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A closed 3D printed microfluidic device for automated growth and differentiation of cerebral organoids from single-cell suspension

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KANDRA Mário VÁŇOVÁ Tereza JONGEN Vincent Alexander POSPÍŠIL Jakub NOVAK Josef CHOCHOLA Václav BURYSKA Tomas PROKOP Zbyněk HODNY Zdenek HAMPL Aleš BOHAČIAKOVÁ Dáša JAROŠ Josef

Rok publikování 2024
Druh Článek v odborném periodiku
Časopis / Zdroj Biotechnology Journal
Fakulta / Pracoviště MU

Lékařská fakulta

Citace
www https://analyticalsciencejournals.onlinelibrary.wiley.com/doi/10.1002/biot.202400240
Doi http://dx.doi.org/10.1002/biot.202400240
Klíčová slova 3D cell culture; microfluidics; organoids; pluripotent stem cells; tissue engineering
Přiložené soubory
Popis The development of 3D organoids has provided a valuable tool for studying human tissue and organ development in vitro. Cerebral organoids, in particular, offer a unique platform for investigating neural diseases. However, current methods for generating cerebral organoids suffer from limitations such as labor-intensive protocols and high heterogeneity among organoids. To address these challenges, we present a microfluidic device designed to automate and streamline the formation and differentiation of cerebral organoids. The device utilizes microwells with two different shapes to promote the formation of a single aggregate per well and incorporates continuous medium flow for optimal nutrient exchange. In silico simulations supported the effectiveness of the microfluidic chip in replicating cellular microenvironments. Our results demonstrate that the microfluidic chip enables uniform growth of cerebral organoids, significantly reducing the hands-on time required for maintenance. Importantly, the performance of the microfluidic system is comparable to the standard 96-well plate format even when using half the amount of culture medium, and the resulting organoids exhibit substantially developed neuroepithelial buds and cortical structures. This study highlights the potential of custom-designed microfluidic technology in improving the efficiency of cerebral organoid culture.
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