Literature DB >> 32976810

Comprehensive Analysis of G1 Cyclin Docking Motif Sequences that Control CDK Regulatory Potency In Vivo.

Sushobhana Bandyopadhyay1, Samyabrata Bhaduri1, Mihkel Örd2, Norman E Davey3, Mart Loog2, Peter M Pryciak4.   

Abstract

Many protein-modifying enzymes recognize their substrates via docking motifs, but the range of functionally permissible motif sequences is often poorly defined. During eukaryotic cell division, cyclin-specific docking motifs help cyclin-dependent kinases (CDKs) phosphorylate different substrates at different stages, thus enforcing a temporally ordered series of events. In budding yeast, CDK substrates with Leu/Pro-rich (LP) docking motifs are recognized by Cln1/2 cyclins in late G1 phase, yet the key sequence features of these motifs were unknown. Here, we comprehensively analyze LP motif requirements in vivo by combining a competitive growth assay with deep mutational scanning. We quantified the effect of all single-residue replacements in five different LP motifs by using six distinct G1 cyclins from diverse fungi including medical and agricultural pathogens. The results uncover substantial tolerance for deviations from the consensus sequence, plus requirements at some positions that are contingent on the favorability of other motif residues. They also reveal the basis for variations in functional potency among wild-type motifs, and allow derivation of a quantitative matrix that predicts the strength of other candidate motif sequences. Finally, we find that variation in docking motif potency can advance or delay the time at which CDK substrate phosphorylation occurs, and thereby control the temporal ordering of cell cycle regulation. The overall results provide a general method for surveying viable docking motif sequences and quantifying their potency in vivo, and they reveal how variations in docking strength can tune the degree and timing of regulatory modifications.
Copyright © 2020 Elsevier Inc. All rights reserved.

Entities:  

Keywords:  CDK; Cln2; SLiM; Sic1; Ste5; Whi5; cell cycle; cyclin; docking; phosphorylation

Year:  2020        PMID: 32976810      PMCID: PMC8009629          DOI: 10.1016/j.cub.2020.08.099

Source DB:  PubMed          Journal:  Curr Biol        ISSN: 0960-9822            Impact factor:   10.834


  56 in total

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2.  Targeting, disruption, replacement, and allele rescue: integrative DNA transformation in yeast.

Authors:  R Rothstein
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4.  Cyclin-specific docking motifs promote phosphorylation of yeast signaling proteins by G1/S Cdk complexes.

Authors:  Samyabrata Bhaduri; Peter M Pryciak
Journal:  Curr Biol       Date:  2011-09-22       Impact factor: 10.834

5.  A Conserved Motif Provides Binding Specificity to the PP2A-B56 Phosphatase.

Authors:  Emil Peter Thrane Hertz; Thomas Kruse; Norman E Davey; Blanca López-Méndez; Jón Otti Sigurðsson; Guillermo Montoya; Jesper V Olsen; Jakob Nilsson
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6.  Global analysis of Cdk1 substrate phosphorylation sites provides insights into evolution.

Authors:  Liam J Holt; Brian B Tuch; Judit Villén; Alexander D Johnson; Steven P Gygi; David O Morgan
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8.  Cks confers specificity to phosphorylation-dependent CDK signaling pathways.

Authors:  Denise A McGrath; Eva Rose M Balog; Mardo Kõivomägi; Rafael Lucena; Michelle V Mai; Alexander Hirschi; Douglas R Kellogg; Mart Loog; Seth M Rubin
Journal:  Nat Struct Mol Biol       Date:  2013-11-03       Impact factor: 15.369

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Authors:  V Paolillo; C B Jenkinson; T Horio; B R Oakley
Journal:  Stud Mycol       Date:  2018-06-20       Impact factor: 16.097

10.  How the cell cycle clock ticks.

Authors:  Mihkel Örd; Mart Loog
Journal:  Mol Biol Cell       Date:  2019-01-15       Impact factor: 4.138

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4.  Bipartite binding of the N terminus of Skp2 to cyclin A.

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Journal:  Structure       Date:  2021-05-13       Impact factor: 5.871

5.  The Eukaryotic Linear Motif resource: 2022 release.

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6.  G1-Cyclin2 (Cln2) promotes chromosome hypercondensation in eco1/ctf7 rad61 null cells during hyperthermic stress in Saccharomyces cerevisiae.

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  7 in total

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