DOCSLIB.ORG

The Human Na+/H+ Exchanger 1 Is a Membrane Scaffold Protein for Extracellular Signal-Regulated Kinase 2

Total Page:16

File Type:pdf, Size:1020Kb

Download full-text PDF Read full-text
The Human Na+/H+ Exchanger 1 Is a Membrane Scaffold Protein for Extracellular Signal-Regulated Kinase 2 The human Na+/H+ exchanger 1 is a membrane scaffold protein for extracellular signal-regulated kinase 2 Hendus-Altenburger, Ruth; Pedraz Cuesta, Elena; Olesen, Christina Wilkens; Papaleo, Elena; Schnell, Jeff Alexander; Hopper, Jonathan T. S.; Robinson, Carol V.; Pedersen, Stine Helene Falsig; Kragelund, Birthe Brandt Published in: BMC Biology DOI: 10.1186/s12915-016-0252-7 Publication date: 2016 Document version Publisher's PDF, also known as Version of record Document license: CC BY Citation for published version (APA): Hendus-Altenburger, R., Pedraz Cuesta, E., Olesen, C. W., Papaleo, E., Schnell,+ J.+ A., Hopper, J. T. S., Robinson, C. V., Pedersen, S. H. F., & Kragelund, B. B. (2016). The human Na /H exchanger 1 is a membrane scaffold protein for extracellular signal-regulated kinase 2. BMC Biology, 14, [31]. https://doi.org/10.1186/s12915-016-0252-7 Download date: 23. sep.. 2021 Hendus-Altenburger et al. BMC Biology (2016) 14:31 DOI 10.1186/s12915-016-0252-7 RESEARCH ARTICLE Open Access The human Na+/H+ exchanger 1 is a membrane scaffold protein for extracellular signal-regulated kinase 2 Ruth Hendus-Altenburger1,2, Elena Pedraz-Cuesta1, Christina W. Olesen1, Elena Papaleo2, Jeff A. Schnell2, Jonathan T. S. Hopper3, Carol V. Robinson3, Stine F. Pedersen1* and Birthe B. Kragelund2* Abstract Background: Extracellular signal-regulated kinase 2 (ERK2) is an S/T kinase with more than 200 known substrates, and with critical roles in regulation of cell growth and differentiation and currently no membrane proteins have been linked to ERK2 scaffolding. Methods and results: Here, we identify the human Na+/H+ exchanger 1 (hNHE1) as a membrane scaffold protein for ERK2 and show direct hNHE1-ERK1/2 interaction in cellular contexts. Using nuclear magnetic resonance (NMR) spectroscopy and immunofluorescence analysis we demonstrate that ERK2 scaffolding by hNHE1 occurs by one of three D-domains and by two non-canonical F-sites located in the disordered intracellular tail of hNHE1, mutation of which reduced cellular hNHE1-ERK1/2 co-localization, as well as reduced cellular ERK1/2 activation. Time-resolved NMR spectroscopy revealed that ERK2 phosphorylated the disordered tail of hNHE1 at six sites in vitro, in a distinct temporal order, with the phosphorylation rates at the individual sites being modulated by the docking sites in a distant dependent manner. Conclusions: This work characterizes a new type of scaffolding complex, which we term a “shuffle complex”, between the disordered hNHE1-tail and ERK2, and provides a molecular mechanism for the important ERK2 scaffolding function of the membrane protein hNHE1, which regulates the phosphorylation of both hNHE1 and ERK2. Keywords: NHE1, Intrinsically disordered protein, Phosphorylation, MAPK, Shuffle complex, NMR, Scaffold Background identification as such suggested from qualities of multi- Extracellular signal-regulated kinase 2 (ERK2) is a mem- valent binding, non-catalytic placeholders, and bidirec- ber of the mitogen-activated protein kinase (MAPK) tional process control [2]. Several scaffold proteins have family of kinases activated in response to numerous been described for the MAPKs such as kinase suppres- growth factors and cytokines, leading to phosphorylation sor of Ras (KSR) [3], JNK-interacting protein (JIP) [4], and functional regulation of downstream targets. ERK2 IQ motif containing GTPase activating protein 1 has been linked to more than 200 different substrates (IQGAP1) [5], and β-arrestin [6], which interact with whose phosphorylation by ERK2 is orchestrated by members of the MAPK cascade, providing multivalency, coordination of signaling networks through common spatial concentration, and/or