Identification of a new target of miR-16, vacuolar protein sorting 4a

  • Neeta Adhikari
  • , Weihua Guan
  • , Brian Capaldo
  • , Aaron J. Mackey
  • , Marjorie Carlson
  • , Sundaram Ramakrishnan
  • , Dinesha Walek
  • , Manu Gupta
  • , Adam Mitchell
  • , Peter Eckman
  • , Ranjit John
  • , Euan Ashley
  • , Paul J. Barton
  • , Jennifer L. Hall

Research output: Contribution to journalArticlepeer-review

8 Scopus citations

Abstract

Rationale: The rationale was to utilize a bioinformatics approach to identify miRNA binding sites in genes with single nucleotide mutations (SNPs) to discover pathways in heart failure (HF). Objective: The objective was to focus on the genes containing miRNA binding sites with miRNAs that were significantly altered in end-stage HF and in response to a left ventricular assist device (LVAD). Methods and Results: BEDTools v2.14.3 was used to discriminate SNPs within predicted 39UTR miRNA binding sites. A member of the miR-15/107 family, miR-16, was decreased in the circulation of end-stage HF patients and increased in response to a LVAD (p<0.001). MiR-16 decreased Vacuolar Protein Sorting 4a (VPS4a) expression in HEK 293T cells (p<0.01). The SNP rs16958754 was identified in the miR-15/107 family binding site of VPS4a which abolished direct binding of miR-16 to the 3′UTR of VPS4a (p<0.05). VPS4a was increased in the circulation of end-stage HF patients (p<0.001), and led to a decrease in the number of HEK 293T cells in vitro (p<0.001). Conclusions: We provide evidence that miR-16 decreases in the circulation of end-stage HF patients and increases with a LVAD. Modeling studies suggest that miR-16 binds to and decreases expression of VPS4a. Overexpression of VPS4a decreases cell number. Together, these experiments suggest that miR-16 and VPS4a expression are altered in end-stage HF and in response to unloading with a LVAD. This signaling pathway may lead to reduced circulating cell number in HF.

Original languageEnglish (US)
Article numbere101509
JournalPloS one
Volume9
Issue number7
DOIs
StatePublished - Jul 17 2014

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