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Capillary-assisted microfluidic biosensing platform captures single cell secretion dynamics in nanoliter compartments

分泌物 微流控 单细胞分析 生物传感器 纳米技术 癌细胞 化学 生物物理学 细胞内 细胞 生物 材料科学 生物化学 癌症 遗传学
作者
Amin Hassanzadeh‐Barforoushi,Majid Ebrahimi Warkiani,David Gallego‐Ortega,Guozhen Liu,Tracie Barber
出处
期刊:Biosensors and Bioelectronics [Elsevier BV]
卷期号:155: 112113-112113 被引量:27
标识
DOI:10.1016/j.bios.2020.112113
摘要

Cancer cells continuously secrete inflammatory biomolecules which play significant roles in disease progression and tumor metastasis toward secondary sites. Despite recent efforts to capture cancer cells' intercellular secretion heterogeneity using microfluidics, the challenges in operation of these systems as well as the complexity of designing a biosensing assay for long-term and real-time measurement of single cell secretions have become grand research barriers. Here, we present a new capillary-based microfluidic biosensing approach to easily and reliably capture ~500 single cells inside isolated dead-end nanoliter compartments using simple pipette injection, and quantify their individual secretion dynamics at the single cell resolution over a long period of culture (~16 h). We first present a detailed investigation of the fluid mechanics underlying the formation of nanoliter compartments in the microfluidic system. Based on the measurement of single cell capture efficiency, we employ a one-step FRET-based biosensor which monitors the single cancer cells' protease activity. The sensor reports the fluorescent signal as a product of amino acid chain cleavage and reduction in its quenching capability. Using the single cell protease secretion data, we identified modes of cell secretion dynamics in our cell sample. While most of the cells had low secretion levels, two other smaller and more aggressive secretion dynamics were cells with secretion modes that include sharp spikes or slow but progressive trend. The method presented here overcomes the difficulties associated with performing single cell secretion assays, enabling a feasible and reliable technique for high throughput measurement of metabolic activities in cancer cells.

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