Human surface ectoderm and amniotic ectoderm are sequentially specified according to cellular density

Author:

Nakanoh Shota12ORCID,Sham Kendig1ORCID,Ghimire Sabitri1,Mohorianu Irina1ORCID,Rayon Teresa2ORCID,Vallier Ludovic134ORCID

Affiliation:

1. Wellcome-MRC Cambridge Stem Cell Institute, Jeffrey Cheah Biomedical Centre, University of Cambridge, Cambridge CB2 0AW, UK.

2. Epigenetics & Signalling Programmes, Babraham Institute, Cambridge CB22 3AT, UK.

3. Berlin Institute of Health Centre for Regenerative Therapies, Charité - Universitätsmedizin Berlin, Berlin 13353, Germany.

4. Max Planck Institute for Molecular Genetics, Berlin 14195, Germany.

Abstract

Mechanisms specifying amniotic ectoderm and surface ectoderm are unresolved in humans due to their close similarities in expression patterns and signal requirements. This lack of knowledge hinders the development of protocols to accurately model human embryogenesis. Here, we developed a human pluripotent stem cell model to investigate the divergence between amniotic and surface ectoderms. In the established culture system, cells differentiated into functional amnioblast-like cells. Single-cell RNA sequencing analyses of amnioblast differentiation revealed an intermediate cell state with enhanced surface ectoderm gene expression. Furthermore, when the differentiation started at the confluent condition, cells retained the expression profile of surface ectoderm. Collectively, we propose that human amniotic ectoderm and surface ectoderm are specified along a common nonneural ectoderm trajectory based on cell density. Our culture system also generated extraembryonic mesoderm–like cells from the primed pluripotent state. Together, this study provides an integrative understanding of the human nonneural ectoderm development and a model for embryonic and extraembryonic human development around gastrulation.

Publisher

American Association for the Advancement of Science (AAAS)

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