2011
DOI: 10.1016/j.stem.2011.01.001
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FGF2 Sustains NANOG and Switches the Outcome of BMP4-Induced Human Embryonic Stem Cell Differentiation

Abstract: SUMMARY Here we show that as human embryonic stem (ES) cells exit the pluripotent state, NANOG can play a key role in determining lineage outcome. It has previously been reported that BMPs induce differentiation of human ES cells into extraembryonic lineages. Here we find that FGF2, acting through the MEK-ERK pathway, switches BMP4 induced human ES cell differentiation outcome to mesendoderm, characterized by the uniform expression of T (brachyury) and other primitive streak markers. We also find that MEK-ERK … Show more

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Cited by 222 publications
(255 citation statements)
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“…Unexpectedly, the pluripotency marker NANOG was repressed upon MSX2 depletion in both H1 and H9 hESCs (Supplementary information, Figure S3A-S3D). We speculated that this might be related to NANOG function in suppressing neural differentiation and in patterning different subtypes of mesoderm cells after exit of hESCs from pluripotency, as described previously [41,42]. To further confirm the role of MSX2 in hESC early differentiation and exclude the potential ambiguity brought by shRNAs, we deleted MSX2 gene in hESCs using CRISPR-CAS9 technology.…”
Section: Msx2 Is Required For Hpscs' Exit From Pluripotency and Entrymentioning
confidence: 83%
“…Unexpectedly, the pluripotency marker NANOG was repressed upon MSX2 depletion in both H1 and H9 hESCs (Supplementary information, Figure S3A-S3D). We speculated that this might be related to NANOG function in suppressing neural differentiation and in patterning different subtypes of mesoderm cells after exit of hESCs from pluripotency, as described previously [41,42]. To further confirm the role of MSX2 in hESC early differentiation and exclude the potential ambiguity brought by shRNAs, we deleted MSX2 gene in hESCs using CRISPR-CAS9 technology.…”
Section: Msx2 Is Required For Hpscs' Exit From Pluripotency and Entrymentioning
confidence: 83%
“…To further explore this possibility, we compared the global gene expression profiles of TRA-1-60 ( ĂŸ ) cells purified on various days, original HDFs, established iPSCs and differentiated progenies (endoderm, EN; mesoderm, ME; neuroectoderm, NE; and primitive streak-like mesendoderm [11][12][13][14] , PSMN from ESCs/ iPSCs using DNA microarrays ( Supplementary Fig. 4).…”
Section: Resultsmentioning
confidence: 99%
“…To induce mesoderm differentiation, cells (H9) were cultured on GBP or Matrigel with activin A for 1 d and then with BMP4 and bFGF for 3 d (8,11). Compared with cells cultured on Matrigel, cells cultured on GBP underwent a more pronounced decrease in expression of the pluripotency markers (NANOG and POU5F1) and expressed higher levels of primitive streak (T and MIXL1) and mesoderm marker genes (PDGFRA and FOXF1; SI Appendix, Fig.…”
Section: Resultsmentioning
confidence: 99%
“…Matrigel is the most widely used substratum for hPS cell propagation (5) and differentiation (6)(7)(8)(9)(10)(11)(12); it is derived from mouse sarcoma cells, and although its principal components are laminin, collagen, and entactin, Matrigel consists of up to 1,800 different proteins-including encapsulated growth factors-whose levels vary significantly from batch to batch (13). Accordingly, the contributions of Matrigel-delivered signals to specific phenotypic outcomes-self-renewal or differentiation-are difficult to characterize or control.…”
mentioning
confidence: 99%