4.7 Article

A GFP-based ratiometric sensor for cellular methionine oxidation

Journal

TALANTA
Volume 243, Issue -, Pages -

Publisher

ELSEVIER
DOI: 10.1016/j.talanta.2022.123332

Keywords

Fluorescence sensor; GFP; Methionine oxidation; Methionine sulfoxide; GEPMO; Oxidative stress

Funding

  1. German Research Foundation [RTG 2155]
  2. NIH [GM121375]
  3. University Hospital Jena IZKF [MSP 11]

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This study introduces a genetically encoded probe for methionine oxidation using super-folder green fluorescent protein as a sensor, which enables the detection of methionine oxidation in living cells and organisms.
Methionine oxidation is a reversible post-translational protein modification, affecting protein function, and implicated in aging and degenerative diseases. The detection of accumulating methionine oxidation in living cells or organisms, however, has not been achieved. Here we introduce a genetically encoded probe for methionine oxidation (GEPMO), based on the super-folder green fluorescent protein (sfGFP), as a specific, versatile, and integrating sensor for methionine oxidation. Placed at amino-acid position 147 in an otherwise methionine-less sfGFP, the oxidation of this specific methionine to methionine sulfoxide results in a ratiometric fluorescence change when excited with -400 and -470 nm light. The strength and homogeneity of the sensor expression is suited for live-cell imaging as well as fluorescence-activated cell sorting (FACS) experiments using standard laser wavelengths (405/488 nm). Expressed in mammalian cells and also in S. cerevisiae, the sensor protein faithfully reports on the status of methionine oxidation in an integrating manner. Variants targeted to membranes and the mitochondria provide subcellular resolution of methionine oxidation, e.g. reporting on site-specific oxidation by illumination of endogenous protoporphyrin IX.

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