Data in Brief (Dec 2018)

Proteomic profiling data of HEK293 proteins bound to human recombinant renalases-1 and -2

  • Valerii I. Fedchenko,
  • Arthur T. Kopylov,
  • Olga A. Buneeva,
  • Alexei A. Kaloshin,
  • Victor G. Zgoda,
  • Alexei E. Medvedev

Journal volume & issue
Vol. 21
pp. 1477 – 1482

Abstract

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Renalase (RNLS) is a recently discovered protein involved in blood pressure regulation. It exists both as an intracellular catalytically active flavoprotein (EC 1.6.3.5 dihydro-NAD(P):oxygen oxidoreductase) and an extracellular protein that demonstrates various cell protecting effects. Using a twenty-membered peptide corresponding to the residues 220–239 of the renalase sequence (RP-220) and the HK-2 cell line Wang et al. identified a renalase-binding protein, which was considered as a receptor for extracellular renalase crucial for MAPK signaling (Wang et al., 2015) [1]. In this study we have investigated profiles of renalase binding proteins in HEK293 cells by using affinity based proteomic profiling with full-length recombinant human RNLS-1 and human RNLS-2 as affinity ligands followed by analysis of bound proteins by liquid chromatography-mass spectrometry. Both renalases (RNLS-1 and RNLS-2) contain the RP-220 sequence (residues 220–239) but differ in their C-terminal region (residues 293–342 and 293–325, respectively). Profiling of HEK293 proteins resulted in identification of two different sets of proteins specifically bound to RNLS-1 and RNLS-2, respectively. We thus demonstrate that the C-terminal region is crucial for specific binding of renalase to its targets and/or receptors. Keywords: Renalase, Renalase-binding protein, RP-220 peptide, Affinity-based proteomic profiling, LC–MS