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微接触印刷和微点样作为直接在等离子体沉积的聚乙烯氧化物上进行蛋白质图案化的方法:在干细胞图案化中的应用。

Microcontact printing and microspotting as methods for direct protein patterning on plasma deposited polyethylene oxide: application to stem cell patterning.

机构信息

European Commission, Joint Research Centre, Institute for Health and Consumer Protection, TP 203, Via Fermi, 21027 Ispra, VA, Italy.

出版信息

Biomed Microdevices. 2013 Jun;15(3):495-507. doi: 10.1007/s10544-013-9749-9.

DOI:10.1007/s10544-013-9749-9
PMID:23404262
Abstract

Two methods for protein patterning on antifouling surfaces have been applied to analyze the density and bioactivity of the proteins after deposition. Microcontact printing has been used as a technique to transfer fibronectin through conformal contact, while piezoelectric deposition has been employed as a non-contact technique for producing arrays of fibronectin (FN). Plasma deposited polyethylene oxide-like (PEO-like) films have been used as non-fouling background to achieve the bioadhesive/biorepellent surface contrast. Both patterning methods allow the direct fabrication of protein arrays on a non-fouling substrate, and the subsequent formation of a pattern of stem cells by cell attachment on the arrayed substrates. Microcontact printing produced fully packed homogeneous fibronectin patterns, much denser than microspotted patterns. Both printing and spotting technologies generated functional protein arrays, their bioactivity being primarily modulated by the density of the deposited protein layer. Optimization of the FN parameters used for deposition has lead to the achievement of high-quality microarrays with large population of neural stem cells immobilized in the patterns in serum-free conditions, where cells exhibit a more homogeneous starting population and factors influencing fate decisions can be more easily tracked. The immunorecognition of fibronectin targeted antibodies, as well as the cell density, increase with the protein density up to a saturation point. Over 100 ng/cm² of fibronectin on the surface leads to a decrease in the number of attached cells and a raise of cell spreading.

摘要

已经应用了两种蛋白质图案化方法在抗污表面上,以分析沉积后蛋白质的密度和生物活性。微接触印刷已被用作通过共形接触转移纤连蛋白的技术,而压电沉积已被用作产生纤连蛋白(FN)阵列的非接触技术。等离子体沉积的聚氧化乙烯类(PEO 类)薄膜已被用作非粘性背景,以实现生物粘附/抗生物表面对比。这两种图案化方法都允许在非粘性基底上直接制备蛋白质阵列,并通过在阵列基底上的细胞附着形成干细胞图案。微接触印刷产生了完全填充的均匀纤连蛋白图案,比微点图案密集得多。印刷和点样技术都产生了功能性蛋白质阵列,其生物活性主要由沉积蛋白质层的密度来调节。优化用于沉积的 FN 参数导致在无血清条件下在图案中固定大量神经干细胞的高质量微阵列的实现,其中细胞表现出更均匀的起始群体,并且可以更容易地跟踪影响命运决策的因素。针对纤连蛋白的靶向抗体的免疫识别以及细胞密度随着蛋白质密度的增加而增加,直到达到饱和点。表面上超过 100ng/cm²的纤连蛋白会导致附着细胞数量减少和细胞铺展增加。

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