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微流控控制肿瘤和基质细胞球体配对和融合用于三维转移研究。

Microfluidic Control of Tumor and Stromal Cell Spheroids Pairing and Merging for Three-Dimensional Metastasis Study.

机构信息

Institute of Precision Medicine and Health, Research Center for Bioengineering and Sensing Technology, Beijing Key Laboratory for Bioengineering and Sensing Technology, School of Chemistry and Biological Engineering, University of Science and Technology Beijing, Beijing, China, 100083.

出版信息

Anal Chem. 2020 Jun 2;92(11):7638-7645. doi: 10.1021/acs.analchem.0c00408. Epub 2020 May 14.

Abstract

Three-dimensional cell culture provides an efficient way to simulate the in vivo tumorigenic microenvironment where tumor-stroma interaction intrinsically plays a pivotal role. Conventional three-dimensional (3D) culture is inadequate to address precise coexistential heterogeneous pairing and quantitative measurement in a parallel algorithm format. Herein, we implemented a set of microwell array microfluidic devices to study the cell spheroids-based tumor-stromal metastatic process in vitro. This approach enables accurate one-to-one pairing between tumor and fibroblast spheroid for dissecting 3D tumor invasion in the manner of high-content imaging. On one single device, 240 addressable tumor-stroma pairings can be formed with convenient pipetting and centrifugation within a small area of 1 cm. Consequential confocal imaging analysis disclosed that the tumor spheroid could envelop the fibroblast spheroid. Specific chemicals can effectively hamper or promote this 3D metastasis. Due to the addressable time-resolved measurements of the merging process of hundreds of doublets, our approach allows us to decipher the metastatic phenotype between different tumor spheroids. Compared with traditional protocols, massive heterogeneous cellular spheroids pairing and merging using this method is well-defined with microfluidic control, which leads to a favorable high-content tumor-stroma doublet metastasis analysis. This simple technique will be a useful tool for investigating heterotypic spheroid-spheroid interactions.

摘要

三维细胞培养提供了一种有效的方法来模拟体内肿瘤发生的微环境,其中肿瘤-基质相互作用起着关键作用。传统的三维(3D)培养不足以解决精确的共存异质配对和并行算法格式中的定量测量。在这里,我们实施了一组微孔阵列微流控装置,以研究基于细胞球体的肿瘤-基质转移过程。这种方法能够在高内涵成像的方式下准确地对肿瘤和成纤维细胞球体进行一对一配对,以剖析 3D 肿瘤侵袭。在一个单独的装置上,可以在 1cm 小面积内通过方便的移液和离心形成 240 个可寻址的肿瘤-基质配对。随后的共聚焦成像分析表明,肿瘤球体可以包裹成纤维细胞球体。特定的化学物质可以有效地阻止或促进这种 3D 转移。由于可以对数百个双联体的融合过程进行可寻址的时间分辨测量,我们的方法允许我们解析不同肿瘤球体之间的转移表型。与传统方案相比,使用这种方法可以很好地控制大量异质细胞球体的配对和融合,从而有利于进行高内涵肿瘤-基质双联体转移分析。这种简单的技术将成为研究异质球体-球体相互作用的有用工具。

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