Exosomal circ_0001583 Drives Glioblastoma Cell Advancement Through the miR-647/CKAP2L Pathway

Yuhao Zhang; Shiming Liu; Cheng Wu; Xin Gao; Hongtao Zhao; Ou Li; Kaichuang Yang; Faliang Gao

doi:10.1007/s12035-025-04875-9

Exosomal circ_0001583 Drives Glioblastoma Cell Advancement Through the miR-647/CKAP2L Pathway

Mol Neurobiol. 2025 Apr 15. doi: 10.1007/s12035-025-04875-9. Online ahead of print.

Authors

Yuhao Zhang^#¹, Shiming Liu^#¹, Cheng Wu¹, Xin Gao¹, Hongtao Zhao¹, Ou Li², Kaichuang Yang¹, Faliang Gao³

Affiliations

¹ Department of Neurosurgery, Cancer Center, Zhejiang Provincial People's Hospital (Affiliated People's Hospital), Hangzhou Medical College, No. 158, Shangtang Road, Gongshu District, Hangzhou City, 310000, Zhejiang Province, China.
² General Surgery, Cancer Center, Department of Gastrointestinal and Pancreatic Surgery, Zhejiang Provincial People's Hospital (Affiliated People's Hospital), Hangzhou Medical College, No. 158, Shangtang Road, Gongshu District, Hangzhou City, Zhejiang Province, 310000, China.
³ Department of Neurosurgery, Cancer Center, Zhejiang Provincial People's Hospital (Affiliated People's Hospital), Hangzhou Medical College, No. 158, Shangtang Road, Gongshu District, Hangzhou City, 310000, Zhejiang Province, China. Gao_faliang351216@126.com.

^# Contributed equally.

PMID: 40229458
DOI: 10.1007/s12035-025-04875-9

Abstract

Our study aimed to explore the involvement of circ_0001583 in the progression of glioblastoma (GBM). The expression levels of CircRNA in GBM were examined using the GEO database, and quantification of circ_0001583 levels was performed through qRT-PCR in both GBM tissues and cell lines. Survival analysis was conducted using Kaplan-Meier plots. The effects of circ_0001583 knockdown on cell proliferation, invasion, and glycolysis were evaluated through functional assays and measurements of glycolytic activity. Bioinformatics and reporter assays revealed that miR-647 serves as a target for circ_0001583. Tumorigenesis following circ_0001583 knockdown was investigated in a nude mouse model utilizing U251 cells. Additionally, a co-culture system with normal human astrocytes (NHAs) and GBM-conditioned medium was employed to study circ_0001583 expression and its influence on cell proliferation. The presence of circ_0001583 in normal human astrocytes was assessed using PKH67 labeling and immunofluorescence techniques. Bioinformatics analyses revealed a notable increase in the expression of circ_0001583 in GBM, correlating with metastasis. The inhibition of circ_0001583 expression led to decreased viability, proliferation, and invasive potential of GBM cells. It was found that circ_0001583 targets miR-647, which is downregulated in GBM. Silencing circ_0001583 resulted in elevated levels of miR-647. CKAP2L, a target of miR-647, showed an overexpression in GBM cases. Additionally, a positive relationship was established between circ_0001583 and CKAP2L, contrasting with a negative association with miR-647. An increase in miR-647 expression led to a decrease in CKAP2L protein levels. Rescue assays further validated that circ_0001583 influences the functions of GBM cells through the miR-647/CKAP2L pathway. In vivo investigations demonstrated that the knockdown of circ_0001583 resulted in retarded tumor growth, enhanced levels of miR-647, and diminished expression of Ki-67, CKAP2L, HK2, and LDHA within tumors. Moreover, co-culture studies involving GBM-conditioned medium demonstrated an upregulation of circ_0001583 in NHAs, which promoted cell proliferation. Our data collectively suggest that exosomal circ_0001583 promotes glioblastoma progression via the miR-647/CKAP2L pathway.

Keywords: Circ_0001583; Exosome; Glioblastoma; MiR-647/CKAP2L signaling pathway.

Grants and funding

2023M733164/China Postdoctoral Science Foundation