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仿生基底的设计用于长期维持肺泡上皮细胞。

Design of biomimetic substrates for long-term maintenance of alveolar epithelial cells.

机构信息

Institute of Biomaterials & Biomedical Engineering, University of Toronto, 200 College St., Toronto, ON M5S 3E5, Canada.

出版信息

Biomater Sci. 2018 Jan 30;6(2):292-303. doi: 10.1039/c7bm00647k.

Abstract

There is a need to establish in vitro lung alveolar epithelial culture models to better understand the fundamental biological mechanisms that drive lung diseases. While primary alveolar epithelial cells (AEC) are a useful option to study mature lung biology, they have limited utility in vitro. Cells that survive demonstrate limited proliferative capacity and loss of phenotype over the first 3-5 days in traditional culture conditions. To address this limitation, we generated a novel physiologically relevant cell culture system for enhanced viability and maintenance of phenotype. Here we describe a method utilizing e-beam lithography, reactive ion etching, and replica molding to generate poly-dimethylsiloxane (PDMS) substrates containing hemispherical cavities that mimic the architecture and size of mouse and human alveoli. Primary AECs grown on these cavity-containing substrates form a monolayer that conforms to the substrate enabling precise control over cell sheet architecture. AECs grown in cavity culture conditions remain viable and maintain their phenotype over one week. Specifically, cells grown on substrates consisting of 50 μm diameter cavities remained 96 ± 4% viable and maintained expression of surfactant protein C (SPC), a marker of type 2 AEC over 7 days. While this report focuses on primary lung alveolar epithelial cells, our culture platform is potentially relevant and useful for growing primary cells from other tissues with similar cavity-like architecture and could be further adapted to other biomimetic shapes or contours.

摘要

需要建立体外肺肺泡上皮细胞培养模型,以更好地理解驱动肺部疾病的基本生物学机制。虽然原代肺泡上皮细胞(AEC)是研究成熟肺部生物学的有用选择,但它们在体外的应用有限。在传统培养条件下,存活的细胞表现出有限的增殖能力和表型丧失,在第 3-5 天内。为了解决这个限制,我们生成了一种新的生理相关细胞培养系统,以提高细胞活力和维持表型。在这里,我们描述了一种利用电子束光刻、反应离子刻蚀和复制成型来生成含有半球形腔的聚二甲基硅氧烷(PDMS)基底的方法,这些腔模拟了小鼠和人类肺泡的结构和大小。在这些含有腔的基底上生长的原代 AEC 形成一层符合基底的单层,从而可以精确控制细胞片层结构。在腔培养条件下生长的 AEC 保持活力并保持其表型超过一周。具体来说,在直径为 50μm 的腔组成的基底上生长的细胞保持 96±4%的活力,并在 7 天内维持表面活性蛋白 C(SPC)的表达,这是 2 型 AEC 的标志物。虽然本报告重点介绍了原代肺肺泡上皮细胞,但我们的培养平台对于生长具有类似腔样结构的其他组织的原代细胞具有潜在的相关性和实用性,并且可以进一步适应其他仿生形状或轮廓。

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