pulmonary hypertension (MCT-PHT). Decellularization of control and MCT-PHT Sprague-Dawley rat lungs was accomplished by treating the lungs with a combination of Triton X-100, sodium deoxycholate, NaCl, and DNase. The resulting acellular matrices were characterized by DNA quantification, Western blotting, immunohistochemistry, and proteomic analyses revealing that decellularization was able to remove cells while leaving the extracellular matrix (ECM) components and lung ultrastructure intact. Decellularization significantly reduced DNA content (∼30-fold in MCT-PHT lungs and ∼50-fold in the control lungs) and enriched ECM components (>60-fold in both the control and MCT-PHT lungs) while depleting cellular proteins. MicroCT visualization of MCT-PHT rat lungs indicated that the vasculature was narrowed as a result of MCT treatment, and this characteristic was unchanged by decellularization. Mean arterial vessel diameter of representative decellularized MCT-PHT and control scaffolds was estimated to be 0.152±0.134 mm and 0.247±0.160 mm, respectively. Decellularized MCT-PHT lung scaffolds supported attachment and survival of rat adipose-derived stem cells (rASCs), seeded into the airspace or the vasculature, for at least 2 weeks. The cells seeded in MCT-PHT lung scaffolds proliferated and underwent apoptosis similar to control scaffolds; however, the initial percentage of apoptotic cells was slightly higher in MCT-PHT lungs (2.79±2.03% vs. 1.05±1.02% of airway-seeded rASCs, and 4.47±1.21% vs. 2.66±0.10% of vascular seeded rASCs). The ECM of cell-seeded scaffolds showed no signs of degradation by the cells after 14 days in culture. These data suggest that diseased hypertensive lungs can be efficiently decellularized similar to control lungs and have the potential to be recellularized with mesenchymal stem cells with the ultimate goal of generating healthy, functional pulmonary tissue.
可用于肺移植的供体器官数量不足,无法满足需求。这个问题可以通过从患病或受损的肺中再生功能性组织来解决,否则这些肺将被认为不适合移植。去污剂介导的全肺脱细胞处理产生一种三维天然支架,可重新填充各种细胞类型。在本研究中,我们使用单氰胺诱导的肺动脉高压(MCT-PHT)大鼠模型研究了患病肺的脱细胞和初始再细胞化过程。通过用Triton X-100、脱氧胆酸钠、NaCl和DNase的组合处理肺,实现了对照和MCT-PHT Sprague-Dawley大鼠肺的脱细胞。通过DNA定量、蛋白质印迹、免疫组织化学和蛋白质组学分析对所得的无细胞基质进行表征,结果表明脱细胞能够去除细胞,同时使细胞外基质(ECM)成分和肺超微结构保持完整。脱细胞显著降低了DNA含量(MCT-PHT肺中约为30倍,对照肺中约为50倍),富集了ECM成分(对照和MCT-PHT肺中均超过60倍),同时消耗了细胞蛋白。MCT-PHT大鼠肺的MicroCT可视化显示,由于MCT处理,血管变窄,并且这种特征在脱细胞后没有改变。代表性的脱细胞MCT-PHT和对照支架的平均动脉血管直径估计分别为0.152±0.134毫米和0.247±0.160毫米。脱细胞的MCT-PHT肺支架支持接种到气腔或血管中的大鼠脂肪来源干细胞(rASCs)附着和存活至少2周。接种在MCT-PHT肺支架中的细胞增殖并经历凋亡,与对照支架相似;然而,MCT-PHT肺中凋亡细胞的初始百分比略高(气道接种的rASCs中为2.79±2.03%对1.05±1.02%,血管接种的rASCs中为4.47±1.21%对2.66±0.10%)。培养14天后,接种细胞的支架的ECM没有显示出被细胞降解的迹象。这些数据表明,患病的高血压肺可以像对照肺一样有效地进行脱细胞处理,并且有潜力用间充质干细胞进行再细胞化,最终目标是生成健康、功能性的肺组织。
