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Development of a Modular Automated System for Maintenance and Differentiation of Adherent Human Pluripotent Stem Cells

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Version 2 2024-05-30, 14:22
Version 1 2022-03-10, 08:05
journal contribution
posted on 2024-05-30, 14:22 authored by DE Crombie, M Daniszewski, HH Liang, T Kulkarni, F Li, GE Lidgerwood, A Conquest, Damian Hernandez, SS Hung, KP Gill, E De Smit, LS Kearns, L Clarke, VM Sluch, X Chamling, DJ Zack, RCB Wong, AW Hewitt, A Pébay
Patient-specific induced pluripotent stem cells (iPSCs) have tremendous potential for development of regenerative medicine, disease modeling, and drug discovery. However, the processes of reprogramming, maintenance, and differentiation are labor intensive and subject to intertechnician variability. To address these issues, we established and optimized protocols to allow for the automated maintenance of reprogrammed somatic cells into iPSCs to enable the large-scale culture and passaging of human pluripotent stem cells (PSCs) using a customized TECAN Freedom EVO. Generation of iPSCs was performed offline by nucleofection followed by selection of TRA-1-60–positive cells using a Miltenyi MultiMACS24 Separator. Pluripotency markers were assessed to confirm pluripotency of the generated iPSCs. Passaging was performed using an enzyme-free dissociation method. Proof of concept of differentiation was obtained by differentiating human PSCs into cells of the retinal lineage. Key advantages of this automated approach are the ability to increase sample size, reduce variability during reprogramming or differentiation, and enable medium- to high-throughput analysis of human PSCs and derivatives. These techniques will become increasingly important with the emergence of clinical trials using stem cells.

History

Journal

SLAS Discovery

Volume

22

Pagination

1016-1025

Location

United States

Open access

  • Yes

ISSN

2472-5552

eISSN

2472-5560

Language

English

Publication classification

C1 Refereed article in a scholarly journal

Issue

8

Publisher

SAGE PUBLICATIONS INC