Identification of oxidative modifications of hemopexin and their predicted physiological relevance

Peter Hahl; Rachel Hunt; Edward S Bjes; Andrew Skaff; Andrew Keightley; Ann Smith

doi:10.1074/jbc.M117.783951

Identification of oxidative modifications of hemopexin and their predicted physiological relevance

J Biol Chem. 2017 Aug 18;292(33):13658-13671. doi: 10.1074/jbc.M117.783951. Epub 2017 Jun 8.

Authors

Peter Hahl¹, Rachel Hunt¹, Edward S Bjes¹, Andrew Skaff¹, Andrew Keightley¹, Ann Smith²

Affiliations

¹ From the Department of Molecular Biology and Biochemistry, School of Biological Sciences, University of Missouri-Kansas City, Kansas City, Missouri 64110-2239.
² From the Department of Molecular Biology and Biochemistry, School of Biological Sciences, University of Missouri-Kansas City, Kansas City, Missouri 64110-2239 smithan@umkc.edu.

Abstract

Hemopexin protects against heme toxicity in hemolytic diseases and conditions, sepsis, and sickle cell disease. This protection is sustained by heme-hemopexin complexes in biological fluids that resist oxidative damage during heme-driven inflammation. However, apo-hemopexin is vulnerable to inactivation by reactive nitrogen (RNS) and oxygen species (ROS) that covalently modify amino acids. The resultant nitration of amino acids is considered a specific effect reflecting biological events. Using LC-MS, we discovered low endogenous levels of tyrosine nitration in the peptide YYCFQGNQFLR in the heme-binding site of human hemopexin, which was similarly nitrated in rabbit and rat hemopexins. Immunoblotting and selective reaction monitoring were used to quantify tyrosine nitration of in vivo samples and when hemopexin was incubated in vitro with nitrating nitrite/myeloperoxidase/glucose oxidase. Significantly, heme binding by hemopexin declined as tyrosine nitration proceeded in vitro Three nitrated tyrosines reside in the heme-binding site of hemopexin, and we found that one, Tyr-199, interacts directly with the heme ring D propionate. Investigating the oxidative modifications of amino acids after incubation with tert-butyl hydroperoxide and hypochlorous acid in vitro, we identified additional covalent oxidative modifications on four tyrosine residues and one tryptophan residue of hemopexin. Importantly, three of the four modified tyrosines, some of which have more than one modification, cluster in the heme-binding site, supporting a hierarchy of vulnerable amino acids. We propose that during inflammation, apo-hemopexin is nitrated and oxidated in niches of the body containing activated RNS- and ROS-generating immune and endothelial cells, potentially impairing hemopexin's protective extracellular antioxidant function.

Keywords: covalent modification; glycoprotein; hemopexin; mass spectrometry (MS); proteomics; reactive nitrogen species (RNS); reactive oxygen species (ROS); tyrosine nitration.

Publication types

Comparative Study
Research Support, Non-U.S. Gov't
Research Support, N.I.H., Extramural

MeSH terms

Amino Acid Sequence
Animals
Apoproteins / chemistry
Apoproteins / isolation & purification
Apoproteins / metabolism
Binding Sites
Chromatography, High Pressure Liquid
Conserved Sequence
Heme / chemistry
Heme / metabolism
Hemopexin / chemistry
Hemopexin / isolation & purification
Hemopexin / metabolism*
Humans
Kinetics
Ligands
Models, Molecular*
Molecular Structure
Oxidation-Reduction
Protein Conformation
Rabbits
Rats
Reactive Oxygen Species / chemistry
Reactive Oxygen Species / metabolism
Species Specificity
Tandem Mass Spectrometry
Tryptophan / chemistry
Tyrosine / chemistry

Substances

Apoproteins
Ligands
Reactive Oxygen Species
Tyrosine
Heme
Tryptophan
Hemopexin

Associated data

PDB/1QHU

Grants and funding

R21 DK064363/DK/NIDDK NIH HHS/United States