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通过光模压图案化制备 3D 细胞水凝胶微结构。

Fabrication of 3D cell-laden hydrogel microstructures through photo-mold patterning.

机构信息

Department of Electronics, Information and Bioengineering, Politecnico di Milano, Milano, Italy.

出版信息

Biofabrication. 2013 Sep;5(3):035002. doi: 10.1088/1758-5082/5/3/035002. Epub 2013 May 20.

DOI:10.1088/1758-5082/5/3/035002
PMID:23685332
Abstract

Native tissues are characterized by spatially organized three-dimensional (3D) microscaled units which functionally define cells-cells and cells-extracellular matrix interactions. The ability to engineer biomimetic constructs mimicking these 3D microarchitectures is subject to the control over cell distribution and organization. In the present study we introduce a novel protocol to generate 3D cell laden hydrogel micropatterns with defined size and shape. The method, named photo-mold patterning (PMP), combines hydrogel micromolding within polydimethylsiloxane (PDMS) stamps and photopolymerization through a recently introduced biocompatible ultraviolet (UVA) activated photoinitiator (VA-086). Exploiting PDMS micromolds as geometrical constraints for two methacrylated prepolymers (polyethylene glycol diacrylate and gelatin methacrylate), micrometrically resolved structures were obtained within a 3 min exposure to a low cost and commercially available UVA LED. The PMP was validated both on a continuous cell line (human umbilical vein endothelial cells expressing green fluorescent protein, HUVEC GFP) and on primary human bone marrow stromal cells (BMSCs). HUVEC GFP and BMSCs were exposed to 1.5% w/v VA-086 and UVA light (1 W, 385 nm, distance from sample = 5 cm). Photocrosslinking conditions applied during the PMP did not negatively affect cells viability or specific metabolic activity. Quantitative analyses demonstrated the potentiality of PMP to uniformly embed viable cells within 3D microgels, creating biocompatible and favorable environments for cell proliferation and spreading during a seven days' culture. PMP can thus be considered as a promising and cost effective tool for designing spatially accurate in vitro models and, in perspective, functional constructs.

摘要

天然组织的特点是具有空间组织的三维(3D)微观单元,这些单元在功能上定义了细胞-细胞和细胞-细胞外基质的相互作用。能够工程仿生构建体来模拟这些 3D 微观结构的能力取决于对细胞分布和组织的控制。在本研究中,我们介绍了一种生成具有定义大小和形状的 3D 细胞负载水凝胶微图案的新方法。该方法称为光模图案化(PMP),它结合了聚二甲基硅氧烷(PDMS)印章内的水凝胶微成型和通过最近引入的生物相容性紫外线(UVA)激活光引发剂(VA-086)的光聚合。利用 PDMS 微模具作为两种甲基丙烯酰化预聚物(聚乙二醇二丙烯酸酯和明胶甲基丙烯酸酯)的几何约束,在 3 分钟内暴露于低成本且商业上可获得的 UVA LED 下,可获得微分辨率结构。PMP 不仅在连续细胞系(表达绿色荧光蛋白的人脐静脉内皮细胞,HUVEC GFP)上进行了验证,还在原代人骨髓基质细胞(BMSCs)上进行了验证。将 HUVEC GFP 和 BMSCs 暴露于 1.5%w/v VA-086 和 UVA 光(1 W,385nm,样品距离= 5cm)下。在 PMP 过程中应用的光交联条件不会对细胞活力或特定代谢活性产生负面影响。定量分析表明,PMP 具有将活细胞均匀嵌入 3D 微凝胶中的潜力,为细胞增殖和扩展创造了生物相容性和有利的环境,在七天的培养过程中。因此,PMP 可以被认为是设计空间精确的体外模型的有前途且具有成本效益的工具,并且在未来,可以设计功能性构建体。

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