A multi-omics integrative analysis based on CRISPR screens re-defines the pluripotency regulatory network in ESCs

Author:

Jian Rui1ORCID,Ruan Yan1,Wang Jiaqi1,Yu Meng2,Wang Fengsheng1,Wang Jiangjun2,Xu Yixiao3,Liu Lianlian2,Cheng Yuda2,Yang Ran1,Zhang Chen1,Yang Yi4,Wang JiaLi2,Wu Wei5,Chen Guangxing1,Huang Yi4,Tian Yanping2ORCID,Zhang Junlei1ORCID

Affiliation:

1. Army Medical University

2. Laboratory of Stem Cell & Developmental Biology, Department of Histology and Embryology, Army Medical University

3. Southwest hospital/southwest eye hospital, the First Hospital Affiliated to Army Medical University

4. Experimental Center of Basic Medicine, College of Basic Medical Sciences, Army Medical University

5. Thoracic Surgery Department, Southwest Hospital, the First Hospital Affiliated to Army Medical University

Abstract

Abstract A comprehensive and precise definition of the pluripotency gene regulatory network (PGRN) is crucial for clarifying the regulatory mechanisms in embryonic stem cells (ESCs). Here, after a CRISPR/Cas9-based functional genomics screen and integrative analysis with other functional genomes, transcriptomes, proteomes and epigenome data, an expanded pluripotency-associated gene set is obtained, and a new PGRN with nine sub-classes is constructed. By integrating the DNA binding, epigenetic modification, chromatin conformation, and RNA expression profiles, the PGRN is resolved to six functionally independent transcriptional modules (CORE, MYC, PAF, PRC, PCGF and TBX). Spatiotemporal transcriptomics reveal activated CORE/MYC/PAF module activity and repressed PRC/PCGF/TBX module activity in both mouse ESCs (mESCs) and pluripotent cells of early embryos. Moreover, this module activity pattern is found to be shared by human ESCs (hESCs) and cancers. Thus, our results provide novel insights into elucidating the molecular basis of ESC pluripotency.

Publisher

Research Square Platform LLC

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