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在无血清培养基中使用玻连蛋白作为生长底物对C2C12肌管进行光刻图案化处理。

Photolithographic patterning of C2C12 myotubes using vitronectin as growth substrate in serum-free medium.

作者信息

Molnar Peter, Wang Weishi, Natarajan Anupama, Rumsey John W, Hickman James J

机构信息

Nanoscience Technology Center, University of Central Florida, 12424 Research Parkway, Suite 400, Orlando, Florida 32826, USA.

出版信息

Biotechnol Prog. 2007 Jan-Feb;23(1):265-8. doi: 10.1021/bp060302q.

Abstract

The C2C12 cell line is frequently used as a model of skeletal muscle differentiation. In our serum-free defined culture system, differentiation of C2C12 cells into myotubes required surface-bound signals such as substrate-adsorbed vitronectin or laminin. On the basis of this substrate requirement of myotube formation, we developed a photolithography-based method to pattern C2C12 myotubes, where myotubes formed exclusively on vitronectin surface patterns. We have determined that the optimal line width to form single myotubes is approximately 30 mum. To illustrate a possible application of this method, we patterned myotubes on the top of commercial substrate-embedded microelectrodes. In contrast to previous experiments where cell patterning was achieved by selective attachment of the cells to patterned surfaces in a medium that contained all of the factors necessary for differentiation, this study illustrates that surface patterning of a signaling molecule, which is essential for skeletal muscle differentiation in a defined system, can result in the formation of aligned myotubes on the patterns. This technique is being developed for applications in cell biology, tissue engineering, and robotics.

摘要

C2C12细胞系经常被用作骨骼肌分化的模型。在我们无血清的特定培养体系中,C2C12细胞分化为肌管需要表面结合信号,如底物吸附的玻连蛋白或层粘连蛋白。基于肌管形成对这种底物的需求,我们开发了一种基于光刻的方法来对C2C12肌管进行图案化,其中肌管仅在玻连蛋白表面图案上形成。我们已经确定形成单个肌管的最佳线宽约为30微米。为了说明该方法的一种可能应用,我们在商业底物嵌入微电极的顶部对肌管进行了图案化。与之前通过在含有分化所需所有因子的培养基中将细胞选择性附着到图案化表面来实现细胞图案化的实验不同,本研究表明,在特定体系中对骨骼肌分化至关重要的信号分子进行表面图案化,可导致在图案上形成排列整齐的肌管。这项技术正在被开发用于细胞生物学、组织工程和机器人技术等领域。

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