Stem Cell Research & Therapy (Feb 2025)

OCT4 translationally promotes AKT signaling as an RNA-binding protein in stressed pluripotent stem cells

  • Wenjie Chen,
  • Xinyu Chen,
  • Cheng Chen,
  • Shiqi She,
  • Xia Li,
  • Lina Shan,
  • Xiaobing Zhang,
  • Songsong Dan,
  • Yisha Wang,
  • Yan-Wen Zhou,
  • Qingyi Cao,
  • Wenxin Wang,
  • Jianwen Hu,
  • Yaxun Wei,
  • Yaqiang Xue,
  • Yi Zhang,
  • Songying Zhang,
  • Ying-Jie Wang,
  • Bo Kang

DOI
https://doi.org/10.1186/s13287-025-04229-1
Journal volume & issue
Vol. 16, no. 1
pp. 1 – 26

Abstract

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Abstract Background Despite numerous studies addressing the molecular mechanisms by which pluripotent stem cells (PSCs) maintain self-renewal and pluripotency under normal culture conditions, the fundamental question of how PSCs manage to survive stressful conditions remains largely unresolved. Post-transcriptional/translational regulation emerges to be vital for PSCs, but how PSCs coordinate and balance their survival and differentiation at translational level under extrinsic and intrinsic stress conditions is unclear. Methods The high-throughput sequencing of cross-linking immunoprecipitation cDNA library (HITS-CLIP) was employed to decipher the genome-wide OCT4-RNA interactome in human PSCs, a combined RNC-seq/RNA-seq analysis to assess the role of OCT4 in translational regulation of hypoxic PSCs, and an OCT4-protein interactome to search for OCT4 binding partners that regulate cap-independent translation initiation. By taking the Heterozygous Knocking In N-terminal Tags (HKINT) approach that specifically disrupts the 5′-UTR secondary structure and tagging its protein product of the mRNA from one allele while leaving that from the other allele intact, we examined the effect of disrupting the OCT4/5′-UTR interaction on translation of AKT1 mRNA. Results We revealed OCT4 as a bona fide RNA-binding protein (RBP) in human PSCs that bound to the 5′-UTR, 3′-UTR and CDS regions of mRNAs. Multiple known proteins participating in IRES-mediated translation initiation were detected in the OCT4-protein interactome, and a combined RNC-seq/RNA-seq analysis further confirmed a crucial role of OCT4 in translational regulation of PSCs in response to hypoxic stress. Remarkably, OCT4 bound to the GC-rich elements in the 5′-UTR of AKT1 and multiple PI3K/AKT-pathway-gene mRNAs, and promoted their translation initiation via IRES-mediated pathways under stress conditions. Specifically disrupting the AKT1 mRNA 5′-UTR structure and the OCT4/5′-UTR interaction by the HKINT approach significantly reduced the translation level of AKT1 that led to a higher susceptibility of PSCs to oxidative stress-induced apoptotic death and prioritized differentiation toward ectoderm and endoderm. Conclusions Our results reveal OCT4 as an anti-stress RBP for translational regulation that critically coordinates the survival and differentiation of PSCs in response to various stressors.

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