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A microfluidic device for depositing and addressing two cell populations with intercellular population communication capability

机译:具有细胞间群体通信能力的用于沉积和寻址两个细胞群体的微流体装置

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摘要

We present a method for depositing cells in the microchambers of a sealed microfluidic device and establishing flow across the chambers independently and serially. The device comprises a transparent poly(dimethyl-siloxane) (PDMS) microfluidic network (MFN) having 2 cell chambers with a volume of 0.49 μL, 6 microchannels for servicing the chambers, and 1 microchannel linking both chambers. The MFN is sealed with a Si chip having 6 vias and ports that can be left open or connected to high-precision pumps. Liquids are drawn through each chamber in parallel or sequentially at flow rates from 0.1 to 10 uL min"1. Plugs of liquid as small as 0.5 μL can be passed in one chamber within 5 s to 5 min. Plugs of liquid can also be introduced into a chamber for residence times of up to 30 min. By injecting different liquids into 3 ports, 3 adjacent laminar streams of liquid can be drawn inside one chamber with lateral concentration gradients between the streams ranging from 20 to 500 μm. The flexibility of this device for depositing cells and exposing them to liquids in parallel or serially is illustrated by depositing two types of cells, murine N9 microglia and human SH-S5Y5 neuroblastoma.rnMicrofluidic communication between the chambers is illustrated by stimulating N9 microglia using ATP to induce these cells to release plasma membrane vesicles. The vesicles are drawn through the second chamber containing neuroblastoma and collected in a port of the device for off-chip analysis using confocal fluorescence microscopy. Cells in the MFN can also be fixed using a solution of formaldehyde for further analysis after disassembly of the MFN and Si lid. This microfluidic device offers a simple, flexible, and powerful method for depositing two cell populations in separate chambers and may help investigating pathways between the cells populations.
机译:我们提出了一种用于在密封的微流控设备的微腔室中沉积细胞并独立地和连续地跨腔室建立流动的方法。该设备包括一个透明的聚二甲基硅氧烷(PDMS)微流体网络(MFN),该网络具有2个容积为0.49μL的池室,6个用于维护室的微通道和1个连接两个室的微通道。 MFN用具有6个通孔和端口的Si芯片密封,这些通孔和端口可以保持打开状态或连接到高精度泵。液体以0.1至10 uL min“ 1的速率平行或依次吸入每个腔室。小至0.5μL的液体塞可以在5 s至5分钟内通过一个腔室。也可以引入液体塞进入一个腔室,停留时间最多为30分钟,通过将不同的液体注入3个端口,可以在一个腔室内抽取3个相邻的层流,流之间的横向浓度梯度范围为20至500μm。通过沉积鼠N9小胶质细胞和人SH-S5Y5神经母细胞瘤两种类型的细胞来说明用于沉积细胞并将其平行或串行暴露于液体中的装置。通过使用ATP刺激N9小胶质细胞以诱导这些细胞向细胞内的微流通讯,可以说明小室之间的微流体连通。释放出的质膜囊泡穿过包含神经母细胞瘤的第二个腔室,并收集在装置的端口中,以使用共聚焦荧光灯进行芯片外分析荧光显微镜。拆卸MFN和Si盖后,也可以使用甲醛溶液固定MFN中的细胞,以进行进一步分析。这种微流控设备提供了一种简单,灵活且功能强大的方法,可将两个细胞群体沉积在不同的腔室中,并可能有助于研究细胞群体之间的通路。

著录项

  • 来源
    《Biomedical Microdevices》 |2010年第2期|275-282|共8页
  • 作者单位

    IBM Research - Zurich, Saeumerstrasse 4, Rueschlikon 8803, Switzerland;

    Neuro-Zone s.r.l., via Fratelli Cervi 93, Segrate, Milan, Italy;

    Neuro-Zone s.r.l., via Fratelli Cervi 93, Segrate, Milan, Italy;

    Neuro-Zone s.r.l., via Fratelli Cervi 93, Segrate, Milan, Italy Department of Pharmacology, CNR Institute of Neuroscience and Fondazione Filarete, University of Milano and IRCCS Don Gnocchi, Milan, Italy;

    IBM Research - Zurich, Saeumerstrasse 4, Rueschlikon 8803, Switzerland;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    microfluidics; cell culture; PDMS; cellular assays;

    机译:微流体细胞培养;PDMS;细胞分析;

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