Essential role of STAT3 for embryonic stem cell pluripotency
STAT3 Transcription Factor
0303 health sciences
Stem Cells
Gene Expression Regulation, Developmental
Cell Differentiation
DNA-Binding Proteins
Mice
03 medical and health sciences
Trans-Activators
Animals
Cell Division
Cells, Cultured
Signal Transduction
DOI:
10.1073/pnas.96.6.2846
Publication Date:
2002-07-26T14:39:15Z
AUTHORS (5)
ABSTRACT
Propagation of mouse embryonic stem (ES) cells
in vitro
requires exogenous leukemia inhibitory factor (LIF) or related cytokines. Potential downstream effectors of the LIF signal in ES cells include kinases of the Src, Jak, and mitogen-activated protein families and the signal transducer and transcriptional activator STAT3. Activation of nuclear STAT3 and the ability of ES cells to grow as undifferentiated clones were monitored during LIF withdrawal. A correlation was found between levels of STAT3 activity and maintenance of an undifferentiated phenotype at clonal density. In contrast, variation in STAT3 activity did not affect cell proliferation. The requirement for STAT3 was analyzed by targeted mutagenesis in ES cell lines exhibiting different degrees of LIF dependency. An insertional mutation was devised that abrogated
Stat3
gene expression but could be reversed by Cre recombination-mediated excision. ES cells heterozygous for the
Stat3
mutation could be isolated only from E14 cells, the line least dependent on LIF for self-renewal. Targeted clones isolated from other ES cell lines were invariably trisomic for chromosome 11, which carries the
Stat3
locus, and retained normal levels of activated STAT3. Cre-regulated reduction of
Stat3
gene copy number in targeted, euploid E14 clones resulted in dose-dependent losses of STAT3 activity and the efficiency of self-renewal without commensurate changes in cell cycle progression. These results demonstrate an essential role for a critical amount of STAT3 in the maintenance of an undifferentiated ES cell phenotype.
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