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Optimization of the formation of embedded multicellular spheroids of MCF-7 cells: How to reliably produce a biomimetic 3D model.MCF-7细胞嵌入式多细胞球体形成的优化:如何可靠地构建仿生3D模型。
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Surface Tension Guided Hanging-Drop: Producing Controllable 3D Spheroid of High-Passaged Human Dermal Papilla Cells and Forming Inductive Microtissues for Hair-Follicle Regeneration.表面张力引导悬滴法:制备高传代人真皮乳头细胞的可控三维球体并形成用于毛囊再生的诱导性微组织。
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Seamless Combination of Fluorescence-Activated Cell Sorting and Hanging-Drop Networks for Individual Handling and Culturing of Stem Cells and Microtissue Spheroids.用于干细胞和微组织球体个体处理与培养的荧光激活细胞分选与悬滴网络的无缝结合。
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基于液滴接触的球体转移实现球体阵列的高通量培养与包埋

High-throughput culture and embedment of spheroid array using droplet contact-based spheroid transfer.

作者信息

Kim Hwisoo, Cho Chang Hyun, Park Je-Kyun

机构信息

Department of Bio and Brain Engineering, Korea Advanced Institute of Science and Technology (KAIST), 291 Daehak-ro, Yuseong-gu, Daejeon 34141, Republic of Korea.

出版信息

Biomicrofluidics. 2018 Jul 18;12(4):044109. doi: 10.1063/1.5039965. eCollection 2018 Jul.

DOI:10.1063/1.5039965
PMID:30867862
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6404923/
Abstract

Spheroids are one of the most representative models of 3D cell culture, which can be easily formed using conventional hanging drop method. However, medium change and spheroid transferring process are the bottlenecks that reduce the throughput of the entire process in the hanging drop culture. In addition, the embedment of spheroid into hydrogel still depends on the individual pipetting process. To overcome these issues, we present poly(dimethylsiloxane) (PDMS)-based simple devices which can exploit droplet contact-based spheroid transfer using a drop array chip (DAC) having an array of well structures and peripheral rims. When the upper spheroid-containing drops were in contact with the lower liquid drops, the air-liquid interface disappeared at the merged surface and the spheroids settled down due to gravitational force. This method was applied to repetitive medium change and live/dead staining of spheroids cultured with the hanging drop method. To simultaneously embed the spheroids into the corresponding collagen hydrogel drops, a PDMS-based pillar array chip (PAC) was contacted in advance with the spheroid-containing DAC. The contacted PAC then contained the spheroids trapped in small drops of liquid reduced in volume to around 0.5 l. Consequently, the spheroids were embedded into the collagen drops at once by contacting the spheroid-containing PAC with the collagen-loaded DAC. The embedded spheroids using the DAC-PAC contacting method showed a reliable invasion behavior compared to the embedded spheroids using conventional manual pipetting.

摘要

球体是3D细胞培养中最具代表性的模型之一,可使用传统的悬滴法轻松形成。然而,换液和球体转移过程是悬滴培养中降低整个过程通量的瓶颈。此外,将球体嵌入水凝胶仍依赖于个体移液过程。为克服这些问题,我们展示了基于聚二甲基硅氧烷(PDMS)的简单装置,其可利用基于液滴接触的球体转移,该装置使用具有孔结构阵列和周边边缘的滴阵列芯片(DAC)。当上含球体的液滴与下液体液滴接触时,合并表面的气液界面消失,球体因重力沉降。该方法应用于用悬滴法培养的球体的重复换液和活/死染色。为将球体同时嵌入相应的胶原水凝胶滴中,预先将基于PDMS的柱阵列芯片(PAC)与含球体的DAC接触。然后,接触的PAC包含被困在体积减小至约0.5μl的小液滴中的球体。因此,通过使含球体的PAC与加载胶原的DAC接触,球体立即被嵌入胶原滴中。与使用传统手动移液嵌入的球体相比,使用DAC - PAC接触法嵌入的球体表现出可靠的侵袭行为。