signaling fidelity. However, binding to so-called scaffold proteins [1]. The definition although MAPKs are known to regulate the action of of a scaffold protein was recently refined and their several membrane proteins and receptors, none of these scaffold proteins are themselves membrane proteins, requiring additional mechanisms for colocalization of * Correspondence: [email protected]; [email protected] the scaffold protein, the membrane protein, as well as 1Cell and Developmental Biology, Department of Biology, University of the kinases. Moreover, most of the available molecular Copenhagen, Universitetsparken 13, DK-2100 Copenhagen Ø, Denmark insights are from structures of kinases in complex with 2Structural Biology and NMR Laboratory, Department of Biology, University of Copenhagen, Ole Maaløes Vej 5, DK-2200 Copenhagen N, Denmark folded domains or with small peptides of the scaffold Full list of author information is available at the end of the article © 2016 Hendus-Altenburger et al. Open Access This article is distributed under the terms of the Creative Commons Attribution 4.0 International License (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated. Hendus-Altenburger et al. BMC Biology (2016) 14:31 Page 2 of 17 proteins, and details regarding scaffolding by non-globular predictions, as well as by nuclear magnetic resonance proteins are lacking. (NMR) spectroscopy and other biophysical techniques, MAPKs are S/T kinases that interact with targets and that the distal ~ 130 residues of the hNHE1 C-terminal regulators via two types of domains, D-domains and intracellular domain (hNHE1cdt), containing most of F-sites [7–11]. D-domains, also known as docking the known NHE1 phosphorylation sites, are intrinsically sites for ERK and JNK, LXL (DEJL) domains, or kinase disordered (ID) [35, 36]. To our knowledge, no studies interaction motifs (KIMs) have the canonical sequence of have yet addressed the mechanisms through which 2–5 basic residues (R/K), spaced by 1–6residuestoa MAPKs interact with ID proteins (IDPs), although about hydrophobic motif ΦXΦ,whereΦ is generally V, L, one third of all proteins in higher eukaryotes contain or I [8, 9]. D-domains are found in MAPK substrates significant ID regions (IDRs) [37], and ID is abundant in such as the transcription factor Elk-1 and p90 riboso- cellular signalling [38], scaffolding [39], as well as in mal S kinase (RSK1-3), as well as in other MAPK tar- MAPKs themselves [40]. gets[8,9,11].InERK2,D-domainsinteractwiththe Here, we demonstrate that hNHE1 acts as an ERK2 D-domain recognition site also known as the CD/ED membrane protein scaffold in vivo that is necessary for (common docking domain/glutamate/aspartate dock- ERK2 activation via direct interactions, and we show ing) domain, located more than 10 Å from the active that loss of scaffolding by hNHE1 leads to decreased site [8, 9, 11]. The F-site recruitment site in ERK2 is ERK2 activation. Using NMR spectroscopy we show that much less studied and incompletely understood. It NHE1 scaffolds inactive (ia) ERK2 in a “shuffle complex” binds to F-sites, also called DEF (docking site for that involves a D-domain and two non-canonical F-sites. ERK, FXFP)-domains with the canonical FXFP se- We characterize the order and kinetics of both previ- quence [12]. F-sites allow for aromatic residues at the ously reported and novel ERK2-mediated phosphoryla- P1 (F, W) and P3 positions (F, Y, W) [13], and F-sites tions of hNHE1 in vitro. Our findings provide a have been reported in substrates such as Elk-1 (FQFP) molecular mechanism for the widely recognized and [14] and c-Fos (FTYP) [15], and within the nucleoporin functionally important scaffolding function of hNHE1, FG-repeats (FXFG) [16, 17]. So far the only structure and give mechanistic insight into the regulation of ERK2 available of an F-site recruitment site-interacting protein activity by the intrinsically disordered hNHE1cdt. is that of ERK2 in complex with the 15 kDa phosphopro- tein