Development of a new microfluidic platform integrating co-cultures of intestinal and liver cell lines

被引:77
|
作者
Bricks, Thibault [1 ]
Paullier, Patrick [1 ]
Legendre, Audrey [1 ]
Fleury, Marie-Jose [1 ]
Zeller, Perrine [1 ]
Merlier, Franck [2 ]
Anton, Pauline M. [3 ]
Leclerc, Eric [1 ]
机构
[1] Univ Technol Compiegne, CNRS UMR 7338, Lab Biomecan & Bioingn, Compiegne, France
[2] Univ Technol Compiegne, CNRS FRE 3580, Lab Genie Enzymat & Cellulaire, Compiegne, France
[3] Inst Polytech Lasalle Beauvais, EGEAL, Beauvais, France
关键词
Co-cultures; Microfluidic biochips; Caco-2; TC7; HepG2; C3A; Phenacetin; Drug screening; CULTURE ANALOG DEVICE; IN-VITRO; CACO-2; CELLS; DRUG ABSORPTION; TOXICITY; EXPRESSION; SYSTEM; TISSUE; MODEL; HEPATOCYTES;
D O I
10.1016/j.tiv.2014.02.005
中图分类号
R99 [毒物学(毒理学)];
学科分类号
100405 ;
摘要
We developed a new biological model to mimic the organ organ interactions between the intestine and the liver. We coupled polycarbonate cell culture inserts and microfluidic biochips in an integrated fluidic platform allowing dynamic co-cultures (called IIDMP for Integrated Insert in a Dynamic Microfluidic Platform). The intestinal compartment was simulated using Caco-2 TC7 cells and the liver one by HepG2 C3A. We showed that Caco-2 TC7 viability, barrier integrity and functionality (assessed by paracellular and active transport), were not altered during co-cultures in the bioreactor in comparison with the conventional insert Petri cultures. In parallel, the viability and metabolism of the HepG2 C3A cells were maintained in the microfluidic biochips. Then, as proof of concept, we used the bioreactor to follow the transport of phenacetin through the intestinal barrier and its metabolism into paracetamol by the CYP1A of the HepG2 C3A cells. Our results demonstrated the performance of this bioreactor with cell co-cultures compared to static co-culture controls in which weak biotransformation into paracetamol was detected. Our study illustrated the interest of such a bioreactor combining the advantages of a cell culture barrier and of liver microfluidic cultures in a common framework for in vitro studies. (C) 2014 Elsevier Ltd. All rights reserved.
引用
收藏
页码:885 / 895
页数:11
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