Structures and Short Linear Motif of Disordered Transcription Factor Regions Provide Clues to the Interactome of the Cellular Hub Protein Radical-induced Cell Death1

Charlotte O'Shea; Lasse Staby; Sidsel Krogh Bendsen; Frederik Grønbæk Tidemand; Andreas Redsted; Martin Willemoës; Birthe B Kragelund; Karen Skriver

doi:10.1074/jbc.M116.753426

Structures and Short Linear Motif of Disordered Transcription Factor Regions Provide Clues to the Interactome of the Cellular Hub Protein Radical-induced Cell Death1

J Biol Chem. 2017 Jan 13;292(2):512-527. doi: 10.1074/jbc.M116.753426. Epub 2016 Nov 23.

Authors

Charlotte O'Shea¹, Lasse Staby¹, Sidsel Krogh Bendsen¹, Frederik Grønbæk Tidemand¹, Andreas Redsted¹, Martin Willemoës¹, Birthe B Kragelund¹, Karen Skriver²

Affiliations

¹ From the Linderstrøm-Lang Centre for Protein Science, Department of Biology, University of Copenhagen, 5 Ole Maaloes Vej, Copenhagen DK-2200, Denmark.
² From the Linderstrøm-Lang Centre for Protein Science, Department of Biology, University of Copenhagen, 5 Ole Maaloes Vej, Copenhagen DK-2200, Denmark kskriver@bio.ku.dk.

Abstract

Intrinsically disordered protein regions (IDRs) lack a well defined three-dimensional structure but often facilitate key protein functions. Some interactions between IDRs and folded protein domains rely on short linear motifs (SLiMs). These motifs are challenging to identify, but once found they can point to larger networks of interactions, such as with proteins that serve as hubs for essential cellular functions. The stress-associated plant protein radical-induced cell death1 (RCD1) is one such hub, interacting with many transcription factors via their flexible IDRs. To identify the SLiM bound by RCD1, we analyzed the IDRs in three protein partners, DREB2A (dehydration-responsive element-binding protein 2A), ANAC013, and ANAC046, considering parameters such as disorder, context, charges, and pI. Using a combined bioinformatics and experimental approach, we have identified the bipartite RCD1-binding SLiM as (DE)X(1,2)(YF)X(1,4)(DE)L, with essential contributions from conserved aromatic, acidic, and leucine residues. Detailed thermodynamic analysis revealed both favorable and unfavorable contributions from the IDRs surrounding the SLiM to the interactions with RCD1, and the SLiM affinities ranged from low nanomolar to 50 times higher K_d values. Specifically, although the SLiM was surrounded by IDRs, individual intrinsic α-helix propensities varied as shown by CD spectroscopy. NMR spectroscopy further demonstrated that DREB2A underwent coupled folding and binding with α-helix formation upon interaction with RCD1, whereas peptides from ANAC013 and ANAC046 formed different structures or were fuzzy in the complexes. These findings allow us to present a model of the stress-associated RCD1-transcription factor interactome and to contribute to the emerging understanding of the interactions between folded hubs and their intrinsically disordered partners.

Keywords: Arabidopsis thaliana; SLiM; affinity; coupled folding and binding; interactome; intrinsically disordered protein; nuclear magnetic resonance (NMR); plant stress; protein-protein interaction; thermodynamics.

MeSH terms

Amino Acid Motifs
Arabidopsis / chemistry*
Arabidopsis / genetics
Arabidopsis / metabolism
Arabidopsis Proteins / chemistry*
Arabidopsis Proteins / genetics
Arabidopsis Proteins / metabolism
Models, Molecular*
Nuclear Magnetic Resonance, Biomolecular
Nuclear Proteins / chemistry*
Nuclear Proteins / genetics
Nuclear Proteins / metabolism
Protein Binding
Protein Folding*
Transcription Factors / chemistry*
Transcription Factors / genetics
Transcription Factors / metabolism

Substances

ANAC013 protein, Arabidopsis
Arabidopsis Proteins
DREB2A protein, Arabidopsis
Nuclear Proteins
RCD1 protein, Arabidopsis
Transcription Factors