enriched in astrocytes (PEA-15), which notably lacks Results any of the above-mentioned motifs [18]. The recently suggested links between hNHE1 and The plasma membrane Na+/H+ exchanger 1 (NHE1, ERK1/2 prompted us to investigate whether ERK1/2 and SLC9A1) is a major regulator of pH and volume in es- NHE1 directly interact in a cellular context. Using AP-1 sentially all cells studied. Furthermore, NHE1 is involved cells (which lack endogenous NHE1 [41]) stably express- in the regulation of cell proliferation, survival, motility, ing full-length WT hNHE1, we asked if hNHE1 and and other essential physiological processes, and its dys- ERK1/2 engage in a direct interaction in vivo. Inter- regulation contributes importantly to major human ma- action was assessed using in situ proximity ligation assay lignancies, including cancer and cardiovascular diseases (PLA), which interrogates close interaction (<40 nm) be- [19, 20]. Numerous hormones and growth factors acting tween proteins (Fig. 1). As seen, the detection of mul- via receptor tyrosine kinases or GTP-binding protein- tiple PLA puncta when cells were incubated with both coupled receptors can elicit posttranslational regulation NHE1 and ERK1/2 antibodies revealed the presence of of NHE1 [21–23]. The MAPKs ERK1/2, p38 MAPK, and hNHE1-ERK1/2 complexes in AP-1 WT hNHE1 cells c-Jun N-terminal kinase (JNK) are widely implicated in (Fig. 1a), compared to a much lower signal in negative NHE1 regulation [24–28], and direct phosphorylation of controls incubated with one antibody only (Fig. 1b). Data human (h) NHE1 by ERK1/2 was previously proposed from multiple experiments are quantified in Fig. 1c, based on 32P measurements [25] and mass spectrometry demonstrating that the PLA signal is significantly greater [29]. Conversely, NHE1 has been reported to regulate in NHE1-ERK antibody-labelled cells than in negative signaling through regulation of ERK1/2 and p38 MAPK controls. Thus, these data show that hNHE1 and ERK1/ activity [26, 28, 30–32], and yeast two-hybrid screens 2 directly interact in the cell.
Load more

Recommended publications
  • Behaviour of Intrinsically Disordered Proteins in Protein–Protein Complexes with an Emphasis on Fuzziness
    Cell. Mol. Life Sci. (2017) 74:3175–3183 DOI 10.1007/s00018-017-2560-7 Cellular and Molecular Life Sciences MULTI-AUTHOR REVIEW Behaviour of intrinsically disordered proteins in protein–protein complexes with an emphasis on fuzziness 1 1 1 Johan G. Olsen • Kaare Teilum • Birthe B. Kragelund Received: 18 May 2017 / Accepted: 1 June 2017 / Published online: 8 June 2017 Ó The Author(s) 2017. This article is an open access publication Abstract Intrinsically disordered proteins (IDPs) do not, Introduction by themselves, fold into a compact globular structure. They are extremely dynamic and flexible, and are typically Signalling and regulation are essential to all living cells involved in signalling and transduction of information and are based on intermolecular interactions, most of which through binding to other macromolecules. The reason for are mediated by proteins. A substantial fraction of proteins their existence may lie in their malleability, which enables include large regions of disorder without clearly defined them to bind several different partners with high speci- three-dimensional structure. Such intrinsically disordered ficity. In addition, their interactions with other proteins (IDPs) are not only very abundant—30–40% of all macromolecules can be regulated by a variable amount of proteins in the human proteome are disordered or contain chemically diverse post-translational modifications. Four intrinsically disordered regions (IDRs) [1, 2]—they also kinetically and energetically different types of complexes constitute significant parts of membrane proteins [3, 4] and between an IDP and another macromolecule are reviewed: occupy pivotal positions in cellular regulation on all levels (1) simple two-state binding involving a single binding site, [5].
