O-GlcNAcylation of Sox2 at threonine 258 regulates the self-renewal and early cell fate of embryonic stem cells

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作者
Dong Keon Kim
Jang-Seok Lee
Eun Young Lee
Hansol Jang
Suji Han
Hee Yeon Kim
In-Young Hwang
Ji-Woong Choi
Hyun Mu Shin
Hye Jin You
Hong-Duk Youn
Hyonchol Jang
机构
[1] Anticancer Resistance Branch,Department of Molecular Medicine and Biopharmaceutical Sciences
[2] Division of Rare and Refractory Cancer,Department of Cancer Biomedical Science
[3] Research Institute,undefined
[4] National Cancer Center,undefined
[5] National Creative Research Center for Epigenome Reprogramming Network,undefined
[6] Department of Biomedical Sciences,undefined
[7] Ischemic/Hypoxic Disease Institute,undefined
[8] Seoul National University College of Medicine,undefined
[9] Graduate School of Convergence Science and Technology,undefined
[10] Seoul National University,undefined
[11] National Cancer Center Graduate School of Cancer Science and Policy,undefined
[12] European Molecular Biology Laboratory,undefined
[13] Genome Biology Unit,undefined
[14] Wide River Institute of Immunology,undefined
[15] Seoul National University,undefined
[16] BK21 FOUR Biomedical Science Project & Department of Biomedical Sciences,undefined
[17] Seoul National University College of Medicine,undefined
[18] Cancer Microenvironment Branch,undefined
[19] Division of Cancer Biology,undefined
[20] Research Institute,undefined
[21] National Cancer Center,undefined
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摘要
Sox2 is a core transcription factor in embryonic stem cells (ESCs), and O-GlcNAcylation is a type of post-translational modification of nuclear-cytoplasmic proteins. Although both factors play important roles in the maintenance and differentiation of ESCs and the serine 248 (S248) and threonine 258 (T258) residues of Sox2 are modified by O-GlcNAcylation, the function of Sox2 O-GlcNAcylation is unclear. Here, we show that O-GlcNAcylation of Sox2 at T258 regulates mouse ESC self-renewal and early cell fate. ESCs in which wild-type Sox2 was replaced with the Sox2 T258A mutant exhibited reduced self-renewal, whereas ESCs with the Sox2 S248A point mutation did not. ESCs with the Sox2 T258A mutation heterologously introduced using the CRISPR/Cas9 system, designated E14-Sox2TA/WT, also exhibited reduced self-renewal. RNA sequencing analysis under self-renewal conditions showed that upregulated expression of early differentiation genes, rather than a downregulated expression of self-renewal genes, was responsible for the reduced self-renewal of E14-Sox2TA/WT cells. There was a significant decrease in ectodermal tissue and a marked increase in cartilage tissue in E14-Sox2TA/WT-derived teratomas compared with normal E14 ESC-derived teratomas. RNA sequencing of teratomas revealed that genes related to brain development had generally downregulated expression in the E14-Sox2TA/WT-derived teratomas. Our findings using the Sox2 T258A mutant suggest that Sox2 T258 O-GlcNAc has a positive effect on ESC self-renewal and plays an important role in the proper development of ectodermal lineage cells. Overall, our study directly links O-GlcNAcylation and early cell fate decisions.
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页码:1759 / 1768
页数:9
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