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基于清洁剂的小鼠肺去细胞化和再细胞化方案的比较评估。

Comparative assessment of detergent-based protocols for mouse lung de-cellularization and re-cellularization.

机构信息

Department of Medicine, University of Vermont College of Medicine, Burlington, Vermont, USA.

出版信息

Tissue Eng Part C Methods. 2012 Jun;18(6):420-32. doi: 10.1089/ten.tec.2011.0567. Epub 2012 Jan 26.

Abstract

Several different detergent-based methods are currently being explored for de-cellularizing whole lungs for subsequent use as three-dimensional scaffolds for ex vivo lung tissue generation. However, it is not yet clear which of these methods may provide a scaffold that best supports re-cellularization and generation of functional lung tissue. Notably, the detergents used for de-cellularization activate matrix metalloproteinases that can potentially degrade extracellular matrix (ECM) proteins important for subsequent binding and growth of cells inoculated into the de-cellularized scaffolds. We assessed gelatinase activation and the histologic appearance, protein composition, and lung mechanics of the end product scaffolds produced with three different detergent-based de-cellularization methods utilizing either Triton-X 100/sodium deoxycholate (Triton/SDC), sodium dodecyl sulfate (SDS), or 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS). There were significant differences both in gelatinase activation and in the retention of ECM and other intracellular proteins, assessed by immunohistochemistry, mass spectrometry, and western blotting as well as in airways resistance and elastance of lungs de-cellularized with the different methods. However, despite these differences, binding and initial growth following intratracheal inoculation with either bone marrow-derived mesenchymal stromal cells or with C10 mouse lung epithelial cells was similar between lungs de-cellularized with each method. Therefore despite differences in the structural composition of the de-cellularized lungs, initial re-cellularization does not appear significantly different between the three de-cellularization approaches studied.

摘要

目前,人们正在探索几种基于去污剂的方法来去除整个肺的细胞,以便随后将其用作三维支架,用于体外肺组织的生成。然而,目前尚不清楚这些方法中的哪一种可能提供最适合支持再细胞化和功能性肺组织生成的支架。值得注意的是,用于去细胞化的去污剂会激活基质金属蛋白酶,这些酶可能会降解对于随后接种到去细胞化支架中的细胞的结合和生长很重要的细胞外基质(ECM)蛋白。我们评估了三种不同的基于去污剂的去细胞化方法中使用的三种不同的去污剂(Triton-X 100/脱氧胆酸钠(Triton/SDC)、十二烷基硫酸钠(SDS)或 3-[[3-(胆酰胺丙基)二甲氨基]丙基]-1-丙磺酸盐(CHAPS))产生的终产物支架的明胶酶激活以及组织学外观、蛋白质组成和肺力学。在通过免疫组织化学、质谱和 Western blot 评估明胶酶激活以及 ECM 和其他细胞内蛋白质的保留情况以及通过不同方法去细胞化的肺的气道阻力和弹性方面,均存在显著差异。然而,尽管存在这些差异,但在用每种方法去细胞化的肺中,经气管内接种骨髓间充质基质细胞或 C10 小鼠肺上皮细胞后的结合和初始生长是相似的。因此,尽管去细胞化肺的结构组成存在差异,但在研究的三种去细胞化方法之间,初始再细胞化似乎没有显著差异。

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