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一种基于 PDMS 的简易微流控通道设计,可去除气泡,实现哺乳动物细胞的长期片上培养。

A simple PDMS-based microfluidic channel design that removes bubbles for long-term on-chip culture of mammalian cells.

机构信息

CAS Key Lab for Biological Effects of Nanomaterials and Nanosafety, National Center for NanoScience & Technology, 11 ZhongGuanCun BeiYiTiao, Beijing, 100190, China.

出版信息

Lab Chip. 2010 Nov 7;10(21):2906-10. doi: 10.1039/c005274d. Epub 2010 Sep 15.

Abstract

This report shows methods to fabricate polydimethylsiloxane (PDMS) microfluidic systems for long-term (up to 10 day) cell culture. Undesired bubble accumulation in microfluidic channels abruptly changes the microenvironment of adherent cells and leads to the damage and death of cells. Existing bubble trapping approaches have drawbacks such as the need to pause fluid flow, requirement for external vacuum or pressure source, and possible cytotoxicity. This study reports two kinds of integrated bubble trap (IBT) which have excellent properties, including simplicity in structure, ease in fabrication, no interference with the flow, and long-term stability. IBT-A provides the simplest solution to prevent bubbles from entering microfluidic channels. In situ time-lapse imaging experiments indicate that IBT-B is an excellent device both for bubble trapping and debubbling in cell-loaded microfluidics. MC 3T3 E1 cells, cultured in a long and curved microfluidic channel equipped with IBT-B, showed high viability and active proliferation after 10 days of continuous fluid flow. The comprehensive measures taken in our experiments have led to successful long-term, bubble-free, on-chip culture of cells.

摘要

本报告展示了制造用于长期(长达 10 天)细胞培养的聚二甲基硅氧烷(PDMS)微流控系统的方法。不希望在微流道中积聚气泡会突然改变贴壁细胞的微环境,导致细胞损伤和死亡。现有的气泡捕获方法存在需要暂停流体流动、需要外部真空或压力源以及可能的细胞毒性等缺点。本研究报告了两种集成式气泡阱(IBT),它们具有出色的性能,包括结构简单、易于制造、不干扰流动和长期稳定性。IBT-A 提供了最简单的解决方案,可防止气泡进入微流道。原位时程成像实验表明,IBT-B 是一种用于在装有细胞的微流控中捕获和除泡的出色装置。在配备有 IBT-B 的长而弯曲的微流控通道中培养的 MC3T3E1 细胞在连续 10 天的流体流动后显示出高存活率和活跃的增殖。我们在实验中采取的综合措施导致了成功的无气泡、长期、芯片上细胞培养。

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