Literature DB >> 18321067

Characterization of the neuron-specific L1-CAM cytoplasmic tail: naturally disordered in solution it exercises different binding modes for different adaptor proteins.

Sergiy Tyukhtenko1, Lalit Deshmukh, Vineet Kumar, Jeffrey Lary, James Cole, Vance Lemmon, Olga Vinogradova.   

Abstract

L1, a highly conserved transmembrane glycoprotein member of the immunoglobulin superfamily of cell adhesion molecules, mediates many developmental processes in the nervous system. Here we present the biophysical characterization and the binding properties of the least structurally defined part of this receptor: its cytoplasmic tail (CT). We have shown by analytical ultracentrifugation and dynamic light scattering experiments that it is mostly monomeric and unstructured in aqueous solution. We have defined by nuclear magnetic resonance the molecular details of L1-CT binding to two major targets: a membrane-cytoskeletal linker (MCL), ezrin, and an endocytosis mediator, AP2. Surprisingly, in addition to the two previously identified ezrin binding motifs, the juxtamembrane and the (1176)YRSLE regions, we have discovered a third one, a part of which has been previously associated with binding to another MCL, ankyrin. For the L1 interaction with AP2 we have determined the precise interaction region surrounding the (1176)YRSLE binding site and that this overlaps with the second ezrin binding site. In addition, we have shown that the juxtamembrane region of L1-CT has some binding affinity to AP2-mu2, although the specificity of this interaction needs further investigation. These data indicate that L1-CT belongs to the class of intrinsically disordered proteins. Endogenous flexibility of L1-CT might play an important role in dynamic regulation of intracellular signaling: the ability of cytoplasmic tails to accommodate different targets has the potential to fine-tune signal transduction via cell surface receptors.

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Year:  2008        PMID: 18321067      PMCID: PMC2426742          DOI: 10.1021/bi702433q

Source DB:  PubMed          Journal:  Biochemistry        ISSN: 0006-2960            Impact factor:   3.162


  34 in total

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Authors:  O Vinogradova; T Haas; E F Plow; J Qin
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2.  A third specificity-determining site in mu 2 adaptin for sequences upstream of Yxx phi sorting motifs.

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Journal:  Traffic       Date:  2001-02       Impact factor: 6.215

3.  The role of endocytic l1 trafficking in polarized adhesion and migration of nerve growth cones.

Authors:  H Kamiguchi; F Yoshihara
Journal:  J Neurosci       Date:  2001-12-01       Impact factor: 6.167

4.  Structural basis of adhesion-molecule recognition by ERM proteins revealed by the crystal structure of the radixin-ICAM-2 complex.

Authors:  Keisuke Hamada; Toshiyuki Shimizu; Shigenobu Yonemura; Shoichiro Tsukita; Sachiko Tsukita; Toshio Hakoshima
Journal:  EMBO J       Date:  2003-02-03       Impact factor: 11.598

5.  Solution NMR study of the monomeric form of p13suc1 protein sheds light on the hinge region determining the affinity for a phosphorylated substrate.

Authors:  Benoît Odaert; Isabelle Landrieu; Klaas Dijkstra; Gea Schuurman-Wolters; Peter Casteels; Jean-Michel Wieruszeski; Dirk Inze; Ruud Scheek; Guy Lippens
Journal:  J Biol Chem       Date:  2002-01-25       Impact factor: 5.157

6.  Size-distribution analysis of macromolecules by sedimentation velocity ultracentrifugation and lamm equation modeling.

Authors:  P Schuck
Journal:  Biophys J       Date:  2000-03       Impact factor: 4.033

7.  Activation of the MAPK signal cascade by the neural cell adhesion molecule L1 requires L1 internalization.

Authors:  A W Schaefer; H Kamiguchi; E V Wong; C M Beach; G Landreth; V Lemmon
Journal:  J Biol Chem       Date:  1999-12-31       Impact factor: 5.157

8.  Plasmin-sensitive dibasic sequences in the third fibronectin-like domain of L1-cell adhesion molecule (CAM) facilitate homomultimerization and concomitant integrin recruitment.

Authors:  S Silletti; F Mei; D Sheppard; A M Montgomery
Journal:  J Cell Biol       Date:  2000-06-26       Impact factor: 10.539

9.  L1 endocytosis is controlled by a phosphorylation-dephosphorylation cycle stimulated by outside-in signaling by L1.

Authors:  Andrew W Schaefer; Yoshimasa Kamei; Hiroyuki Kamiguchi; Eric V Wong; Iris Rapoport; Tomas Kirchhausen; Carol M Beach; Gary Landreth; Sandra K Lemmon; Vance Lemmon
Journal:  J Cell Biol       Date:  2002-06-24       Impact factor: 10.539

10.  Functional binding interaction identified between the axonal CAM L1 and members of the ERM family.

Authors:  Tracey C Dickson; C David Mintz; Deanna L Benson; Stephen R J Salton
Journal:  J Cell Biol       Date:  2002-06-17       Impact factor: 10.539

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  4 in total

1.  Inside-out regulation of L1 conformation, integrin binding, proteolysis, and concomitant cell migration.

Authors:  Maxine M Chen; Chia-Yao Lee; Hyuma A Leland; Grace Y Lin; Anthony M Montgomery; Steve Silletti
Journal:  Mol Biol Cell       Date:  2010-03-24       Impact factor: 4.138

2.  Tyrosine and serine phosphorylation regulate the conformation and subsequent threonine phosphorylation of the L1 cytoplasmic domain.

Authors:  Maxine M Chen; Hyuma A Leland; Chia-Yao Lee; Steve Silletti
Journal:  Biochem Biophys Res Commun       Date:  2009-08-29       Impact factor: 3.575

3.  Full-length L1CAM and not its Δ2Δ27 splice variant promotes metastasis through induction of gelatinase expression.

Authors:  Stephanie Hauser; Laura Bickel; Dirk Weinspach; Michael Gerg; Michael K Schäfer; Marco Pfeifer; John Hazin; Florian Schelter; Ulrich H Weidle; Juliane Ramser; Juliane Volkmann; Alfons Meindl; Manfred Schmitt; Florian Schrötzlmair; Peter Altevogt; Achim Krüger
Journal:  PLoS One       Date:  2011-04-25       Impact factor: 3.240

4.  Investigation of the adaptor protein PLIC-2 in multiple pathways.

Authors:  Khiem Nguyen; Robbins Puthenveetil; Olga Vinogradova
Journal:  Biochem Biophys Rep       Date:  2017-02-03
  4 in total

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