Differentiation of induced pluripotent stem cells (iPSCs) into endoderm

Table of Contents

• Introduction
• Materials
• Media & Buffer Recipes
• Protocol
• References

Introduction

Transforming your induced pluripotent stem cells (iPSCs) into high-quality definitive endoderm (DE) lineages is a key milestone for many regenerative medicine and developmental biology projects. By mimicking the signaling environment of the early embryo, you can reliably direct these pluripotent cells toward fates that eventually form the liver, lungs, and pancreas. We know that consistency is everything in stem cell research, so we have optimized this guide to help you achieve robust and reproducible differentiation. Let's get started on generating your endodermal progenitors!

Materials

EDTA (HB5135) ROCK inhibitor Y-27632 (HB2297) CHIR 99021 (HB1261) LY 294002 hydrochloride (HB2266) FGF2 or TCB Small Molecule FGF2 Replacements Recombinant Activin A Recombinant BMP4 E8 Medium IMDM Base Medium

Vitronectin coating protein Enzymatic cell detachment solution Serum-free maintenance medium Serum-free supplement Non-Essential Amino Acids (100x) RPMI 1640 Medium F-12 Nutrient Mix Primary antibodies against GATA4 and SOX17 Secondary antibodies (see our range of validated secondary antibodies)

Media & Buffer Recipes

Aseptically combine components and filter the media before use.

Protocol

1. Maintain feeder-free iPSC cultures in E8 Medium. Perform routine passaging twice per week by detaching cells with 0.5 mM EDTA (HB5135) and plating them at a 1:6 ratio on surfaces coated with 5 µg/ml Vitronectin.
2. To begin differentiation, dissociate iPSCs using an enzymatic cell detachment solution. Seed the cells at a density of 1,000 cells per well in a 96-well plate previously coated with Vitronectin (5 µg/ml). Use E8 Medium supplemented with 10 µM ROCK inhibitor Y-27632 (HB2297) for this initial seeding.
3. On Day 1, remove the maintenance medium and replace it with freshly prepared DE 1 differentiation medium. Note: FGF2 can be replaced with stable, cost-effective small molecule FGFR1 agonists TCB-32, TCB-541, or TCB-621 to enable weekend-free feeding and significantly reduce media costs.
4. On Day 2, perform a complete medium change by replacing the DE 1 medium with freshly prepared DE 2 medium.
5. On Day 3, exchange the DE 2 medium for freshly prepared DE 3 medium to finalize the specification of the definitive endoderm.
6. On Day 4, verify successful differentiation using immunocytochemistry (ICC). Fix the cells with 4% paraformaldehyde and proceed with staining following our comprehensive ICC protocol for key endodermal markers such as SOX17 and GATA4.

References

• Fang, Y. et al. 2022. Metabolic and Epigenetic Regulation of Endoderm Differentiation. Trends in Cell biology. PMID: 34607773
• Ikonomou, L. et al. 2015. Derivation of endodermal progenitors from pluripotent stem cells. Journal of Cellular Physiology. PMID: 25160562
• McLean, A. B. et al. 2007. Activin A Efficiently Specifies Definitive Endoderm from Human Embryonic Stem Cells Only When Phosphatidylinositol 3-Kinase Signaling Is Suppressed. Stem Cells. PMID: 17204604
• Varum, S. et al. 2011. Energy Metabolism in Human pluripotent stem cells and their differentiated counterparts. PLoS ONE. PMID: 21698063
• Zorn, A. M. et al. 2009. Vertebrate Endoderm Development and Organ Formation. Annual review of cell and development biology. PMID: 19575677