Tyrosine‐Targeted Spin Labeling and EPR Spectroscopy: An Alternative Strategy for Studying Structural Transitions in Proteins

Abstract

Such a difficulty was recently encountered in the study of a small and flexible chloroplast protein CP12 from the green alga Chlamydomonas reinhardtii by spin-labeling EPR spectroscopy. In this organism, CP12 contains four cysteine residues involved in two disulfide bridges in its oxidized state. Although the introduction of spin labels at the two cysteine residues of the C-terminal disulfide bridge enabled us to identify a new role of the partner protein glyceraldehyde 3-phosphate dehydrogenase (GAPDH), it precluded the direct study of the complex formation GAPDH/CP12. [4] To overcome this difficulty, grafting of the nitroxide probe to residues other than cysteines is required. One strategy using a genetically encoded unnatural amino acid has been recently proposed. [5] The incorporation of such unnatural amino acids relies, however, on a rather complex strategy involving an orthogonal tRNA/aminoacyl-tRNA synthetase pair specific for the unnatural amino acid. As such a strategy is difficult to set up, we propose an alternative method consisting of selectively targeting residues other than cysteines with a nitroxide probe. Bioconjugation of small molecules to protein residues is very challenging, and several reactions have recently been proposed to target specific residues selectively. [6] In particular, efforts have been paid to modify the aromatic amino acid side chains of tryptophan [7] and tyrosine. [8] Among them, a threecomponent Mannich-type reaction has been developed that allows the modification of tyrosine under mild, biocompatible, and metal-free conditions. [8a] Inspired by these recent studies, we present the selective grafting of a nitroxide probe to tyrosine by using the Mannich-type reaction on CP12, a protein bearing only one natural tyrosine residue. This unique tyrosine residue, located at position 78 in the sequence of a total of 80 amino acids, makes this protein an ideal candidate for demonstrating the feasibility of tyrosine-targeted spin