piRNA PROPER Suppresses DUSP1 Translation by Targeting N6‐Methyladenosine‐Mediated RNA Circularization to Promote Oncogenesis of Prostate Cancer

Author:

Ben Shuai1234,Ding Zhutao23,Xin Junyi5,Li Feng6,Cheng Yifei23,Chen Silu23,Fan Lulu23,Zhang Qin7,Li Shuwei23,Du Mulong8,Zhang Zhengdong23,Wei Gong‐Hong79,Cheng Gong10,Wang Meilin123ORCID

Affiliation:

1. The Affiliated Suzhou Hospital of Nanjing Medical University Suzhou Municipal Hospital Gusu School Nanjing Medical University Suzhou 215002 China

2. Department of Environmental Genomics Jiangsu Key Laboratory of Cancer Biomarkers Prevention and Treatment Collaborative Innovation Center for Cancer Personalized Medicine School of Public Health Nanjing Medical University Nanjing 211166 China

3. Department of Genetic Toxicology The Key Laboratory of Modern Toxicology of Ministry of Education Center for Global Health School of Public Health Nanjing Medical University Nanjing 211166 China

4. Department of Ophthalmology Shanghai General Hospital School of Medicine Shanghai Jiao Tong University Shanghai 200080 China

5. Department of Bioinformatic School of Biomedical Engineering and Informatics Nanjing Medical University Nanjing Jiangsu 211166 China

6. State Key Laboratory of Reproductive Medicine Nanjing Medical University Nanjing Jiangsu 211100 China

7. Disease Networks Research Unit Faculty of Biochemistry and Molecular Medicine & Biocenter Oulu University of Oulu Oulu 90220 Finland

8. Department of Biostatistics Center for Global Health School of Public Health Nanjing Medical University Nanjing 211166 China

9. Fudan University Shanghai Cancer Center & MOE Key Laboratory of Metabolism and Molecular Medicine and Department of Biochemistry and Molecular Biology of School of Basic Medical Sciences Shanghai Medical College of Fudan University Shanghai 200032 China

10. Department of Urology The First Affiliated Hospital of Nanjing Medical University & Jiangsu Province People's Hospital Nanjing 210029 China

Abstract

AbstractGenetic and epigenetic alterations occur in many physiological and pathological processes. The existing knowledge regarding the association of PIWI‐interacting RNAs (piRNAs) and their genetic variants on risk and progression of prostate cancer (PCa) is limited. In this study, three genome‐wide association study datasets are combined, including 85,707 PCa cases and 166,247 controls, to uncover genetic variants in piRNAs. Functional investigations involved manipulating piRNA expression in cellular and mouse models to study its oncogenetic role in PCa. A specific genetic variant, rs17201241 is identified, associated with increased expression of PROPER (piRNA overexpressed in prostate cancer) in tumors and are located within the gene, conferring an increased risk and malignant progression of PCa. Mechanistically, PROPER coupled with YTHDF2 to recognize N6‐methyladenosine (m6A) and facilitated RNA‐binding protein interactions between EIF2S3 at 5′‐untranslated region (UTR) and YTHDF2/YBX3 at 3′‐UTR to promote DUSP1 circularization. This m6A‐dependent mRNA‐looping pattern enhanced DUSP1 degradation and inhibited DUSP1 translation, ultimately reducing DUSP1 expression and promoting PCa metastasis via the p38 mitogen‐activated protein kinase (MAPK) signaling pathway. Inhibition of PROPER expression using antagoPROPER effectively suppressed xenograft growth, suggesting its potential as a therapeutic target. Thus, targeting piRNA PROPER‐mediated genetic and epigenetic fine control is a promising strategy for the concurrent prevention and treatment of PCa.

Publisher

Wiley

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