Purification of human β- and γ-actin from budding yeast.

Journal of cell science2023PMID: 37070275

Plain Language Summary

Develops a yeast-based system for purifying human β- and γ-actin (non-muscle actin isoforms), which are difficult to obtain in native form. The purification protocol exploits actin's interactions with co-purified partners including thymosin β4, which is used to stabilize purified actin monomers and confirm functionality. Establishes a high-yield yeast expression system for non-muscle actin research and characterizes the isoform-specific binding preferences of Tβ4 (higher affinity for β/γ-actin than α-actin).

Abstract

Biochemical studies of human actin and its binding partners rely heavily on abundant and easily purified α-actin from skeletal muscle. Therefore, muscle actin has been used to evaluate and determine the activities of most actin regulatory proteins but there is an underlying concern that these proteins perform differently from actin present in non-muscle cells. To provide easily accessible and relatively abundant sources of human β- or γ-actin (i.e. cytoplasmic actins), we developed Saccharomyces cerevisiae strains that express each as their sole source of actin. Both β- or γ-actin purified in this system polymerize and interact with various binding partners, including profilin, mDia1 (formin), fascin and thymosin-β4 (Tβ4). Notably, Tβ4 and profilin bind to β- or γ-actin with higher affinity than to α-actin, emphasizing the value of testing actin ligands with specific actin isoforms. These reagents will make specific isoforms of actin more accessible for future studies on actin regulation.

Authors

Haarer, Brian K; Pimm, Morgan L; de Jong, Ebbing P; Amberg, David C; Henty-Ridilla, Jessica L

Keywords

Cytoplasmic actinNon-muscle actinβ-actinγ-actin