AI Article Synopsis

  • Researchers developed [2.2.1]azabicyclic vinyl sulfone reagents that selectively modify cysteine in proteins and have potential for further chemical reactions.
  • *These reagents quickly and efficiently label cysteine-tagged proteins without affecting their function, even in a biological context like human plasma.
  • *The technology allows for precise protein labeling and can be used in live cells for applications such as apoptosis imaging, showcasing its potential for biochemical studies.*

Article Abstract

We have developed [2.2.1]azabicyclic vinyl sulfone reagents that simultaneously enable cysteine-selective protein modification and introduce a handle for further bioorthogonal ligation. The reaction is fast and selective for cysteine relative to other amino acids that have nucleophilic side-chains, and the formed products are stable in human plasma and are moderately resistant to retro Diels-Alder degradation reactions. A model biotinylated [2.2.1]azabicyclic vinyl sulfone reagent was shown to efficiently label two cysteine-tagged proteins, ubiquitin and C2Am, under mild conditions (1-5 equiv. of reagent in NaP pH 7.0, room temperature, 30 min). The resulting thioether-linked conjugates were stable and retained the native activity of the proteins. Finally, the dienophile present in the azabicyclic moiety on a functionalised C2Am protein could be fluorescently labelled through an inverse electron demand Diels-Alder reaction in cells to allow selective apoptosis imaging. The combined advantages of directness, site-specificity and easy preparation mean [2.2.1]azabicyclic vinyl sulfones can be used for residue-specific dual protein labelling/construction strategies with minimal perturbation of native function based simply on the attachment of an [2.2.1]azabicyclic moiety to cysteine.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC6482879PMC
http://dx.doi.org/10.1039/c9sc00125eDOI Listing

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