    [Show full text]
  • Intrinsically Disordered Chromatin Protein NUPR1 Binds to the C-Terminal Region of Polycomb RING1B
    Intrinsically disordered chromatin protein NUPR1 binds to the C-terminal region of Polycomb RING1B Patricia Santofimia-Castañoa,1, Bruno Rizzutib, Ángel L. Peyc, Philippe Soubeyrana, Miguel Vidald, Raúl Urrutiae, Juan L. Iovannaa, and José L. Neiraf,g,1,2 aCentre de Recherche en Cancérologie de Marseille, INSERM U1068, CNRS UMR 7258, Aix-Marseille Université and Institut Paoli-Calmettes, Parc Scientifique et Technologique de Luminy, 13288 Marseille, France; bLiquid Crystal Laboratory, Consiglio Nazionale delle Ricerche–NANOTEC, Università della Calabria, 87036 Rende, Italy; cDepartment of Physical Chemistry, University of Granada, 18071 Granada, Spain; dDepartment of Cellular and Molecular Biology, Centro de Investigaciones Biológicas, Consejo Superior de Investigaciones Científicas, 28040 Madrid, Spain; eLaboratory of Epigenetics and Chromatin Dynamics, Division of Gastroenterology and Hepatology, Department of Internal Medicine, Epigenomics Translational Program, Center for Individualized Medicine, Mayo Clinic, Rochester, MN 55905; fInstituto de Biología Molecular y Celular, Universidad Miguel Hernández, 03202 Elche, Alicante, Spain; and gBiophysics Unit, Biocomputation and Complex Systems Physics Institute, 50009 Zaragoza, Spain Edited by Alan R. Fersht, Medical Research Council Laboratory of Molecular Biology, Cambridge, United Kingdom, and approved June 21, 2017 (received for review December 4, 2016) Intrinsically disordered proteins (IDPs) are ubiquitous in eukaryotes, and heterodimeric RING finger E3 ligase, whose subunit binding the they are often associated with diseases in humans. The protein E2 ligase is RING1B, or its paralog RING1A. The other member NUPR1 is a multifunctional IDP involved in chromatin remodeling and of the heterodimer is one out of a group of six Polycomb Ring in the development and progression of pancreatic cancer; however, the finger proteins (whose best-known member is perhaps BMI1), details of such functions are unknown.
    [Show full text]
  • Src Family Tyrosine Kinases in Intestinal Homeostasis, Regeneration and Tumorigenesis Audrey Sirvent, Rudy Mevizou, Dana Naim, Marie Lafitte, Serge Roche
    Src Family Tyrosine Kinases in Intestinal Homeostasis, Regeneration and Tumorigenesis Audrey Sirvent, Rudy Mevizou, Dana Naim, Marie Lafitte, Serge Roche To cite this version: Audrey Sirvent, Rudy Mevizou, Dana Naim, Marie Lafitte, Serge Roche. Src Family Tyrosine Kinases in Intestinal Homeostasis, Regeneration and Tumorigenesis. Cancers, MDPI, 2020, 12 (8), pp.2014. 10.3390/cancers12082014. hal-02989641 HAL Id: hal-02989641 https://hal.archives-ouvertes.fr/hal-02989641 Submitted on 17 Nov 2020 HAL is a multi-disciplinary open access L’archive ouverte pluridisciplinaire HAL, est archive for the deposit and dissemination of sci- destinée au dépôt et à la diffusion de documents entific research documents, whether they are pub- scientifiques de niveau recherche, publiés ou non, lished or not. The documents may come from émanant des établissements d’enseignement et de teaching and research institutions in France or recherche français ou étrangers, des laboratoires abroad, or from public or private research centers. publics ou privés. cancers Review Src Family Tyrosine Kinases in Intestinal Homeostasis, Regeneration and Tumorigenesis Audrey Sirvent , Rudy Mevizou , Dana Naim , Marie Lafitte and Serge Roche * CRBM, CNRS, University of Montpellier, Equipe labellisée Ligue Contre le Cancer, F-34000 Montpellier, France; [email protected] (A.S.); [email protected] (R.M.); [email protected] (D.N.); marie.lafi[email protected] (M.L.) * Correspondence: [email protected] Received: 17 June 2020; Accepted: 19 July 2020; Published: 23 July 2020 Abstract: Src, originally identified as an oncogene, is a membrane-anchored tyrosine kinase and the Src family kinase (SFK) prototype. SFKs regulate the signalling induced by a wide range of cell surface receptors leading to epithelial cell growth and adhesion.
