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无细胞正常和纤维化人肺基质作为体外研究的培养系统。

Acellular normal and fibrotic human lung matrices as a culture system for in vitro investigation.

机构信息

Division of Pulmonary and Critical Care Medicine, University of Michigan Medical School, 1150 West Medical Center Drive, Ann Arbor, MI 48109-5642, USA.

出版信息

Am J Respir Crit Care Med. 2012 Nov 1;186(9):866-76. doi: 10.1164/rccm.201204-0754OC. Epub 2012 Aug 30.

Abstract

RATIONALE

Extracellular matrix (ECM) is a dynamic tissue that contributes to organ integrity and function, and its regulation of cell phenotype is a major aspect of cell biology. However, standard in vitro culture approaches are of unclear physiologic relevance because they do not mimic the compositional, architectural, or distensible nature of a living organ. In the lung, fibroblasts exist in ECM-rich interstitial spaces and are key effectors of lung fibrogenesis.

OBJECTIVES

To better address how ECM influences fibroblast phenotype in a disease-specific manner, we developed a culture system using acellular human normal and fibrotic lungs.

METHODS

Decellularization was achieved using treatment with detergents, salts, and DNase. The resultant matrices can be sectioned as uniform slices within which cells were cultured.

MEASUREMENTS AND MAIN RESULTS

We report that the decellularization process effectively removes cellular and nuclear material while retaining native dimensionality and stiffness of lung tissue. We demonstrate that lung fibroblasts reseeded into acellular lung matrices can be subsequently assayed using conventional protocols; in this manner we show that fibrotic matrices clearly promote transforming growth factor-β-independent myofibroblast differentiation compared with normal matrices. Furthermore, comprehensive analysis of acellular matrix ECM details significant compositional differences between normal and fibrotic lungs, paving the way for further study of novel hypotheses.

CONCLUSIONS

This methodology is expected to allow investigation of important ECM-based hypotheses in human tissues and permits future scientific exploration in an organ- and disease-specific manner.

摘要

背景

细胞外基质(ECM)是一种动态组织,有助于器官的完整性和功能,其对细胞表型的调节是细胞生物学的主要方面。然而,由于标准的体外培养方法不能模拟活器官的组成、结构或可伸展性,因此其生理相关性尚不清楚。在肺部,成纤维细胞存在于富含细胞外基质的细胞外间质中,是肺纤维化发生的关键效应细胞。

目的

为了更好地研究 ECM 如何以特定于疾病的方式影响成纤维细胞表型,我们开发了一种使用去细胞化的人正常和纤维化肺的培养系统。

方法

使用去污剂、盐和 DNA 酶处理来实现去细胞化。得到的基质可以切成均匀的薄片,在薄片内培养细胞。

测量和主要结果

我们报告称,去细胞化过程有效地去除了细胞和核材料,同时保留了肺组织的原始维度和硬度。我们证明,重新接种到去细胞化肺基质中的肺成纤维细胞可以使用常规方案进行后续分析;通过这种方式,我们表明与正常基质相比,纤维化基质明显促进了转化生长因子-β 非依赖性肌成纤维细胞分化。此外,对去细胞化基质细胞外基质的综合分析显示正常和纤维化肺之间存在显著的组成差异,为进一步研究新的假说铺平了道路。

结论

该方法有望允许在人体组织中研究基于 ECM 的重要假说,并允许以器官和疾病特异性的方式进行未来的科学探索。

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