| Literature DB >> 29273502 |
Dongtak Jeong1, Jimeen Yoo1, Philyoung Lee1, Sacha V Kepreotis1, Ahyoung Lee1, Christine Wahlquist2, Brian D Brown3, Changwon Kho1, Mark Mercola2, Roger J Hajjar4.
Abstract
MicroRNAs are promising therapeutic targets, because their inhibition has the potential to normalize gene expression in diseased states. Recently, our group found that miR-25 is a key SERCA2a regulating microRNA, and we showed that multiple injections of antagomirs against miR-25 enhance cardiac contractility and function through SERCA2a restoration in a murine heart failure model. However, for clinical application, a more stable suppressor of miR-25 would be desirable. Tough Decoy (TuD) inhibitors are emerging as a highly effective method for microRNA inhibition due to their resistance to endonucleolytic degradation, high miRNA binding affinity, and efficient delivery. We generated a miR-25 TuD inhibitor and subcloned it into a cardiotropic AAV9 vector to evaluate its efficacy. The AAV9 TuD showed selective inhibition of miR-25 in vitro cardiomyoblast culture. In vivo, AAV9-miR-25 TuD delivered to the murine pressure-overload heart failure model selectively decreased expression of miR-25, increased levels of SERCA2a protein, and ameliorated cardiac dysfunction and fibrosis. Our data indicate that miR-25 TuD is an effective long-term suppressor of miR-25 and a promising therapeutic candidate to treat heart failure.Entities:
Keywords: AAV9; SERCA2a; Tough Decoy; TuD; calcium signaling; gene therapy; heart failure; miR-25; miRNA
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Year: 2017 PMID: 29273502 PMCID: PMC5910658 DOI: 10.1016/j.ymthe.2017.11.014
Source DB: PubMed Journal: Mol Ther ISSN: 1525-0016 Impact factor: 11.454