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Production and Assessment of Decellularized Pig and Human Lung Scaffolds

去细胞化 弹性蛋白 细胞外基质 纤维连接蛋白 免疫细胞化学 病理 组织工程 化学 脚手架 层粘连蛋白 生物医学工程 解剖 医学 内科学 生物化学
作者
Joan E. Nichols,Jean A. Niles,Michael Riddle,Gracie Vargas,Tuya Schilagard,Liang Ma,Kert Edward,Saverio La Francesca,Jason Sakamoto,Stephanie P. Vega,Marie Ogadegbe,Ronald P. Mlcak,Donald J. Deyo,Lee C. Woodson,Christopher McQuitty,Scott D. Lick,Daniel L. Beckles,Esther Melo,Joaquin Cortiella
出处
期刊:Tissue Engineering Part A [Mary Ann Liebert, Inc.]
卷期号:19 (17-18): 2045-2062 被引量:160
标识
DOI:10.1089/ten.tea.2012.0250
摘要

The authors have previously shown that acellular (AC) trachea-lung scaffolds can (1) be produced from natural rat lungs, (2) retain critical components of the extracellular matrix (ECM) such as collagen-1 and elastin, and (3) be used to produce lung tissue after recellularization with murine embryonic stem cells. The aim of this study was to produce large (porcine or human) AC lung scaffolds to determine the feasibility of producing scaffolds with potential clinical applicability. We report here the first attempt to produce AC pig or human trachea-lung scaffold. Using a combination of freezing and sodium dodecyl sulfate washes, pig trachea-lungs and human trachea-lungs were decellularized. Once decellularization was complete we evaluated the structural integrity of the AC lung scaffolds using bronchoscopy, multiphoton microscopy (MPM), assessment of the ECM utilizing immunocytochemistry and evaluation of mechanics through the use of pulmonary function tests (PFTs). Immunocytochemistry indicated that there was loss of collagen type IV and laminin in the AC lung scaffold, but retention of collagen-1, elastin, and fibronectin in some regions. MPM scoring was also used to examine the AC lung scaffold ECM structure and to evaluate the amount of collagen I in normal and AC lung. MPM was used to examine the physical arrangement of collagen-1 and elastin in the pleura, distal lung, lung borders, and trachea or bronchi. MPM and bronchoscopy of trachea and lung tissues showed that no cells or cell debris remained in the AC scaffolds. PFT measurements of the trachea-lungs showed no relevant differences in peak pressure, dynamic or static compliance, and a nonrestricted flow pattern in AC compared to normal lungs. Although there were changes in content of collagen I and elastin this did not affect the mechanics of lung function as evidenced by normal PFT values. When repopulated with a variety of stem or adult cells including human adult primary alveolar epithelial type II cells both pig and human AC scaffolds supported cell attachment and cell viability. Examination of scaffolds produced using a variety of detergents indicated that detergent choice influenced human immune response in terms of T cell activation and chemokine production.
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