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用于直接观察趋化性穿迁移的微流控成像室。

A microfluidic imaging chamber for the direct observation of chemotactic transmigration.

机构信息

Department of Physiology and Biophysics, Case Western Reserve University School of Medicine, 10900 Euclid Ave., Cleveland, OH 44106, USA.

出版信息

Biomed Microdevices. 2010 Jun;12(3):543-53. doi: 10.1007/s10544-010-9411-8.

Abstract

To study the roles of nonmuscle myosin II (NM-II) during invasive cell migration, microfluidic migration chambers have been designed and fabricated using photo- and soft-lithography microfabrication techniques. The chamber consists of two channels separated by a vertical barrier with multiple bays of pores with widths varying from 6 microm to 16 microm, and lengths varying from 25 microm to 50 microm. The cells are plated in the channel on one side of the barrier while a chemoattractant is flowed through the channel on the other side of the barrier. In these chambers, cells can be observed with transmitted light or fluorescence optics while they chemotax through various sized pores that impose differential mechanical resistance to transmigration. As an initial test of this device, we compared breast-cancer cell chemotactic transmigration through different pore sizes with and without inhibition of NM-II. Two distinct rates were observed as cells attempted to pull their nucleus through the smaller pores, and the faster nuclear transit mode was critically dependent on NM-II motor activity. The ability to monitor cells as they chemotax through pores of different dimensions within a single experimental system provides novel information on how pore size affects cell morphology and migration rate, providing a dramatic improvement of imaging potential relative to other in vitro transmigration systems such as Boyden chambers.

摘要

为了研究非肌肉肌球蛋白 II(NM-II)在侵袭性细胞迁移中的作用,我们使用光和软光刻微纳加工技术设计并制造了微流控迁移室。该室由两个通道组成,由垂直障碍物隔开,障碍物上有多个宽度从 6 微米到 16 微米不等、长度从 25 微米到 50 微米不等的小孔。细胞被接种在障碍物一侧的通道中,同时有化学引诱剂流过障碍物另一侧的通道。在这些腔室中,可以通过透射光或荧光光学观察细胞,同时它们通过各种大小的孔进行趋化运动,这些孔对穿越施加不同的机械阻力。作为该装置的初步测试,我们比较了乳腺癌细胞在没有和抑制 NM-II 的情况下通过不同孔径的趋化性迁移。当细胞试图将细胞核穿过较小的孔时,观察到两种不同的速度,而更快的核迁移模式严重依赖于 NM-II 马达的活性。在单个实验系统中监测细胞通过不同尺寸孔趋化运动的能力,提供了关于孔径如何影响细胞形态和迁移率的新信息,与 Boyden 室等其他体外迁移系统相比,大大提高了成像潜力。

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