细胞
细胞生物学
细胞溶解
微流控
效应器
T细胞
CD8型
单细胞分析
免疫突触
免疫系统
细胞内
分泌物
电池类型
细胞毒性T细胞
化学
生物物理学
生物
免疫学
材料科学
纳米技术
体外
T细胞受体
生物化学
作者
Saheli Sarkar,Pooja Sabhachandani,Dina Stroopinsky,Kristen Palmer,Noa Cohen,Jacalyn Rosenblatt,David Avigan,Tania Konry
出处
期刊:Biomicrofluidics
[American Institute of Physics]
日期:2016-09-01
卷期号:10 (5): 054115-054115
被引量:75
摘要
Cell-cell communication mediates immune responses to physiological stimuli at local and systemic levels. Intercellular communication occurs via a direct contact between cells as well as by secretory contact-independent mechanisms. However, there are few existing methods that allow quantitative resolution of contact-dependent and independent cellular processes in a rapid, precisely controlled, and dynamic format. This study utilizes a high-throughput microfluidic droplet array platform to analyze cell-cell interaction and effector functions at single cell level. Controlled encapsulation of distinct heterotypic cell pairs was achieved in a single-step cell loading process. Dynamic analysis of dendritic cell (DC)-T cell interactions demonstrated marked heterogeneity in the type of contact and duration. Non-stimulated DCs and T cells interacted less frequently and more transiently while antigen and chemokine-loaded DCs and T cells depicted highly stable interactions in addition to transient and sequential contact. The effector function of CD8+ T cells was assessed via cytolysis of multiple myeloma cell line. Variable cell conjugation periods and killing time were detected irrespective of the activation of T cells, although activated T cells delivered significantly higher cytotoxicity. T cell alloreactivity against the target cells was partially mediated by secretion of interferon gamma, which was abrogated by the addition of a neutralizing antibody. These results suggest that the droplet array-based microfluidic platform is a powerful technique for dynamic phenotypic screening and potentially applicable for evaluation of novel cell-based immunotherapeutic agents.
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