1. Coupling to short linear motifs creates versatile PME-1 activities in PP2A holoenzyme demethylation and inhibition
- Author
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Li, Yitong, Balakrishnan, Vijaya Kumar, Rowse, Michael, Wu, Cheng-Guo, Bravos, Anastasia Phoebe, Yadav, Vikash K., Ivarsson, Ylva, Strack, Stefan, Novikova, Irina, V, Xing, Yongna, Li, Yitong, Balakrishnan, Vijaya Kumar, Rowse, Michael, Wu, Cheng-Guo, Bravos, Anastasia Phoebe, Yadav, Vikash K., Ivarsson, Ylva, Strack, Stefan, Novikova, Irina, V, and Xing, Yongna
- Abstract
Protein phosphatase 2A (PP2A) holoenzymes target broad substrates by recognizing short motifs via regulatory subunits. PP2A methylesterase 1 (PME-1) is a cancer-promoting enzyme and undergoes methylesterase activation upon binding to the PP2A core enzyme. Here, we showed that PME-1 readily demethylates different families of PP2A holoenzymes and blocks substrate recognition in vitro. The high-resolution cryoelectron microscopy structure of a PP2A-B56 holoenzyme-PME-1 complex reveals that PME-1 disordered regions, including a substrate-mimicking motif, tether to the B56 regulatory subunit at remote sites. They occupy the holoenzyme substratebinding groove and allow large structural shifts in both holoenzyme and PME-1 to enable multipartite contacts at structured cores to activate the methylesterase. B56 interface mutations selectively block PME-1 activity toward PP2A-B56 holoenzymes and affect the methylation of a fraction of total cellular PP2A. The B56 interface mutations allow us to uncover B56-specific PME-1 functions in p53 signaling. Our studies reveal multiple mechanisms of PME-1 in suppressing holoenzyme functions and versatile PME-1 activities derived from coupling substrate-mimicking motifs to dynamic structured cores.
- Published
- 2022
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