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高通量单细胞微阵列用于测定细胞膜通透性。

A highly-occupied, single-cell trapping microarray for determination of cell membrane permeability.

机构信息

The Center for Engineering in Medicine, BioMEMS Resource Center, Massachusetts General Hospital, Harvard Medical School, Charlestown, MA 02129, USA.

出版信息

Lab Chip. 2017 Nov 21;17(23):4077-4088. doi: 10.1039/c7lc00883j.

Abstract

Semi- and selective permeability is a fundamentally important characteristic of the cell membrane. Membrane permeability can be determined by monitoring the volumetric change of cells following exposure to a non-isotonic environment. For this purpose, several microfluidic perfusion chambers have been developed recently. However, these devices only allow the observation of one single cell or a group of cells that may interact with one another in an uncontrolled way. Some of these devices have integrated on-chip temperature control to investigate the temperature-dependence of membrane permeability, but they inevitably require sophisticated fabrication and assembly, and delicate temperature and pressure calibration. Therefore, it is highly desirable to design a simple single-cell trapping device that allows parallel monitoring of multiple separate, individual cells subjected to non-isotonic exposure at various temperatures. In this study, we developed a pumpless, single-layer microarray with high trap occupancy of single cells. The benchmark performance of the device was conducted by targeting spherical particles of 18.8 μm in diameter as a model, yielding trap occupancy of up to 86.8% with a row-to-row shift of 10-30 μm. It was also revealed that in each array the particles larger than a corresponding critical size would be excluded by the traps in a deterministic lateral displacement mode. Demonstrating the utility of this approach, we used the single-cell trapping device to determine the membrane permeability of rat hepatocytes and patient-derived circulating tumor cells (Brx-142) at 4, 22 and 37 °C. The membrane of rat hepatocytes was found to be highly permeable to water and small molecules such as DMSO and glycerol, via both lipid- and aquaporin-mediated pathways. Brx-142 cells, however, displayed lower membrane permeability than rat hepatocytes, which was associated with strong coupling of water and DMSO transport but less interaction between water and glycerol. The membrane permeability data reported here provide new insights into the biophysics of membrane transport such as aquaporin expression and coupling transport of water and solutes, as well as providing essential data for the ultimate goal of biobanking rare cells and precious tissues.

摘要

半透性和选择性是细胞膜的一个基本特征。可以通过监测细胞在暴露于非等渗环境后的体积变化来确定膜的通透性。为此,最近已经开发了几种微流控灌注室。然而,这些设备只能观察到一个或一组细胞,这些细胞可能以不受控制的方式相互作用。其中一些设备已经集成了片上温度控制,以研究膜通透性的温度依赖性,但它们不可避免地需要复杂的制造和组装,以及精细的温度和压力校准。因此,设计一种简单的单细胞捕获装置,允许在不同温度下平行监测多个单独的、个体的细胞对非等渗暴露的反应,这是非常理想的。在这项研究中,我们开发了一种无泵、单层微阵列,具有高的单细胞捕获率。该设备的基准性能通过以直径为 18.8μm 的球形颗粒为模型进行了测试,结果表明,捕获率高达 86.8%,行与行之间的偏移量为 10-30μm。还揭示了在每个微阵列中,大于相应临界尺寸的颗粒将以确定性侧向位移模式被捕获。为了证明这种方法的实用性,我们使用单细胞捕获装置在 4°C、22°C 和 37°C 下测定了大鼠肝细胞和患者来源的循环肿瘤细胞(Brx-142)的膜通透性。结果发现,大鼠肝细胞的膜对水和小分子(如 DMSO 和甘油)具有高度通透性,这是通过脂质和水通道蛋白介导的途径实现的。然而,Brx-142 细胞的膜通透性低于大鼠肝细胞,这与水和 DMSO 运输的强耦合有关,但水和甘油之间的相互作用较少。这里报道的膜通透性数据为水通道蛋白表达和水与溶质的偶联运输等膜转运的生物物理学提供了新的见解,并为最终目的提供了必要的数据,即稀有细胞和珍贵组织的生物库存储。

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本文引用的文献

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