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通过光化学固定聚苯乙烯和聚乙烯基吡咯烷酮对纤维连接蛋白生物黏附微图案进行描绘。

Delineating fibronectin bioadhesive micropatterns by photochemical immobilization of polystyrene and poly(vinylpyrrolidone).

机构信息

Laboratory for Surface Science and Technology, Department of Materials, ETH Zurich , Vladimir-Prelog-Weg 5, CH-8093, Zürich, Switzerland.

出版信息

ACS Appl Mater Interfaces. 2014;6(21):18683-92. doi: 10.1021/am5042093. Epub 2014 Oct 15.

Abstract

Bioadhesive micropatterns, capable of laterally confining cells to a 2D lattice, have proven effective in simulating the in vivo tissue environment. They reveal fundamental aspects of the role of adhesion in cell mechanics, proliferation, and differentiation. Here we present an approach based on photochemistry for the fabrication of synthetic polymer micropatterns. Perfluorophenyl azide (PFPA), upon deep-UV exposure, forms a reactive nitrene capable of covalently linking to a molecule that is in close proximity. PFPA has been grafted onto a backbone of poly(allyl amine), which readily forms a self-assembled monolayer on silicon wafers or glass. A film of polystyrene was applied by spin-coating, and by laterally confining the UV exposure through a chromium-on-quartz photomask, monolayers of polymers could be immobilized in circular microdomains. Poly(vinylpyrrolidone) (PVP) was attached to the background to form a barrier to nonspecific protein adsorption and cell adhesion. Micropatterns were characterized with high-lateral-resolution time-of-flight secondary ion mass spectrometry (TOF-SIMS), which confirmed the formation of polystyrene domains within a PVP background. Fluorescence-microscopy adsorption assays with rhodamine-labeled bovine serum albumin demonstrated the nonfouling efficiency of PVP and, combined with TOF-SIMS, allowed for a comprehensive characterization of the pattern geometry. The applicability of the micropatterned platform in single-cell assays was tested by culturing two cell types, WM 239 melanoma cells and SaOs-2 osteoblasts, on micropatterned glass, either with or without backfilling of the patterns with fibronectin. It was demonstrated that the platform was efficient in confining cells to the fibronectin-backfilled micropatterns for at least 48 h. PVP is thus proposed as a viable, highly stable alternative to poly(ethylene glycol) for nonfouling applications. Due to the versatility of the nitrene-insertion reaction, the platform could be extended to other polymer pairs or proteins and the surface chemistry adapted to specific applications.

摘要

生物粘附微图案能够将细胞横向限制在二维晶格中,已被证明可有效模拟体内组织环境。它们揭示了粘附在细胞力学、增殖和分化中的基本作用。本文介绍了一种基于光化学的合成聚合物微图案制造方法。全氟苯甲酰叠氮(PFPA)经深紫外光照射后形成反应性氮烯,能够与近距离的分子共价结合。PFPA 已嫁接到聚烯丙胺的主链上,该主链很容易在硅片或玻璃上自组装成单层。通过旋涂法施加聚苯乙烯膜,并通过铬/石英光掩模横向限制紫外光曝光,可以将聚合物单层固定在圆形微区中。将聚乙烯基吡咯烷酮(PVP)附着在背景上以形成非特异性蛋白质吸附和细胞附着的屏障。高横向分辨率飞行时间二次离子质谱(TOF-SIMS)对微图案进行了表征,证实了聚苯乙烯域在 PVP 背景中的形成。用罗丹明标记的牛血清白蛋白进行荧光显微镜吸附分析表明 PVP 的非污染效率,并与 TOF-SIMS 结合,可全面表征图案的几何形状。通过在微图案玻璃上培养两种细胞类型(WM 239 黑色素瘤细胞和 SaOs-2 成骨细胞),并在有或没有纤维连接蛋白填充图案的情况下,测试了微图案平台在单细胞分析中的适用性。结果表明,该平台能够有效地将细胞限制在纤维连接蛋白填充的微图案中至少 48 小时。因此,PVP 被提议作为非污染应用中聚乙二醇的可行、高度稳定的替代品。由于氮烯插入反应的多功能性,该平台可以扩展到其他聚合物对或蛋白质,并且可以根据特定应用调整表面化学。

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