| Literature DB >> 33357379 |
Antonella Chiapparino1, Antonija Grbavac2, Hendrik Ra Jonker3, Yvonne Hackmann1, Sofia Mortensen1, Ewa Zatorska2, Andrea Schott2, Gunter Stier1, Krishna Saxena3, Klemens Wild1, Harald Schwalbe3, Sabine Strahl2, Irmgard Sinning1.
Abstract
Protein O-mannosyltransferases (PMTs) represent a conserved family of multispanning endoplasmic reticulum membrane proteins involved in glycosylation of S/T-rich protein substrates and unfolded proteins. PMTs work as dimers and contain a luminal MIR domain with a β-trefoil fold, which is susceptive for missense mutations causing α-dystroglycanopathies in humans. Here, we analyze PMT-MIR domains by an integrated structural biology approach using X-ray crystallography and NMR spectroscopy and evaluate their role in PMT function in vivo. We determine Pmt2- and Pmt3-MIR domain structures and identify two conserved mannose-binding sites, which are consistent with general β-trefoil carbohydrate-binding sites (α, β), and also a unique PMT2-subfamily exposed FKR motif. We show that conserved residues in site α influence enzyme processivity of the Pmt1-Pmt2 heterodimer in vivo. Integration of the data into the context of a Pmt1-Pmt2 structure and comparison with homologous β-trefoil - carbohydrate complexes allows for a functional description of MIR domains in protein O-mannosylation.Entities:
Keywords: NMR; S. cerevisiae; carbohydrate-binding module; enzymatic processivity; glycosyltransferase; molecular biophysics; protein O-mannosylation; structural biology; x-ray crystallography
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Year: 2020 PMID: 33357379 PMCID: PMC7759382 DOI: 10.7554/eLife.61189
Source DB: PubMed Journal: Elife ISSN: 2050-084X Impact factor: 8.140