Chemical conversion of human conventional PSCs to TSCs following transient naive gene activation

Author:

Zorzan Irene1ORCID,Betto Riccardo Massimiliano1ORCID,Rossignoli Giada2ORCID,Arboit Mattia2ORCID,Drusin Andrea2,Corridori Clelia2ORCID,Martini Paolo3ORCID,Martello Graziano2ORCID

Affiliation:

1. Department of Molecular Medicine, Medical School University of Padua Padua Italy

2. Department of Biology University of Padua Padua Italy

3. Department of Molecular and Translational Medicine University of Brescia Brescia Italy

Abstract

AbstractIn human embryos, naive pluripotent cells of the inner cell mass (ICM) generate epiblast, primitive endoderm and trophectoderm (TE) lineages, whence trophoblast cells derive. In vitro, naive pluripotent stem cells (PSCs) retain this potential and efficiently generate trophoblast stem cells (TSCs), while conventional PSCs form TSCs at low efficiency. Transient histone deacetylase and MEK inhibition combined with LIF stimulation is used to chemically reset conventional to naive PSCs. Here, we report that chemical resetting induces the expression of both naive and TSC markers and of placental imprinted genes. A modified chemical resetting protocol allows for the fast and efficient conversion of conventional PSCs into TSCs, entailing shutdown of pluripotency genes and full activation of the trophoblast master regulators, without induction of amnion markers. Chemical resetting generates a plastic intermediate state, characterised by co‐expression of naive and TSC markers, after which cells steer towards one of the two fates in response to the signalling environment. The efficiency and rapidity of our system will be useful to study cell fate transitions and to generate models of placental disorders.

Funder

H2020 European Research Council

Fondazione Telethon

Giovanni Armenise-Harvard Foundation

Publisher

Springer Science and Business Media LLC

Subject

Genetics,Molecular Biology,Biochemistry

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