4.6 Article

A transient post-translational modification of active site cysteine alters binding properties of the parkinsonism protein DJ-1

Journal

Publisher

ACADEMIC PRESS INC ELSEVIER SCIENCE
DOI: 10.1016/j.bbrc.2018.08.190

Keywords

Parkinson's disease; DJ-1; PARK7; S-carboxymethylcysteine; Oxidative stress

Funding

  1. Nazarbayev University Social Policy
  2. ORAU
  3. DOE Office of Science [DE-AC02-06CH11357]
  4. Michigan Economic Development Corporation
  5. Michigan Technology Tri-Corridor [085P1000817]

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Mutations in the human protein DJ-1 cause early onset of Parkinson's disease. A reactive cysteine residue) (Cys(106)) of DJ-1 is crucial for its protective function, although the underlying mechanisms are unclear. Here we show that a fraction of bacterially expressed polyhistidine-tagged human DJ-1 could not be eluted from a Ni-nitrilotriacetate (Ni-NTA) column with 150 mM imidazole. This unusually tight binding was accompanied by the appearance of blue violet color on the Ni-NTA column. We demonstrate by Xray crystallography that Cys(106) is carboxymethylated in a fraction of DJ-1 tightly bound to Ni-NTA and that the replacement of Cys(106) by serine abrogates the tight binding and the appearance of blue violet color. However, carboxymethylation of purified DJ-1 is insufficient to confer the tight binding to Ni-NTA. Moreover, when eluted protein was re-applied to the Ni-NTA column, no tight binding was observed, indicating that the formation of high affinity complex with Ni-NTA depends on a transient modification of Cys(106) that transforms into a Cys(106)-carboxymethyl adduct upon elution from Ni-NTA. We conclude that an unknown metabolite reacts with Cys(106) of DJ-1 to result in a transient post-translational modification. This modification is distinct from simple oxidation to sulfinic or sulfenic acids and confers altered binding properties to DJ-1 suggesting that it could serve as a signal for sensing oxidant stress. (C) 2018 Elsevier Inc. All rights reserved.

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