Interactions between Multiple Cell Types in Parallel Microfluidic Channels: Monitoring Platelet Adhesion to an Endothelium in the Presence of an Anti-Adhesion Drug
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- 作者:Chia-Jui Ku ; Teresa D’ ; Amico Oblak ; Dana M. Spence
- 刊名:Analytical Chemistry
- 出版年:2008
- 出版时间:October 1, 2008
- 年:2008
- 卷:80
- 期:19
- 页码:7543-7548
- 全文大小:238K
- 年卷期:v.80,no.19(October 1, 2008)
- ISSN:1520-6882
文摘
A simple method for immobilizing endothelial cells in the channels of a microfluidic device fabricated with soft lithography is presented that requires no surface oxidation of the substrate material used in conjunction with the microfluidic device and is operable even with a reversible seal. Specifically, optimal conditions for culturing bovine pulmonary artery endothelial cells (bPAECs) to the surface of a Petri dish were investigated. The parameters investigated included fibronectin concentration, temperature, seeding density, and immobilization time. To enhance the utility of the device, all optimization studies, and studies involving platelet adhesion to the immobilized endothelium, were performed in parallel channels, thereby enabling improved throughput over a single channel device. The optimal conditions for cell immobilization included coating the Petri dish with 100 μg/mL fibronectin, a seeding cell density of 1.00 × 105 cells mL−1, and an immobilization time of 90 min at 37 °C. The device was then employed to monitor the physical interaction (adhesion) of platelets to the immobilized endothelium in the presence of a known platelet activator (ADP) and a drug inhibitor of platelet activation. The number of platelets adhering to the endothelial cells in the channels increased from 17.0 ± 2.3 in the absence of ADP to 63.2 ± 2.4 in the presence of 5.00 μM ADP. Moreover, the data presented here also shows that inhibition of endothelium nitric oxide (NO) production, a recognized inhibitor of platelet adhesion to the endothelium, increased the number of platelets adhering to the surface to 35.4 ± 1.0. In the presence of NO inhibition and 5.00 μM ADP, the affect on platelet adhesion was further increased to 127 ± 5.2. Finally, this device was employed to investigate the effect of a drug known to inhibit platelet adhesion (clopidogrel) and, in the presence of the drug, the platelet adhesion due to activation by 5.00 μM ADP decreased to 24.0 ± 3.8. This work is the first representation of multiple cell types physically interacting in the channels of a microfluidic device and further demonstrates the potential of these devices in the drug discovery process and drug efficacy studies.