    [Show full text]
  • The Human Na+/H+ Exchanger 1 Is a Membrane Scaffold Protein for Extracellular Signal-Regulated Kinase 2 Ruth Hendus-Altenburger1,2, Elena Pedraz-Cuesta1, Christina W
    Hendus-Altenburger et al. BMC Biology (2016) 14:31 DOI 10.1186/s12915-016-0252-7 RESEARCH ARTICLE Open Access The human Na+/H+ exchanger 1 is a membrane scaffold protein for extracellular signal-regulated kinase 2 Ruth Hendus-Altenburger1,2, Elena Pedraz-Cuesta1, Christina W. Olesen1, Elena Papaleo2, Jeff A. Schnell2, Jonathan T. S. Hopper3, Carol V. Robinson3, Stine F. Pedersen1* and Birthe B. Kragelund2* Abstract Background: Extracellular signal-regulated kinase 2 (ERK2) is an S/T kinase with more than 200 known substrates, and with critical roles in regulation of cell growth and differentiation and currently no membrane proteins have been linked to ERK2 scaffolding. Methods and results: Here, we identify the human Na+/H+ exchanger 1 (hNHE1) as a membrane scaffold protein for ERK2 and show direct hNHE1-ERK1/2 interaction in cellular contexts. Using nuclear magnetic resonance (NMR) spectroscopy and immunofluorescence analysis we demonstrate that ERK2 scaffolding by hNHE1 occurs by one of three D-domains and by two non-canonical F-sites located in the disordered intracellular tail of hNHE1, mutation of which reduced cellular hNHE1-ERK1/2 co-localization, as well as reduced cellular ERK1/2 activation. Time-resolved NMR spectroscopy revealed that ERK2 phosphorylated the disordered tail of hNHE1 at six sites in vitro, in a distinct temporal order, with the phosphorylation rates at the individual sites being modulated by the docking sites in a distant dependent manner. Conclusions: This work characterizes a new type of scaffolding complex, which we term a “shuffle complex”, between the disordered hNHE1-tail and ERK2, and provides a molecular mechanism for the important ERK2 scaffolding function of the membrane protein hNHE1, which regulates the phosphorylation of both hNHE1 and ERK2.
    [Show full text]
  • Simple Biochemical Features Underlie Transcriptional Activation Domain Diversity and Dynamic, Fuzzy Binding to Mediator
    bioRxiv preprint doi: https://doi.org/10.1101/2020.12.18.423551; this version posted December 18, 2020. The copyright holder for this preprint (which was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission. Simple biochemical features underlie transcriptional activation domain diversity and dynamic, fuzzy binding to Mediator Adrian L. Sanborn,1,2,* Benjamin T. Yeh,2 Jordan T. Feigerle,1 Cynthia V. Hao,1 Raphael J. L. Townshend,2 Erez Lieberman Aiden,3,4 Ron O. Dror,2 Roger D. Kornberg1,*,+ 1Department of Structural Biology, Stanford University School of Medicine, Stanford, CA 94305, USA 2Department of Computer Science, Stanford University, Stanford, CA 94305, USA 3The Center for Genome Architecture, Baylor College of Medicine, Houston, USA 4Center for Theoretical Biological Physics, Rice University, Houston, USA *Correspondence: [email protected], [email protected] +Lead Contact SUMMARY and Tjian, 1989). Instead, ADs were classified based on their enrichment of certain residues, whether acidic, glutamine- Gene activator proteins comprise distinct DNA-binding and rich, or proline-rich. transcriptional activation domains (ADs). Because few ADs Acidic ADs are the most common and best characterized. have been described, we tested domains tiling all yeast Acidic ADs retain activity when transferred between yeast transcription factors for activation in vivo and identified 150 and animals, pointing to a conserved eukaryotic mechanism ADs. By mRNA display, we showed that 73% of ADs bound the (Fischer et al., 1988; Struhl, 1988). While some have found Med15 subunit of Mediator, and that binding strength was that acidic residues are necessary for activation, others have correlated with activation.
