LanthaScreen Conjugating Assay Reagents

LanthaScreen conjugation assay reagents provide sensitive high-throughput screening (HTS) reagents to either monitor the rate of conjugation of ubiquitin or ubiquitin-like (UBL) molecules to target proteins, or the extent of this conjugation.  By incorporating the TR-FRET donor (terbium) or acceptor (fluorescein) onto ubiquitin and SUMO proteins, these universal assay reagents can be used to rapidly develop screening assays for conjugating enzymes.  To maintain biochemical reactivity, the ubiquitin and UBL conjugates are selectively modified near the N-terminus via an introduced cysteine residue with thiol reactive dyes.  This type of chemical modification leaves all of the internal lysine residues free for conjugation to another ubiquitin or UBL molecule to form poly-ubiquitin (or UBL) chains.

For a typical HTS TR-FRET ubiquitination assay, fluorescein- and/or Terbium-labeled ubiquitin is incubated with the ubiquitin-conjugating enzymes (E1, E2 and E3), a target protein to be ubiquitinated, and an ATP solution to initiate the reaction.  The enzymes conjugate the labeled ubiquitins to the target protein, resulting in mono- or poly- ubiquitination.  Depending on the specific assay, a detection reagent (a Tb-anti-epitope-tagged antibody) may be added to the reaction to complete the TR-FRET pairing (Figures 1 and 2).  Similar assays reagents have also been developed for the Ubiquitin-like proteins SUMO1, SUMO2, and SUMO3.