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用于细胞图案化的等离子体模板法

Plasma stencilling methods for cell patterning.

作者信息

Frimat Jean-Philippe, Menne Heike, Michels Antje, Kittel Silke, Kettler Raffael, Borgmann Sabine, Franzke Joachim, West Jonathan

机构信息

Institute for Analytical Sciences, Bunsen-Kirchhoff-Str. 11, 44139, Dortmund, Germany.

出版信息

Anal Bioanal Chem. 2009 Oct;395(3):601-9. doi: 10.1007/s00216-009-2824-7. Epub 2009 May 17.

Abstract

In this paper we describe plasma stencilling techniques for patterning 10 mammalian cell lines on hydrophobic and cell repellent poly(dimethylsiloxane) (PDMS), methylated glass and bacterial grade polystyrene surfaces. An air plasma produced with a Tesla generator operating at atmospheric pressure was used with microengineered stencils for patterned surface oxidation, selectively transforming the surface to a hydrophilic state to enable cell adhesion and growth. Plasma stencilling obviates the need for directly patterning cell adhesion molecules. Instead, during cell culture, adhesion proteins from the media assemble in a bioactive form on the hydrophilic regions. Critically, the removal of protein patterning prior to cell culture provides the option to also use PDMS-PDMS plasma bonding to incorporate cell patterns within microfluidic systems. Linear patterns were generated using PDMS microchannel stencils, and polyimide stencils with through holes were used for the production of cellular arrays. For the production of smaller cellular arrays, a novel microcapillary-based dielectric barrier discharge system was developed. A numerical method to characterise the cell patterns is also introduced and was used to demonstrate that plasma stencilling is highly effective, with complete patterns confined during long term cell culture (>10 days). In summary, plasma stencilling is simple, rapid, inexpensive, reproducible and a potentially universal cell line patterning capability.

摘要

在本文中,我们描述了用于在疏水性和细胞排斥性的聚二甲基硅氧烷(PDMS)、甲基化玻璃和细菌级聚苯乙烯表面上对10种哺乳动物细胞系进行图案化的等离子体模板技术。使用由在大气压下运行的特斯拉发生器产生的空气等离子体与微工程模板进行图案化表面氧化,将表面选择性地转变为亲水性状态,以实现细胞粘附和生长。等离子体模板技术无需直接对细胞粘附分子进行图案化。相反,在细胞培养过程中,培养基中的粘附蛋白以生物活性形式聚集在亲水性区域。至关重要的是,在细胞培养前去除蛋白质图案化提供了还可使用PDMS-PDMS等离子体键合将细胞图案整合到微流体系统中的选择。使用PDMS微通道模板生成线性图案,带有通孔的聚酰亚胺模板用于制作细胞阵列。为了制作更小的细胞阵列,开发了一种基于新型微毛细管的介质阻挡放电系统。还介绍了一种表征细胞图案的数值方法,并用于证明等离子体模板技术非常有效,在长期细胞培养(>10天)期间图案完整受限。总之,等离子体模板技术简单、快速、廉价、可重复,并且具有潜在的通用细胞系图案化能力。

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