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https://doi.org/10.1186/s13287-020-01618-6
Title: | Selection of human induced pluripotent stem cells lines optimization of cardiomyocytes differentiation in an integrated suspension microcarrier bioreactor | Authors: | Laco, Filip Lam, Alan Tin-Lun Woo, Tsung-Liang Tong, Gerine Ho, Valerie Soong, Poh-Loong Grishina, Elina Lin, Kun-Han Reuveny, Shaul Oh, Steve Kah-Weng |
Keywords: | Science & Technology Life Sciences & Biomedicine Cell & Tissue Engineering Cell Biology Medicine, Research & Experimental Research & Experimental Medicine Bioprocessing Cardiomyocytes Human induced pluripotent stem cells Microcarriers Stirred tank bioreactor OptioQUANT (TM) platform CARDIAC DIFFERENTIATION EXPANSION CULTURE HYPOXIA GROWTH PLATFORM THERAPY PURIFICATION GENERATION STRATEGIES |
Issue Date: | 13-Mar-2020 | Publisher: | BMC | Citation: | Laco, Filip, Lam, Alan Tin-Lun, Woo, Tsung-Liang, Tong, Gerine, Ho, Valerie, Soong, Poh-Loong, Grishina, Elina, Lin, Kun-Han, Reuveny, Shaul, Oh, Steve Kah-Weng (2020-03-13). Selection of human induced pluripotent stem cells lines optimization of cardiomyocytes differentiation in an integrated suspension microcarrier bioreactor. STEM CELL RESEARCH & THERAPY 11 (1). ScholarBank@NUS Repository. https://doi.org/10.1186/s13287-020-01618-6 | Abstract: | BACKGROUND: The production of large quantities of cardiomyocyte is essential for the needs of cellular therapies. This study describes the selection of a human-induced pluripotent cell (hiPSC) line suitable for production of cardiomyocytes in a fully integrated bioprocess of stem cell expansion and differentiation in microcarrier stirred tank reactor. METHODS: Five hiPSC lines were evaluated first for their cardiac differentiation efficiency in monolayer cultures followed by their expansion and differentiation compatibility in microcarrier (MC) cultures under continuous stirring conditions. RESULTS: Three cell lines were highly cardiogenic but only one (FR202) of them was successfully expanded on continuous stirring MC cultures. FR202 was thus selected for cardiac differentiation in a 22-day integrated bioprocess under continuous stirring in a stirred tank bioreactor. In summary, we integrated a MC-based hiPSC expansion (phase 1), CHIR99021-induced cardiomyocyte differentiation step (phase 2), purification using the lactate-based treatment (phase 3) and cell recovery step (phase 4) into one process in one bioreactor, under restricted oxygen control (< 30% DO) and continuous stirring with periodic batch-type media exchanges. High density of undifferentiated hiPSC (2 ± 0.4 × 106 cells/mL) was achieved in the expansion phase. By controlling the stirring speed and DO levels in the bioreactor cultures, 7.36 ± 1.2 × 106 cells/mL cardiomyocytes with > 80% Troponin T were generated in the CHIR99021-induced differentiation phase. By adding lactate in glucose-free purification media, the purity of cardiomyocytes was enhanced (> 90% Troponin T), with minor cell loss as indicated by the increase in sub-G1 phase and the decrease of aggregate sizes. Lastly, we found that the recovery period is important for generating purer and functional cardiomyocytes (> 96% Troponin T). Three independent runs in a 300-ml working volume confirmed the robustness of this process. CONCLUSION: A streamlined and controllable platform for large quantity manufacturing of pure functional atrial, ventricular and nodal cardiomyocytes on MCs in conventional-type stirred tank bioreactors was established, which can be further scaled up and translated to a good manufacturing practice-compliant production process, to fulfill the quantity requirements of the cellular therapeutic industry. | Source Title: | STEM CELL RESEARCH & THERAPY | URI: | https://scholarbank.nus.edu.sg/handle/10635/219278 | ISSN: | 17576512 | DOI: | 10.1186/s13287-020-01618-6 |
Appears in Collections: | Staff Publications Elements |
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