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在微流控芯片上形成单细胞衍生的结肠癌类器官阵列,用于高通量肿瘤异质性分析。

Forming Single-Cell-Derived Colon Cancer Organoid Arrays on a Microfluidic Chip for High Throughput Tumor Heterogeneity Analysis.

机构信息

Department of Laboratory Medicine, The Second Affiliated Hospital, School of Medicine, South China University of Technology, Guangzhou 510180, China.

Guangdong Engineering Technology Research Center of Microfluidic Chip Medical Diagnosis, Guangzhou 510180, China.

出版信息

ACS Biomater Sci Eng. 2024 Aug 12;10(8):5265-5273. doi: 10.1021/acsbiomaterials.4c00727. Epub 2024 Aug 1.

DOI:10.1021/acsbiomaterials.4c00727
PMID:39087916
Abstract

Single-cell-derived tumor organoids (STOs) possess a distinct genetic background, making them valuable tools for demonstrating tumor heterogeneity. In order to fulfill the high throughput demands of STO assays, we have developed a microfluidic chip containing 30 000 microwells, which is dedicated to a single cell culture approach for selective expansion and differential induction of cancer stem cells. The microwells are coated with a hydrophilic copolymer to eliminate cell adhesion, and the cell culture is supported by poly(ethylene glycol) (PEG) to establish a nonadhesive culture environment. By utilizing an input cell density of 7 × 10·mL, it is possible to construct a 4000 single cell culture system through stochastic cell occupation. We demonstrate that the addition of 15% PEG10000 in the cell culture medium effectively prevents cell loss while facilitating tumor stem cell expansion. As were demonstrated by HCT116, HT29, and SW480 colon cancer cells, the microfluidic approach achieved a STO formation rate of ∼20%, resulting in over 800 STOs generated from a single culture. Comprehensive analysis through histomorphology, immunohistochemistry, drug response evaluation, assessment of cell invasion, and biomarker detection reveals the heterogeneity among individual STOs. Specifically, the smaller STOs exhibited higher invasion and drug resistance capabilities compared with the larger ones. The developed microfluidic approach effectively facilitates STO formation and offers promising prospects for investigating tumor heterogeneity, as well as conducting personalized therapy-focused drug screening.

摘要

单细胞来源的肿瘤类器官(STO)具有独特的遗传背景,使其成为展示肿瘤异质性的有价值工具。为了满足 STO 检测的高通量需求,我们开发了一种包含 30000 个微井的微流控芯片,专门用于单细胞培养方法,以选择性扩增和差异化诱导癌症干细胞。微井涂有亲水性共聚物以消除细胞黏附,细胞培养由聚乙二醇(PEG)支持,以建立非黏附的培养环境。通过利用 7×10·mL 的输入细胞密度,可以通过随机细胞占据构建 4000 个单细胞培养系统。我们证明,在细胞培养基中添加 15% PEG10000 可有效防止细胞损失,同时促进肿瘤干细胞的扩增。正如 HCT116、HT29 和 SW480 结肠癌细胞所证明的那样,微流控方法的 STO 形成率约为 20%,从单个培养中产生了超过 800 个 STO。通过组织形态学、免疫组织化学、药物反应评估、细胞侵袭评估和生物标志物检测进行的综合分析揭示了单个 STO 之间的异质性。具体而言,较小的 STO 比较大的 STO 具有更高的侵袭性和耐药性。所开发的微流控方法有效地促进了 STO 的形成,并为研究肿瘤异质性以及进行个性化治疗为重点的药物筛选提供了有前景的方法。

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