Multi-Compartment 3D-Cultured Organ-on-a-Chip: Towards a Biomimetic Lymph Node for Drug Development

被引:56
|
作者
Shanti, Aya [1 ]
Samara, Bisan [1 ]
Abdullah, Amal [1 ]
Hallfors, Nicholas [1 ]
Accoto, Dino [2 ]
Sapudom, Jiranuwat [3 ]
Alatoom, Aseel [3 ]
Teo, Jeremy [3 ,4 ]
Danti, Serena [5 ]
Stefanini, Cesare [1 ]
机构
[1] Khalifa Univ Sci & Technol, Healthcare Engn Innovat Ctr, Biomed Engn Dept, POB 127788, Abu Dhabi, U Arab Emirates
[2] Nanyang Technol Univ, Sch Mech & Aerosp Engn, 50 Nanyang Ave, Singapore 639798, Singapore
[3] New York Univ Abu Dhabi, Div Engn, POB 129188, Abu Dhabi, U Arab Emirates
[4] New York Univ, Dept Biomed & Mech Engn, POB 903, New York, NY 10276 USA
[5] Univ Pisa, Dept Civil & Ind Engn, I-56122 Pisa, Italy
关键词
biomimicry; drug development; lymph node; microfabrication; microfluidics; organ-on-a-chip; T-CELL-ACTIVATION; IN-VITRO; INTERSTITIAL CONVECTION; B-CELLS; DELIVERY; ANTIGEN; CULTURE; MICROENVIRONMENTS; DIFFERENTIATION; DIFFUSION;
D O I
10.3390/pharmaceutics12050464
中图分类号
R9 [药学];
学科分类号
1007 ;
摘要
The interaction of immune cells with drugs and/or with other cell types should be mechanistically investigated in order to reduce attrition of new drug development. However, they are currently only limited technologies that address this need. In our work, we developed initial but significant building blocks that enable such immune-drug studies. We developed a novel microfluidic platform replicating the Lymph Node (LN) microenvironment called LN-on-a-chip, starting from design all the way to microfabrication, characterization and validation in terms of architectural features, fluidics, cytocompatibility, and usability. To prove the biomimetics of this microenvironment, we inserted different immune cell types in a microfluidic device, which showed an in-vivo-like spatial distribution. We demonstrated that the developed LN-on-a-chip incorporates key features of the native human LN, namely, (i) similarity in extracellular matrix composition, morphology, porosity, stiffness, and permeability, (ii) compartmentalization of immune cells within distinct structural domains, (iii) replication of the lymphatic fluid flow pattern, (iv) viability of encapsulated cells in collagen over the typical timeframe of immunotoxicity experiments, and (v) interaction among different cell types across chamber boundaries. Further studies with this platform may assess the immune cell function as a step forward to disclose the effects of pharmaceutics to downstream immunology in more physiologically relevant microenvironments.
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页数:17
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