Divergent lncRNA MYMLR regulates MYC by eliciting DNA looping and promoter-enhancer interaction.
Taisuke KajinoTeppei ShimamuraShuyi GongKiyoshi YanagisawaLisa IdaMasahiro NakatochiSebastian GriesingYukako ShimadaKeiko KanoMotoshi SuzukiSatoru MiyanoTakashi TakahashiPublished in: The EMBO journal (2019)
Long non-coding RNAs (lncRNAs) function in a wide range of processes by diverse mechanisms, though their roles in regulation of oncogenes and/or tumor suppressors remain rather elusive. We performed a global search for lncRNAs affecting MYC activity using a systems biology-based approach with a K supercomputer and the GIMLET algorism based on local distance correlations. Consequently, MYMLR was identified and experimentally shown to maintain MYC transcriptional activity and cell cycle progression despite the low levels of expression. A proteomic search for MYMLR-binding proteins identified PCBP2, while it was also found that MYMLR places a 557-kb upstream enhancer region in the proximity of the MYC promoter in cooperation with PCBP2. These findings implicate a crucial role for MYMLR in regulation of the archetypical oncogene MYC and warrant future studies regarding the involvement of low copy number lncRNAs in regulation of other crucial oncogenes and tumor suppressor genes.
Keyphrases
- transcription factor
- genome wide identification
- cell cycle
- long non coding rna
- copy number
- poor prognosis
- dna methylation
- genome wide
- mitochondrial dna
- gene expression
- binding protein
- cell proliferation
- network analysis
- current status
- oxidative stress
- cell free
- single molecule
- bioinformatics analysis
- circulating tumor cells