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成骨细胞和神经元在独特图案表面上的共培养。

Co-culture of osteocytes and neurons on a unique patterned surface.

机构信息

University of Delaware, Department of Biological Science, Newark, 19716, USA.

出版信息

Biointerphases. 2011 Dec;6(4):200-9. doi: 10.1116/1.3664050.

Abstract

Neural and skeletal communication is essential for the maintenance of bone mass and transmission of pain, yet the mechanism(s) of signal transduction between these tissues is unknown. The authors established a novel system to co-culture murine long bone osteocyte-like cells (MLO-Y4) and primary murine dorsal root ganglia (DRG) neurons. Assessment of morphology and maturation marker expression on perlecan domain IV peptide (PlnDIV) and collagen type-1 (Col1) demonstrated that PlnDIV was an optimal matrix for MLO-Y4 culture. A novel matrix-specificity competition assay was developed to expose these cells to several extracellular matrix proteins such as PlnDIV, Col1, and laminin (Ln). The competition assay showed that approximately 70% of MLO-Y4 cells preferred either PlnDIV or Col1 to Ln. To co-culture MLO-Y4 and DRG, we developed patterned surfaces using micro-contact printing to create 40 μm × 1 cm alternating stripes of PlnDIV and Ln or PlnDIV and Col1. Co-culture on PlnDIV/Ln surfaces demonstrated that these matrix molecules provided unique cues for each cell type, with MLO-Y4 preferentially attaching to the PlnDIV lanes and DRG neurons to the Ln lanes. Approximately 80% of DRG were localized to Ln. Cellular processes from MLO-Y4 were closely associated with axonal extensions of DRG neurons. Approximately 57% of neuronal processes were in close proximity to nearby MLO-Y4 cells at the PlnDIV-Ln interface. The surfaces in this new assay provided a unique model system with which to study the communication between osteocyte-like cells and neurons in an in vitro environment.

摘要

神经和骨骼的交流对于维持骨量和传递疼痛至关重要,但这些组织之间信号转导的机制尚不清楚。作者建立了一种新的共培养体系,用于培养鼠长骨骨细胞样细胞(MLO-Y4)和原代鼠背根神经节(DRG)神经元。通过对多配体蛋白聚糖域 IV 肽(PlnDIV)和胶原蛋白类型-1(Col1)的形态和成熟标志物表达的评估,表明 PlnDIV 是培养 MLO-Y4 的最佳基质。作者开发了一种新的基质特异性竞争测定法,使这些细胞能够接触到几种细胞外基质蛋白,如 PlnDIV、Col1 和层粘连蛋白(Ln)。竞争测定表明,大约 70%的 MLO-Y4 细胞更喜欢 PlnDIV 或 Col1 而不是 Ln。为了共培养 MLO-Y4 和 DRG,我们使用微接触印刷技术开发了图案化表面,以创建 40μm×1cm 的交替 PlnDIV 和 Ln 或 PlnDIV 和 Col1 条纹。在 PlnDIV/Ln 表面上的共培养表明,这些基质分子为每种细胞类型提供了独特的信号,MLO-Y4 优先附着在 PlnDIV 条带上,而 DRG 神经元则附着在 Ln 条带上。大约 80%的 DRG 位于 Ln 上。MLO-Y4 的细胞突起与 DRG 神经元的轴突延伸密切相关。大约 57%的神经元突起与 PlnDIV-Ln 界面附近的附近 MLO-Y4 细胞紧密接近。这个新测定中的表面提供了一个独特的模型系统,用于在体外环境中研究骨细胞样细胞和神经元之间的通信。

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