Dynamic, IPSC-derived hepatic tissue tri-culture system for the evaluation of liver physiology in vitro

被引:0
|
作者
Scheidecker, Benedikt [1 ]
Poulain, Stephane [3 ]
Sugimoto, Masahiro [4 ,5 ]
Kido, Taketomo [6 ]
Kawanishi, Takumi [7 ]
Miyajima, Atsushi [6 ]
Kim, Soo Hyeon [3 ]
Arakawa, Hiroshi [7 ]
Kato, Yukio [7 ]
Nishikawa, Masaki [2 ]
Danoy, Mathieu [2 ]
Sakai, Yasuyuki [2 ]
Leclerc, Eric [1 ,8 ]
机构
[1] Univ Tokyo, Inst Ind Sci, CNRS UMI 2820, Tokyo 1538505, Japan
[2] Univ Tokyo, Dept Chem Syst Engn, Tokyo 1138654, Japan
[3] Univ Tokyo, Inst Ind Sci, Tokyo 1538505, Japan
[4] Keio Univ, Inst Adv Biosci, Yamagata 9970035, Japan
[5] Tokyo Med Univ, Inst Med Sci, Tokyo 1608402, Japan
[6] Univ Tokyo, Inst Quantitat Biosci, Tokyo 1130032, Japan
[7] Kanazawa Univ, Sch Pharmaceut Sci, Kanazawa 9201102, Japan
[8] Univ Technol Compiegne, CNRS UMR 7338, Lab Biomecan & Bioingen, F-60203 Compiegne, France
关键词
IPSC; stem cell; organ-on-a-chip; hepatic tissue; perfusion; single cell RNAseq; PLURIPOTENT STEM-CELLS; PROGENITOR CELLS; RAT HEPATOCYTES; CHALLENGES; NANOCAGE; ZONATION; MODEL;
D O I
10.1088/1758-5090/ad30c5
中图分类号
R318 [生物医学工程];
学科分类号
0831 ;
摘要
Availability of hepatic tissue for the investigation of metabolic processes is severely limited. While primary hepatocytes or animal models are widely used in pharmacological applications, a change in methodology towards more sustainable and ethical assays is highly desirable. Stem cell derived hepatic cells are generally regarded as a viable alternative for the above model systems, if current limitations in functionality and maturation can be overcome. By combining microfluidic organ-on-a-chip technology with individually differentiated, multicellular hepatic tissue fractions, we aim to improve overall functionality of hepatocyte-like cells, as well as evaluate cellular composition and interactions with non-parenchymal cell populations towards the formation of mature liver tissue. Utilizing a multi-omic approach, we show the improved maturation profiles of hepatocyte-like cells maintained in a dynamic microenvironment compared to standard tissue culture setups without continuous perfusion. In order to evaluate the resulting tissue, we employ single cell sequencing to distinguish formed subpopulations and spatial localization. While cellular input was strictly defined based on established differentiation protocols of parenchyma, endothelial and stellate cell fractions, resulting hepatic tissue was shown to comprise a complex mixture of epithelial and non-parenchymal fractions with specific local enrichment of phenotypes along the microchannel. Following this approach, we show the importance of passive, paracrine developmental processes in tissue formation. Using such complex tissue models is a crucial first step to develop stem cell-derived in vitro systems that can compare functionally with currently used pharmacological and toxicological applications.
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页数:19
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