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An open-pattern droplet-in-oil planar array for single cell analysis based on sequential inkjet printing technology

机译:一种基于顺序喷墨打印技术的开放式油滴液滴平面阵列用于单细胞分析

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摘要

Cellular heterogeneity represents a fundamental principle of cell biology for which a readily available single-cell research tool is urgently required. Here, we present a novel method combining cell-sized well arrays with sequential inkjet printing. Briefly, K562 cells with phosphate buffer saline buffer were captured at high efficiency (74.5%) in a cell-sized well as a “primary droplet” and sealed using fluorinated oil. Then, piezoelectric inkjet printing technology was adapted to precisely inject the cell lysis buffer and the fluorogenic substrate, fluorescein-di-β-D-galactopyranoside, as a “secondary droplet” to penetrate the sealing oil and fuse with the “primary droplet.” We thereby successfully measured the intracellular β-galactosidase activity of K562 cells at the single-cell level. Our method allows, for the first time, the ability to simultaneously accommodate the high occupancy rate of single cells and sequential addition of reagents while retaining an open structure. We believe that the feasibility and flexibility of our method will enhance its use as a universal single-cell research tool as well as accelerate the adoption of inkjet printing in the study of cellular heterogeneity.
机译:细胞异质性代表了细胞生物学的基本原理,为此迫切需要一种容易获得的单细胞研究工具。在这里,我们提出了一种新颖的方法,将细胞大小的孔阵列与顺序喷墨打印相结合。简而言之,将具有磷酸盐缓冲液盐水缓冲液的K562细胞高效(74.5%)捕获在细胞大小的孔中,称为“主要液滴”,并使用氟化油密封。然后,采用压电喷墨打印技术将细胞裂解缓冲液和荧光底物荧光素-二-β-D-吡喃半乳糖苷作为“第二滴”注入到密封油中,并与“第一滴”融合。因此,我们成功地在单细胞水平上测量了K562细胞的细胞内β-半乳糖苷酶活性。我们的方法首次实现了在保持开放结构的同时,能够同时容纳单个细胞的高占用率和顺序添加试剂的能力。我们认为,我们方法的可行性和灵活性将增强其作为通用单细胞研究工具的用途,并加速在细胞异质性研究中采用喷墨打印。

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