    [Show full text]
  • Intrinsically Disordered Proteins and Intrinsically Disordered Protein Regions
    BI83CH22-Dunker ARI 3 May 2014 11:29 Intrinsically Disordered Proteins and Intrinsically Disordered Protein Regions Christopher J. Oldfield and A. Keith Dunker Center for Computational Biology and Bioinformatics, Indiana University School of Medicine, Indianapolis, Indiana 46202; email: cjoldfi[email protected], [email protected] Annu. Rev. Biochem. 2014. 83:553–84 Keywords First published online as a Review in Advance on rheomorphic, natively, inherently, unstructured, unfolded, flexible, March 5, 2014 malleable, chameleon The Annual Review of Biochemistry is online at biochem.annualreviews.org Abstract This article’s doi: Intrinsically disordered proteins (IDPs) and IDP regions fail to form 10.1146/annurev-biochem-072711-164947 a stable structure, yet they exhibit biological activities. Their mobile by ALI: Academic Libraries of Indiana on 10/29/14. For personal use only. Copyright c 2014 by Annual Reviews. flexibility and structural instability are encoded by their amino acid Annu. Rev. Biochem. 2014.83:553-584. Downloaded from www.annualreviews.org All rights reserved sequences. They recognize proteins, nucleic acids, and other types of partners; they accelerate interactions and chemical reactions between bound partners; and they help accommodate posttranslational modifi- cations, alternative splicing, protein fusions, and insertions or deletions. Overall, IDP-associated biological activities complement those of struc- tured proteins. Recently, there has been an explosion of studies on IDP regions and their functions, yet the discovery and investigation of these proteins have a long, mostly ignored history. Along with recent discov- eries, we present several early examples and the mechanisms by which IDPs contribute to function, which we hope will encourage compre- hensive discussion of IDPs and IDP regions in biochemistry textbooks.
    [Show full text]
  • Database of Fuzzy Complexes, a Tool to Develop Stochastic Structure
    D228–D235 Nucleic Acids Research, 2017, Vol. 45, Database issue Published online 28 October 2016 doi: 10.1093/nar/gkw1019 FuzDB: database of fuzzy complexes, a tool to develop stochastic structure-function relationships for protein complexes and higher-order assemblies Marton Miskei, Csaba Antal and Monika Fuxreiter* MTA-DE Momentum, Laboratory of Protein Dynamics, Department of Biochemistry and Molecular Biology, University of Debrecen, H-4032 Debrecen, Hungary Received August 19, 2016; Revised October 07, 2016; Editorial Decision October 12, 2016; Accepted October 20, 2016 ABSTRACT multiplicity of structures and their plasticity bias these pro- teins for interactions with many different partners, either FuzDB (http://protdyn-database.org) compiles exper- simultaneously or in spatially/temporally separated fash- imentally observed fuzzy protein complexes, where ion (3). Although the biological importance of ID proteins intrinsic disorder (ID) is maintained upon interact- has been clearly established, the underlying molecular sce- ing with a partner (protein, nucleic acid or small narios remain to be elucidated. A common assumption is molecule) and directly impacts biological function. that while ID proteins/regions have excessive conforma- Entries in the database have both (i) structural ev- tional freedom in their free state in solution, this becomes idence demonstrating the structural multiplicity or rather limited when they interact with their partners (4). dynamic disorder of the ID region(s) in the part- In other words, IDPs/IDRs adopt a well-defined structure ner bound form of the protein and (ii) in vitro or upon recognizing a specific target, a phenomenon termed in vivo biological evidence that indicates the sig- as ‘coupled folding-binding’.
