4.8 Article

Interaction Dynamics Determine Signaling and Output Pathway Responses

Journal

CELL REPORTS
Volume 19, Issue 1, Pages 136-149

Publisher

CELL PRESS
DOI: 10.1016/j.celrep.2017.03.029

Keywords

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Categories

Funding

  1. CRG Biomolecular Screening and Protein Technologies Unit
  2. CRG Genomics Unit
  3. CRG Bioinformatics Unit
  4. European Commission 7th Framework Programme (UNICELLSYS) [201142]
  5. Spanish Ministry of Economy and Competitiveness [BFU2012-33503, BFU2014-52125-REDT, BFU14-51672-REDC, BFU201564437-P, BFU2014-52333-P]
  6. Catalan Government [2014 SGR 599]
  7. EU 7th Framework Programme (SYNCOM) [294294]
  8. Fundacion Botin, Banco Santander
  9. German Research Council [RTG 1772]
  10. Spanish Ministerio de Economia y Competitividad, Plan Nacional
  11. European Fund for Regional Development [BIO2012-39754]
  12. Spanish Ministry of Economy and Competitiveness, Centro de Excelencia Severo Ochoa'' [SEV-2012-0208]
  13. CERCA Programme/Generalitat de Catalunya
  14. Spanish Ministry of Economy and Competitiveness(FEDER) [BFU2012-33503, BFU2014-52125-REDT, BFU14-51672-REDC, BFU201564437-P, BFU2014-52333-P]
  15. ICREA Funding Source: Custom

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The understanding of interaction dynamics in signaling pathways can shed light on pathway architecture and provide insights into targets for intervention. Here, we explored the relevance of kinetic rate constants of a key upstream osmosensor in the yeast high-osmolarity glycerol-mitogen-activated protein kinase (HOG-MAPK) pathway to signaling output responses. We created mutant pairs of the Sln1-Ypd1 complex interface that caused major compensating changes in the association (k(on)) and dissociation (k(off)) rate constants (kinetic perturbations) but only moderate changes in the overall complex affinity (K-d). Yeast cells carrying a Sln1-Ypd1 mutant pair with moderate increases in k(on) and koff displayed a lower threshold of HOG pathway activation than wild-type cells. Mutants with higher k(on) and k(off) rates gave rise to higher basal signaling and gene expression but impaired osmoadaptation. Thus, the k(on) and k(off) rates of the components in the Sln1 osmosensor determine proper signaling dynamics and osmoadaptation.

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