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使用逆向反射型双面微粒的非光谱迁移细胞监测方法

Nonspectroscopic Migratory Cell Monitoring Method Using Retroreflective Janus Microparticles.

作者信息

Kim Ka Ram, Lee Danbi, Jeong Kwan Young, Lee Kyung Won, Kim Moon Suk, Kim Jae-Ho, Yoon Hyun C

机构信息

Department of Molecular Science and Technology, Ajou University, Suwon 16499, Republic of Korea.

出版信息

ACS Omega. 2020 Sep 16;5(38):24790-24798. doi: 10.1021/acsomega.0c03454. eCollection 2020 Sep 29.

Abstract

This study aims to suggest a simple migratory cell monitoring method in the Transwell system by utilizing retroreflective Janus microparticles (RJPs) as an optical probe. The RJP could be internalized on cells without compromising the cell viability and can be registered as bright spots within the cell body by inducing retroreflection from nonspectroscopic light sources. Conventional optical probes (e.g., fluorophores, chromogens, and nanoparticles) have been extensively studied and applied across diverse platforms (e.g., Boyden chamber, wound closing, and microfluidic chips) for understanding in vitro kinetic cell behavior. However, the complexities of running such platforms and setting up analytical instruments are limiting. In this regard, we aimed to demonstrate a modified Transwell migration assay by introducing the retroreflection principle to the cell quantification procedures that ensure a simplified optical setup, assure easy signal acquisition, and are compatible with conventional platforms. To demonstrate retroreflection as a signaling principle, a half-metal-coated silica particle that can induce interior retroreflection was synthesized. Because the RJPs can concentrate incident light and reflect it back to the light source, retroreflection was distinctively recognizable and enabled sensitive visualization. To verify the applicability of the developed migration assay, cell quantification during the incremental progress of macrophage migration, and cell quantification under gradients of chemoattractant monocyte protein-1, was accomplished by obtaining phagocytosed RJP-mediated retroreflection signals. Considering that conventional assays are designed as endpoint measurements, we anticipate the proposed retroreflection-based cell quantification technique to be a promising solution, bypassing current limitations.

摘要

本研究旨在通过利用逆向反射型Janus微粒(RJPs)作为光学探针,在Transwell系统中提出一种简单的迁移细胞监测方法。RJPs能够被细胞内化而不影响细胞活力,并且通过诱导非光谱光源的逆向反射,可在细胞体内被记录为亮点。传统的光学探针(如荧光团、色原和纳米颗粒)已被广泛研究并应用于各种平台(如Boyden小室、伤口闭合和微流控芯片),以了解体外细胞动力学行为。然而,运行此类平台和设置分析仪器的复杂性存在局限性。在这方面,我们旨在通过将逆向反射原理引入细胞定量程序,展示一种改进的Transwell迁移测定法,该方法可确保简化光学设置、易于信号采集,并与传统平台兼容。为了证明逆向反射作为一种信号原理,合成了一种能够诱导内部逆向反射的半金属涂层二氧化硅颗粒。由于RJPs能够聚集入射光并将其反射回光源,逆向反射具有明显的可识别性,并能够实现灵敏的可视化。为了验证所开发的迁移测定法的适用性,通过获取吞噬的RJP介导的逆向反射信号,完成了巨噬细胞迁移增量过程中的细胞定量以及趋化因子单核细胞蛋白-1梯度下的细胞定量。鉴于传统测定法设计为终点测量,我们预期所提出的基于逆向反射的细胞定量技术将成为一种有前景的解决方案,绕过当前的局限性。

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