In vitro maturation of NiSOD reveals a role for cytoplasmic histidine in processing and metalation

Author:

Basak Priyanka1,Cabelli Diane E2,Chivers Peter T3ORCID,Farquhar Erik R4ORCID,Maroney Michael J15ORCID

Affiliation:

1. Department of Chemistry, University of Massachusetts , Amherst , MA 01003 , USA

2. Department of Chemistry, Brookhaven National Laboratory , Upton, NY 11973 , USA

3. Departments of Biosciences and Chemistry, Durham University , Durham, DH1 3LE , UK

4. National Synchrotron Light Source-II, Brookhaven National Laboratory , Upton, NY 11973 , USA

5. Program in Molecular and Cellular Biology, University of Massachusetts , Amherst, MA 01003 , USA

Abstract

Abstract The importance of cellular low molecular weight ligands in metalloenzyme maturation is largely unexplored. Maturation of NiSOD requires post-translational N-terminal processing of the proenzyme, SodN, by its cognate protease, SodX. Here we provide evidence for the participation of L-histidine in the protease-dependent maturation of nickel-dependent superoxide dismutase (NiSOD) from Streptomyces coelicolor. In vitro studies using purified proteins cloned from S. coelicolor and overexpressed in E. coli support a model where a ternary complex formed between the substrate (SodN), the protease (SodX) and L-Histidine creates a novel Ni-binding site that is capable of the N-terminal processing of SodN and specifically incorporates Ni into the apo-NiSOD product. Thus, L-Histidine serves many of the functions associated with a metallochaperone or, conversely, eliminates the need for a metallochaperone in NiSOD maturation.

Funder

National Institutes of Health

Publisher

Oxford University Press (OUP)

Subject

Metals and Alloys,Biochemistry,Biomaterials,Biophysics,Chemistry (miscellaneous)

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