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  2. Efficient and safe single-cell cloning of human pluripotent stem cells using the CEPT cocktail

Efficient and safe single-cell cloning of human pluripotent stem cells using the CEPT cocktail

  • Nat Protoc. 2022 Oct 19. doi: 10.1038/s41596-022-00753-z.
Carlos A Tristan 1 Hyenjong Hong 2 Yogita Jethmalani 2 Yu Chen 2 Claire Weber 2 Pei-Hsuan Chu 2 Seungmi Ryu 2 Vukasin M Jovanovic 2 Inae Hur 2 Ty C Voss 2 Anton Simeonov 2 Ilyas Singeç 3
Affiliations

Affiliations

  • 1 Stem Cell Translation Laboratory (SCTL), Division of Preclinical Innovation, National Center for Advancing Translational Sciences (NCATS), National Institutes of Health (NIH), Rockville, MD, USA. carlos.tristan@nih.gov.
  • 2 Stem Cell Translation Laboratory (SCTL), Division of Preclinical Innovation, National Center for Advancing Translational Sciences (NCATS), National Institutes of Health (NIH), Rockville, MD, USA.
  • 3 Stem Cell Translation Laboratory (SCTL), Division of Preclinical Innovation, National Center for Advancing Translational Sciences (NCATS), National Institutes of Health (NIH), Rockville, MD, USA. ilyassingec@gmail.com.
Abstract

Human pluripotent stem cells (hPSCs) are inherently sensitive cells. Single-cell dissociation and the establishment of clonal cell lines have been long-standing challenges. This inefficiency of cell cloning represents a major obstacle for the standardization and streamlining of gene editing in induced pluripotent stem cells for basic and translational research. Here we describe a chemically defined protocol for robust single-cell cloning using microfluidics-based cell sorting in combination with the CEPT small-molecule cocktail. This advanced strategy promotes the viability and cell fitness of self-renewing stem cells. The use of low-pressure microfluidic cell dispensing ensures gentle and rapid dispensing of single cells into 96- and 384-well plates, while the fast-acting CEPT cocktail minimizes cellular stress and maintains cell structure and function immediately after cell dissociation. The protocol also facilitates clone picking and produces genetically stable clonal cell lines from hPSCs in a safe and cost-efficient fashion. Depending on the proliferation rate of the clone derived from a single cell, this protocol can be completed in 7-14 d and requires experience with aseptic Cell Culture techniques. Altogether, the relative ease, scalability and robustness of this workflow should boost gene editing in hPSCs and leverage a wide range of applications, including cell line development (e.g., reporter and isogenic cell lines), disease modeling and applications in regenerative medicine.

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