    [Show full text]
  • Mechanisms of Macromolecular Interactions Mediated by Protein
    Molecules and Cells Minireview Mechanisms of Macromolecular Interactions Mediated by Protein Intrinsic Disorder Sunghyun Hong1,2, Sangmin Choi1,2, Ryeonghyeon Kim1,2, and Junseock Koh1,* 1School of Biological Sciences, Seoul National University, Seoul 08826, Korea, 2These authors contributed equally to this work. *Correspondence: [email protected] https://doi.org/10.14348/molcells.2020.0186 www.molcells.org Intrinsically disordered proteins or regions (IDPs or IDRs) are INTRODUCTION widespread in the eukaryotic proteome. Although lacking stable three-dimensional structures in the free forms, IDRs In the classical structure-function paradigm, a protein must perform critical functions in various cellular processes. fold into a well-defined three-dimensional structure in or- Accordingly, mutations and altered expression of IDRs are der to carry out its function. The landmark achievements associated with many pathological conditions. Hence, it is underpinning this paradigm were the determination of the of great importance to understand at the molecular level first three-dimensional protein structures (myoglobin and how IDRs interact with their binding partners. In particular, hemoglobin) by Kendrew (Kendrew et al., 1958) and Perutz discovering the unique interaction features of IDRs originating (Perutz et al., 1960). In parallel, the elegant biochemical from their dynamic nature may reveal uncharted regulatory experiments by Anfinsen and colleagues further demonstrat- mechanisms of specific biological processes. Here we ed that the native three dimensional structure of a protein discuss the mechanisms of the macromolecular interactions is determined by its amino acid sequence (Anfinsen et al., mediated by IDRs and present the relevant cellular processes 1961). For more than half a century, the structure-function including transcription, cell cycle progression, signaling, paradigm has been one of the most fundamental frame- and nucleocytoplasmic transport.
    [Show full text]
  • Simple Biochemical Features Underlie Transcriptional Activation Domain Diversity and Dynamic, Fuzzy Binding to Mediator
    RESEARCH ARTICLE Simple biochemical features underlie transcriptional activation domain diversity and dynamic, fuzzy binding to Mediator Adrian L Sanborn1,2*, Benjamin T Yeh2, Jordan T Feigerle1, Cynthia V Hao1, Raphael JL Townshend2, Erez Lieberman Aiden3,4, Ron O Dror2, Roger D Kornberg1* 1Department of Structural Biology, Stanford University School of Medicine, Stanford, United States; 2Department of Computer Science, Stanford University, Stanford, United States; 3The Center for Genome Architecture, Baylor College of Medicine, Houston, United States; 4Center for Theoretical Biological Physics, Rice University, Houston, United States Abstract Gene activator proteins comprise distinct DNA-binding and transcriptional activation domains (ADs). Because few ADs have been described, we tested domains tiling all yeast transcription factors for activation in vivo and identified 150 ADs. By mRNA display, we showed that 73% of ADs bound the Med15 subunit of Mediator, and that binding strength was correlated with activation. AD-Mediator interaction in vitro was unaffected by a large excess of free activator protein, pointing to a dynamic mechanism of interaction. Structural modeling showed that ADs interact with Med15 without shape complementarity (‘fuzzy’ binding). ADs shared no sequence motifs, but mutagenesis revealed biochemical and structural constraints. Finally, a neural network trained on AD sequences accurately predicted ADs in human proteins and in other yeast proteins, including chromosomal proteins and chromatin remodeling complexes. These findings solve the *For correspondence: longstanding enigma of AD structure and function and provide a rationale for their role in biology. [email protected] (ALS); [email protected] (RDK) Competing interests: The authors declare that no Introduction competing interests exist. Transcription factors (TFs) perform the last step in signal transduction pathways.
    [Show full text]
  • Classifying the Binding Modes of Disordered Proteins
    International Journal of Molecular Sciences Review Classifying the Binding Modes of Disordered Proteins Monika Fuxreiter 1,2 1 Department of Biomedical Sciences, University of Padova, 35131 Padova, Italy; [email protected] 2 Laboratory of Protein Dynamics, University of Debrecen, 4032 Debrecen, Hungary Received: 20 October 2020; Accepted: 14 November 2020; Published: 16 November 2020 Abstract: Disordered proteins often act as interaction hubs in cellular pathways, via the specific recognition of a distinguished set of partners. While disordered regions can adopt a well-defined conformation upon binding, the coupled folding to binding model does not explain how interaction versatility is achieved. Here, I present a classification scheme for the binding modes of disordered protein regions, based on their conformational heterogeneity in the bound state. Binding modes are defined as (i) disorder-to-order transitions leading to a well-defined bound state, (ii) disordered binding leading to a disordered bound state and (iii) fuzzy binding when the degree of disorder in the bound state may vary with the partner or cellular conditions. Fuzzy binding includes polymorphic bound structures, conditional folding and dynamic binding. This classification scheme describes the structural continuum of complexes involving disordered regions as well as their context-dependent interaction behaviors. Keywords: protein interaction; disordered protein; fuzzy binding; context-dependence; conformational heterogeneity 1. Introduction Interactions mediated by disordered protein regions are critical for the regulation of numerous cellular pathways [1,2]. Although the benefits of structural plasticity in interaction versatility have been recognized [3], the molecular mechanisms and biophysical principles have remained rather enigmatic. The key questions are (i) the origin of selectivity, (ii) affinity versus specificity, (iii) selectivity for multiple partners and (iv) the plasticity of the interactions depending on the cellular conditions.
