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高通量注塑微流控装置,用于单细胞时空动力学分析。

High-throughput injection molded microfluidic device for single-cell analysis of spatiotemporal dynamics.

机构信息

Department of Mechanical Engineering, Seoul National University, Seoul, Republic of Korea.

出版信息

Lab Chip. 2021 Aug 21;21(16):3150-3158. doi: 10.1039/d0lc01245a. Epub 2021 Jun 28.

Abstract

Single-cell level analysis of various cellular behaviors has been aided by recent developments in microfluidic technology. Polydimethylsiloxane (PDMS)-based microfluidic devices have been widely used to elucidate cell differentiation and migration under spatiotemporal stimulation. However, microfluidic devices fabricated with PDMS have inherent limitations due to material issues and non-scalable fabrication process. In this study, we designed and fabricated an injection molded microfluidic device that enables real-time chemical profile control. This device is made of polystyrene (PS), engineered with channel dimensions optimized for injection molding to achieve functionality and compatibility with single cell observation. We demonstrated the spatiotemporal dynamics in the device with computational simulation and experiments. In temporal dynamics, we observed extracellular signal-regulated kinase (ERK) activation of PC12 cells by stimulating the cells with growth factors (GFs). Also, we confirmed yes-associated protein (YAP) phase separation of HEK293 cells under stimulation using sorbitol. In spatial dynamics, we observed the migration of NIH 3T3 cells (transfected with Lifeact-GFP) under different spatiotemporal stimulations of PDGF. Using the injection molded plastic devices, we obtained comprehensive data more easily than before while using less time compared to previous PDMS models. This easy-to-use plastic microfluidic device promises to open a new approach for investigating the mechanisms of cell behavior at the single-cell level.

摘要

单细胞水平分析各种细胞行为已经受益于微流控技术的最新进展。基于聚二甲基硅氧烷(PDMS)的微流控器件已被广泛用于阐明时空刺激下的细胞分化和迁移。然而,由于材料问题和不可扩展的制造工艺,由 PDMS 制造的微流控器件具有固有局限性。在本研究中,我们设计并制造了一种注塑成型的微流控器件,可实现实时化学轮廓控制。该器件由聚苯乙烯(PS)制成,采用经过优化的通道尺寸进行注塑成型,以实现功能和与单细胞观察的兼容性。我们通过计算模拟和实验演示了设备中的时空动力学。在时间动力学方面,我们通过用生长因子(GFs)刺激细胞来观察 PC12 细胞细胞外信号调节激酶(ERK)的激活。此外,我们还证实了在使用山梨醇刺激下,HEK293 细胞中的 yes 相关蛋白(YAP)相分离。在空间动力学方面,我们观察了在不同时空刺激下 PDGF 转染的 NIH 3T3 细胞(Lifeact-GFP)的迁移。使用注塑成型的塑料器件,我们获得了比以前更全面的数据,同时与以前的 PDMS 模型相比,时间更短。这种易于使用的塑料微流控器件有望为研究单细胞水平的细胞行为机制开辟新途径。

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