Toward universal protein post-translational modification detection in high throughput format



Harri Härmä, Natalia Tong-Ochoa, Arjan J. van Adrichem, Ilian Jelesarov, Krister Wennerberg, Kari Kopra

PublisherROYAL SOC CHEMISTRY

2018

Chemical Communications

CHEMICAL COMMUNICATIONS

CHEM COMMUN

54

23

2910

2913

4

1359-7345

1364-548X

DOIhttps://doi.org/10.1039/c7cc09575a

http://pubs.rsc.org/en/Content/ArticleLanding/2018/CC/C7CC09575A#!divAbstract

https://research.utu.fi/converis/portal/detail/Publication/30836301


Post-translational modification (PTM) of proteins plays essential regulatory roles in a variety of pathological conditions. Reliable and practical assays are required to accelerate the discovery of inhibitors and activators for PTM related diseases. Today, methodologies are based on specific or group-specific PTM recognition of e.g. phosphate for kinase activity without extending to other type of PTMs. Here we have established a universal time-resolved luminescence assay on a peptide-break platform for the direct detection of wide variety of PTMs. The developed assay is based on the leucine zipper concept wherein a europium-chelate labeled detection peptide and a non-labeled peptide substrate form a highly luminescent dimer. As an active PTM enzyme at sub or low nanomolar concentration modifies the substrate peptide, the luminescent signal of the detached detection peptide is quenched in the presence of soluble quenchers. The functionality of this universal assay technique has been demonstrated for the monitoring of phosphorylation, dephosphorylation, deacetylation, and citrullination with high applicability also to other PTMs in a high throughput format.

Last updated on 2024-26-11 at 17:17