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Nanowell-Based Immunoassays for Measuring Single-Cell Secretion: Characterization of Transport and Surface Binding

机译:基于纳米纤维的免疫测定法测定单细胞分泌:运输和表面结合的表征

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摘要

Arrays of subnanoliter wells (nanowells) provide a useful system to isolate single cells and analyze their secreted proteins. Two general approaches have emerged: one that uses open arrays and local capture of secreted proteins, and a second (called microengraving) that relies on closed arrays to capture secreted proteins on a solid substrate, which is subsequently removed from the array. However, the design and operating parameters for efficient capture from these two approaches to analyze single-cell secretion have not been extensively considered. Using numerical simulations, we analyzed the operational envelope for both open and closed formats, as a function of the spatial distribution of capture ligands, their affinities for the protein, and the rates of single-cell secretion. Based on these analyses, we present a modified approach to capture secreted proteins in-well for highly active secreting cells. This simple method for in-well detection should facilitate rapid identification of cell lines with high specific productivities.
机译:亚纳升孔的阵列(纳孔)为分离单个细胞并分析其分泌的蛋白质提供了有用的系统。已经出现了两种通用方法:一种使用开放阵列和分泌蛋白的局部捕获,第二种(称为微雕刻)依靠封闭的阵列捕获固体基质上的分泌蛋白,随后将其从阵列中去除。但是,尚未广泛考虑从这两种分析单细胞分泌物的方法中有效捕获的设计和操作参数。使用数值模拟,我们根据捕获配体的空间分布,它们对蛋白质的亲和力以及单细胞分泌率来分析开放和封闭形式的操作范围。基于这些分析,我们提出了一种改进的方法来捕获孔中的高活性分泌细胞的分泌蛋白。这种用于孔内检测的简单方法应有助于快速鉴定具有高比生产率的细胞系。

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