| Literature DB >> 33293428 |
Yinmin Gu1,2, Shaoxi Niu3, Yang Wang4, Liqiang Duan4, Yongbo Pan4, Zhou Tong4, Xu Zhang3, Zhenyu Yang1,2, Bo Peng1,2, Xiaodong Wang1,2, Xiaoqi Han5, Yuxin Li6, Tianyou Cheng4, Yajuan Liu4, Lina Shang4, Tongfeng Liu5, Xiwang Yang5, Minxuan Sun1, Siyuan Jiang1, Chang Zhang1, Ning Zhang7, Qinong Ye8, Shan Gao9,4.
Abstract
Aberrant N 6-methyladenosine (m6A) modification has emerged as a driver of tumor initiation and progression, yet how long noncoding RNAs (lncRNA) are involved in the regulation of m6A remains unknown. Here we utilize data from 12 cancer types from The Cancer Genome Atlas to comprehensively map lncRNAs that are potentially deregulated by DNA methylation. A novel DNA methylation-deregulated and RNA m6A reader-cooperating lncRNA (DMDRMR) facilitated tumor growth and metastasis in clear cell renal cell carcinoma (ccRCC). Mechanistically, DMDRMR bound insulin-like growth factor 2 mRNA-binding protein 3 (IGF2BP3) to stabilize target genes, including the cell-cycle kinase CDK4 and three extracellular matrix components (COL6A1, LAMA5, and FN1), by specifically enhancing IGF2BP3 activity on them in an m6A-dependent manner. Consequently, DMDRMR and IGF2BP3 enhanced the G1-S transition, thus promoting cell proliferation in ccRCC. In patients with ccRCC, high coexpression of DMDRMR and IGF2BP3 was associated with poor outcomes. Our findings reveal that DMDRMR cooperates with IGF2BP3 to regulate target genes in an m6A-dependent manner and may represent a potential diagnostic, prognostic, and therapeutic target in ccRCC. SIGNIFICANCE: This study demonstrates that the lncRNA DMDRMR acts as a cofactor for IGF2BP3 to stabilize target genes in an m6A-dependent manner, thus exerting essential oncogenic roles in ccRCC. ©2020 American Association for Cancer Research.Entities:
Year: 2020 PMID: 33293428 DOI: 10.1158/0008-5472.CAN-20-1619
Source DB: PubMed Journal: Cancer Res ISSN: 0008-5472 Impact factor: 12.701