{"id":11678,"date":"2026-01-08T15:44:55","date_gmt":"2026-01-08T15:44:55","guid":{"rendered":"https:\/\/www.sygnaturediscovery.com\/?post_type=case-study&p=11678"},"modified":"2026-02-02T17:40:32","modified_gmt":"2026-02-02T17:40:32","slug":"separating-phosphorylation-states-of-a-kinase-using-ion-exchange-chromatography","status":"publish","type":"case-study","link":"https:\/\/www.sygnaturediscovery.com\/fr\/case-study\/separating-phosphorylation-states-of-a-kinase-using-ion-exchange-chromatography\/","title":{"rendered":"Separating Phosphorylation States of a Kinase Using Ion Exchange Chromatography"},"content":{"rendered":"\n

In this case study we present our ability to express, phosphorylate and separate the native (dephosphorylated form) and the active (dual phosphorylated form) of a kinase to produce batches at high yield with excellent purity.<\/h2>\n\n\n\n

Many serine\/threonine kinases are involved in\u00a0 the regulation of essential cellular processes such as proliferation, differentiation, and survival. Often activation of the kinase occurs through dual phosphorylation at threonine residues by an upstream kinase, inducing a conformational change that enables full enzymatic activity. The diphosphorylated form therefore represents the active state of the kinase.<\/p>\n\n\n\n

Within the Protein and Structure department at Sygnature Discovery we have significant experience expressing and purifying multiple forms of various kinases to best suit the particular downstream application. Recently we have had an internal project to optimise our workflow to produce both the inactive unphosphorylated and active diphosphorylated form of a particular kinase. This was with and without various tags and also with and without a biotinylated AVI tag to support SPR studies and other assay formats with the kinase.<\/p>\n\n\n\n

Summary of the various forms that have been successfully produced in our laboratories.<\/p>\n\n\n\n