    [Show full text]
  • Src Family Tyrosine Kinases in Intestinal Homeostasis, Regeneration and Tumorigenesis
    cancers Review Src Family Tyrosine Kinases in Intestinal Homeostasis, Regeneration and Tumorigenesis Audrey Sirvent , Rudy Mevizou , Dana Naim , Marie Lafitte and Serge Roche * CRBM, CNRS, University of Montpellier, Equipe labellisée Ligue Contre le Cancer, F-34000 Montpellier, France; [email protected] (A.S.); [email protected] (R.M.); [email protected] (D.N.); marie.lafi[email protected] (M.L.) * Correspondence: [email protected] Received: 17 June 2020; Accepted: 19 July 2020; Published: 23 July 2020 Abstract: Src, originally identified as an oncogene, is a membrane-anchored tyrosine kinase and the Src family kinase (SFK) prototype. SFKs regulate the signalling induced by a wide range of cell surface receptors leading to epithelial cell growth and adhesion. In the intestine, the SFK members Src, Fyn and Yes regulate epithelial cell proliferation and migration during tissue regeneration and transformation, thus implicating conserved and specific functions. In patients with colon cancer, SFK activity is a marker of poor clinical prognosis and a potent driver of metastasis formation. These tumorigenic activities are linked to SFK capacity to promote the dissemination and tumour-initiating capacities of epithelial tumour cells. However, it is unclear how SFKs promote colon tumour formation and metastatic progression because SFK-encoding genes are unfrequently mutated in human cancer. Here, we review recent findings on SFK signalling during intestinal homeostasis, regeneration and tumorigenesis. We also describe the key nongenetic mechanisms underlying SFK tumour activities in colorectal cancer, and discuss how these mechanisms could be exploited in therapeutic strategies to target SFK signalling in metastatic colon cancer.
    [Show full text]
  • 2021.04.15.439979V1.Full.Pdf
    bioRxiv preprint doi: https://doi.org/10.1101/2021.04.15.439979; this version posted April 15, 2021. The copyright holder for this preprint (which was not certified by peer review) is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity. It is made available under aCC-BY 4.0 International license. Parallel and sequential pathways of molecular recognition of a tandem-repeat protein and its intrinsically disordered binding partner Ben M. Smith1, Pamela J. E. Rowling1*, Chris M. Dobson2 & Laura S. Itzhaki1* 1Department of Pharmacology University of Cambridge, Tennis Court Road, Cambridge CB2 1PD 2Department of Chemistry University of Cambridge, Lensfield Road, Cambridge CB2 1EW * Corresponding authors, [email protected] and [email protected] 1 bioRxiv preprint doi: https://doi.org/10.1101/2021.04.15.439979; this version posted April 15, 2021. The copyright holder for this preprint (which was not certified by peer review) is the author/funder, who has granted bioRxiv a license to display the preprint in perpetuity. It is made available under aCC-BY 4.0 International license. The Wnt signalling pathway plays an important role in cell proliferation, differentiation and fate decisions in embryonic development and in the maintenance of adult tissues, and the twelve Armadillo (ARM) repeat-containing protein β-catenin acts as the signal transducer in this pathway. Here we investigate the interaction between β-catenin and the intrinsically disordered transcription factor TCF7L2, comprising a very long nanomolar-affinity interface of approximately 4800 Å2 that spans ten of the twelve ARM repeats of β-catenin.
    [Show full text]