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一种适用于长期神经培养的多功能蛋白质和细胞图案化方法。

A Versatile Protein and Cell Patterning Method Suitable for Long-Term Neural Cultures.

机构信息

Laboratory of Biosensors and Bioelectronics , ETH Zurich , Gloriastrasse 35 , 8092 Zurich , Switzerland.

Department of Chemical Engineering, Graduate School of Engineering , Kyushu University , 744 Motooka , Nishi-ku, Fukuoka 819-0395 , Japan.

出版信息

Langmuir. 2019 Feb 26;35(8):2966-2975. doi: 10.1021/acs.langmuir.8b03730. Epub 2019 Feb 15.

DOI:10.1021/acs.langmuir.8b03730
PMID:30767535
Abstract

Herein, we present an easy-to-use protein and cell patterning method relying solely on pipetting, rinsing steps and illumination with a desktop lamp, which does not require any expensive laboratory equipment, custom-built hardware or delicate chemistry. This method is based on the adhesion promoter poly(allylamine)-grafted perfluorophenyl azide, which allows UV-induced cross-linking with proteins and the antifouling molecule poly(vinylpyrrolidone). Versatility is demonstrated by creating patterns with two different proteins and a polysaccharide directly on plastic well plates and on glass slides, and by subsequently seeding primary neurons and C2C12 myoblasts on the patterns to form islands and mini-networks. Patterning characterization is done via immunohistochemistry, Congo red staining, ellipsometry, and infrared spectroscopy. Using a pragmatic setup, patterning contrasts down to 5 μm and statistically significant long-term stability superior to the gold standard poly(l-lysine)-grafted poly(ethylene glycol) could be obtained. This simple method can be used in any laboratory or even in classrooms and its outstanding stability is especially interesting for long-term cell experiments, e.g., for bottom-up neuroscience, where well-defined microislands and microcircuits of primary neurons are studied over weeks.

摘要

在这里,我们提出了一种简单易用的蛋白质和细胞图案化方法,仅依赖于移液、冲洗步骤和台式灯的照射,不需要任何昂贵的实验室设备、定制的硬件或精细的化学物质。该方法基于粘附促进剂聚(烯丙胺)接枝全氟苯基叠氮化物,它允许与蛋白质和抗污分子聚(乙烯基吡咯烷酮)进行 UV 诱导交联。通过直接在塑料孔板和载玻片上用两种不同的蛋白质和多糖形成图案,并随后在图案上接种原代神经元和 C2C12 成肌细胞形成岛和迷你网络,展示了其多功能性。通过免疫组织化学、刚果红染色、椭圆偏振术和红外光谱对图案化进行了表征。使用实用的设置,可以获得低至 5 μm 的图案对比度和优于金标准聚(L-赖氨酸)接枝聚(乙二醇)的统计学上显著的长期稳定性。这种简单的方法可以在任何实验室甚至教室中使用,其出色的稳定性特别适用于长期细胞实验,例如用于自下而上的神经科学,其中研究原代神经元的明确定义的微岛和微电路超过数周。

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