Journal of Southern Medical University ›› 2025, Vol. 45 ›› Issue (11): 2320-2329.doi: 10.12122/j.issn.1673-4254.2025.11.04
Chen JIN(
), Jingping LIU, Bo LIU, Xiyun FEI, Yuxiang LIAO(
)
Received:2025-04-02
Online:2025-11-20
Published:2025-11-28
Contact:
Yuxiang LIAO
E-mail:Jinchen@csu.edu.cn;lyxxysw@126.com
Chen JIN, Jingping LIU, Bo LIU, Xiyun FEI, Yuxiang LIAO. circ_EPHB4 synergizes with YTHDF3 to promote glioma progression via m6A-dependent stabilization of Wnt3[J]. Journal of Southern Medical University, 2025, 45(11): 2320-2329.
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URL: https://www.j-smu.com/EN/10.12122/j.issn.1673-4254.2025.11.04
| Gene | Forward Primer (5'-3') | Reverse Primer (5'-3') |
|---|---|---|
| circ_EPHB4 | CAGAGAGCGCATCCGCAATTT | AAAGAAGGTGCGCCCACGGTT |
| Zeb1 | AACAGTGAGCGACCTTCATT | AGAGCGCAGAGAAGGAGAGTT |
| GAPDH | AGAGCGCAGAGAAGGAGAUTT | AAAGAGCGAGAGAAGGAGAT |
Tab.1 Primer sequences for RT-qPCR of the target and housekeeping genes
| Gene | Forward Primer (5'-3') | Reverse Primer (5'-3') |
|---|---|---|
| circ_EPHB4 | CAGAGAGCGCATCCGCAATTT | AAAGAAGGTGCGCCCACGGTT |
| Zeb1 | AACAGTGAGCGACCTTCATT | AGAGCGCAGAGAAGGAGAGTT |
| GAPDH | AGAGCGCAGAGAAGGAGAUTT | AAAGAGCGAGAGAAGGAGAT |
Fig.2 circ_EPHB4 promotes glioma cell migration, invasion, and EMT. A: qRT-PCR of circ_EPHB4 expression in glioma cells after transfection with circ_EPHB4-overexpressing plasmids or circ_EPHB4 siRNA (**P<0.01). B: Scratch wound healing assay for evaluating glioma cell migration ability following circ_EPHB4 overexpression or knockdown (scale bar=100 μm). C: Transwell invasion assay for assessing glioma cell invasion ability after transfection (scale bar=50 μm). D: Western blotting of EMT-related proteins (E-cadherin, N-cadherin and vimentin) in glioma cells following circ_EPHB4 overexpression or knockdown. Data are presented as Mean±SD from 3 independent experiments. *P<0.05 vs siRNA NC; #P<0.05 vs pcDNA3.1 NC.
Fig3 circ_EPHB4 promotes tumorigenesis and metastasis of glioma cells in nude mice. A: Number of pulmonary metastatic nodules in each group. B: Subcutaneous tumor volume at different time points in each group. C: Subcutaneous tumor weight in each group (*P<0.05, **P<0.01, ***P<0.001). D: qRT-PCR analysis of mRNA expressions of E-cadherin, N-cadherin, vimentin) in subcutaneous tumors. E: Immunohistochemicalanalysis of protein expressions of E-cadherin, N-cadherin, and vimentin in subcutaneous tumors from each group. **P<0.01, ***P<0.001 vs siRNA NC group; ##P<0.01, ### P<0.001 vs pcDNA3.1 NC group.
Fig.4 circ_EPHB4 promotes glioma cell metastasis by upregulating Wnt3 expression. A: Overexpression of circ_EPHB4 enhances Wnt3 expression, and circ_EPHB4 knockdown suppresses Wnt3 expression. B: Scratch wound healing assay for evaluating the effect of Wnt3 knockdown on glioma cell migration following circ_EPHB4 overexpression (scale bar=50 μm). C: Transwell invasion assay for assessing the impact of Wnt3 knockdown on invasion ability of circ_EPHB4-overexpressing glioma cells (scale bar=50 μm). D: Western blotting for evaluating the effects of Wnt3 knockdown on expressions of E-cadherin, N-cadherin and vimentin in circ_EPHB4-overexpressing glioma cells.
Fig.5 YTHDF3 enhances Wnt3 mRNA stability in an m6A-dependent manner. A: Direct interaction between YTHDF3 and Wnt3 mRNA in U3T3 and SHG44 cells. B: Effect of YTHDF3 knockdown on Wnt3 expression. C: Positive correlation between YTHDF3 and Wnt3 expression in the StarBase database. D: Effect of circ_EPHB4 on the interaction between YTHDF3 and Wnt3 RNA. E: Effect of combined knockdown of circ_EPHB4 and YTHDF3 on Wnt3 mRNA expression. *P<0.05, **P<0.01, ***P<0.001.
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