Substitution of histidine 30 by asparagine in manganese superoxide dismutase alters biophysical properties and supports proliferation in a K562 leukemia cell line

Author:

Bonetta RosalinORCID,Hunter Gary J.,Trinh Chi H.,Borowski Tomasz,Fenech Anthony G.,Kulp Maria,Tabares Leandro C.,Un Sun,Hunter Thérèse

Abstract

AbstractWe have generated a mutant of C. elegans manganese superoxide dismutase at histidine 30 by site-directed mutagenesis. The structure was solved at a resolution of 1.52 Å by X-ray crystallography (pdb: 6S0D). His30 was targeted, as it forms as a gateway residue at the top of the solvent access funnel to the active site, together with Tyr34. In the wild-type protein, these gateway residues are involved in the hydrogen-bonding network providing the protons necessary for the catalytic reaction at the metal center. However, biophysical characterization and cell viability experiments reveal that a mutation from histidine to asparagine in the H30N mutant modifies metal selectivity in the protein, favoring the uptake of iron over manganese in minimal media conditions, alters active-site coordination from the characteristic trigonal bipyramidal to octahedral geometry, and encourages cellular proliferation in K562 cells, when added exogenously to the cells.

Funder

French Infrastructure for Integrated Structural Biology

Faculty of Medicine and Surgery, University of Malta

French Embassy to Malta, Malta Council for Science and Technology (MT), CNRS

COST Action CM1305

Wellcome Trust

Publisher

Springer Science and Business Media LLC

Subject

General Medicine,Biophysics

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