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微流控灌注培养过程中微珠引导的三维骨细胞网络重建

Microbeads-Guided Reconstruction of 3D Osteocyte Network during Microfluidic Perfusion Culture.

作者信息

Gu Yexin, Zhang Wenting, Sun Qiaoling, Hao Yi, Zilberberg Jenny, Lee Woo Y

机构信息

Department of Chemical Engineering and Materials Science, Stevens Institute of Technology, 1 Castle Point on Hudson, Hoboken, New Jersey, 07030, USA.

Department of Research, Hackensack University Medical Center, 40 Prospect Avenue, Hackensack, New Jersey, 07601, USA.

出版信息

J Mater Chem B. 2015 May 7;3(17):3625-3633. doi: 10.1039/C5TB00421G. Epub 2015 Mar 25.

Abstract

Osteocytes reside as 3-dimensionally networked cells in the lacunocanalicular structure of bones, and function as the master regulators of homeostatic bone remodeling. We report here, for the first time to our best knowledge, the use of a biomimetic approach to reconstruct the 3D osteocyte network with physiological relevant microscale dimensions. In this approach, biphasic calcium phosphate microbeads were assembled with murine early osteocytes (MLO-A5) to provide an initial mechanical framework for 3D network formation and maintenance during long-term perfusion culture in a microfluidic chamber. The microbead size of 20-25 μm was used to: (1) facilitate a single cell to be placed within the interstitial space between the microbeads, (2) mitigate the proliferation of the entrapped cell due to its physical confinement in the interstitial site, and (3) control cell-to-cell distance to be 20-25 μm as observed in murine bones. The entrapped cells formed a 3D cellular network by extending and connecting their processes through openings between the microbeads within 3 days of culture. The entrapped cells produced significant mineralized extracellular matrix to fill up the interstitial spaces, resulting in the formation of a dense tissue structure during the course of 3-week culture. We found that the time-dependent osteocytic transitions of the cells exhibited trends consistent with in vivo observations, particularly with high expression of Sost gene, which is a key osteocyte-specific marker for the mechanotransduction function of osteocytes. In contrast, cells cultured in 2D well-plates did not replicate in vivo trends. These results provide an important new insight in building physiologically relevant in vitro bone tissue models.

摘要

骨细胞以三维网络状细胞的形式存在于骨的骨陷窝-骨小管结构中,是骨稳态重塑的主要调节者。据我们所知,我们首次报道了使用一种仿生方法来重建具有生理相关微观尺度的三维骨细胞网络。在这种方法中,将双相磷酸钙微珠与小鼠早期骨细胞(MLO-A5)组装在一起,为在微流控腔室中长期灌注培养期间三维网络的形成和维持提供初始机械框架。使用20-25μm的微珠尺寸是为了:(1)便于将单个细胞放置在微珠之间的间隙空间内;(2)减轻被困细胞由于其在间隙部位的物理限制而导致的增殖;(3)将细胞间距离控制在20-25μm,这与在小鼠骨骼中观察到的情况一致。被困细胞在培养3天内通过其突起延伸并通过微珠之间的开口连接形成三维细胞网络。被困细胞产生大量矿化的细胞外基质以填充间隙空间,从而在3周的培养过程中形成致密的组织结构。我们发现细胞随时间的骨细胞转变表现出与体内观察结果一致的趋势,特别是Sost基因的高表达,Sost基因是骨细胞机械转导功能的关键骨细胞特异性标志物。相比之下,在二维孔板中培养的细胞没有重现体内趋势。这些结果为构建生理相关的体外骨组织模型提供了重要的新见解。

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