A Designed Enzyme Promotes Selective Post-translational Acylation.
Pallavi M GosaviMegha JayachandranJoel J L RempilloOleksii ZozuliaOlga V MakhlynetsIvan V KorendovychPublished in: Chembiochem : a European journal of chemical biology (2018)
A computationally designed, allosterically regulated catalyst (CaM M144H) produced by substituting a single residue in calmodulin, a non-enzymatic protein, is capable of efficient and site selective post-translational acylation of lysines in peptides with highly diverse sequences. Calmodulin's binding partners are involved in regulating a large number of cellular processes; this new chemical-biology tool will help to identify them and provide structural insight into their interactions with calmodulin.