| Literature DB >> 31852836 |
Dario Hermida1, Gulnahar B Mortuza1, Anna-Kathrine Pedersen2, Irina Pozdnyakova1, Tam T T N Nguyen3, Maria Maroto4, Michael Williamson1, Tasja Ebersole1, Giuseppe Cazzamali1, Kasper Rand3, Jesper V Olsen2, Marcos Malumbres4, Guillermo Montoya5.
Abstract
The human MASTL (Microtubule-associated serine/threonine kinase-like) gene encodes an essential protein in the cell cycle. MASTL is a key factor preventing early dephosphorylation of M-phase targets of Cdk1/CycB. Little is known about the mechanism of MASTL activation and regulation. MASTL contains a non-conserved insertion of 550 residues within its activation loop, splitting the kinase domain, and making it unique. Here, we show that this non-conserved middle region (NCMR) of the protein is crucial for target specificity and activity. We performed a phosphoproteomic assay with different MASTL constructs identifying key phosphorylation sites for its activation and determining whether they arise from autophosphorylation or exogenous kinases, thus generating an activation model. Hydrogen/deuterium exchange data complements this analysis revealing that the C-lobe in full-length MASTL forms a stable structure, whereas the N-lobe is dynamic and the NCMR and C-tail contain few localized regions with higher-order structure. Our results indicate that truncated versions of MASTL conserving a cryptic C-Lobe in the NCMR, display catalytic activity and different targets, thus establishing a possible link with truncated mutations observed in cancer-related databases.Entities:
Keywords: Kinases; cancer biology; cell cycle; mitosis; protein phosphatases
Mesh:
Substances:
Year: 2019 PMID: 31852836 PMCID: PMC7000116 DOI: 10.1074/mcp.RA119.001879
Source DB: PubMed Journal: Mol Cell Proteomics ISSN: 1535-9476 Impact factor: 5.911