Structural analysis of the adenovirus type 2 E3/19K protein using mutagenesis and a panel of conformation-sensitive monoclonal antibodies

Ahmed; Altschul; Andersson; Beatrice Menz; Beier; Bennett; Bruder; Bryson; Burgert; Burgert; Burgert; Burgert; Burgert; Cole; Cox; Deryckere; Edgar; Elsing; Feuerbach; Flomenberg; Flomenberg; Fox; Gabathuler; Gewurz; Ginsberg; Hans-Gerhard Burgert; Hermiston; Hilgendorf; Jackson; Jackson; Jefferies; Katja Koebernick; Kornfeld; Krogh; Kurowski; Köhler; Körner; Lichtenstein; Liu; Liu; Lodoen; Mans; Martina Sester; McNees; McSharry; Nilsson; Persson; Pääbo; Pääbo; Pääbo; Ralf Schmid; Rawle; Rost; Rost; Rost; Sester; Sester; Tanaka; The_UniProt_Consortium; von Herrath; Windheim; Wold; Wold

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Structural analysis of the adenovirus type 2 E3/19K protein using mutagenesis and a panel of conformation-sensitive monoclonal antibodies

Authors: Ahmed
Altschul
Andersson
Beatrice Menz
Beier
Bennett
Bruder
Bryson
Burgert
Burgert
Burgert
Burgert
Burgert
Cole
Cox
Deryckere
Edgar
Elsing
Feuerbach
Flomenberg
Flomenberg
Fox
Gabathuler
Gewurz
Ginsberg
Hans-Gerhard Burgert
Hermiston
Hilgendorf
Jackson
Jackson
Jefferies
Katja Koebernick
Kornfeld
Krogh
Kurowski
Köhler
Körner
Lichtenstein
Liu
Liu
Lodoen
Mans
Martina Sester
McNees
McSharry
Nilsson
Persson
Pääbo
Pääbo
Pääbo
Ralf Schmid
Rawle
Rost
Rost
Rost
Sester
Sester
Tanaka
The_UniProt_Consortium
von Herrath
Windheim
Wold
Wold
Publication date: 1 November 2008
Publisher: 'Elsevier BV'
Doi

Abstract

The E3/19K protein of human adenovirus type 2 (Ad2) was the first viral protein shown to interfere with antigen presentation. This 25 kDa transmembrane glycoprotein binds to major histocompatibility complex (MHC) class I molecules in the endoplasmic reticulum (ER), thereby preventing transport of newly synthesized peptide–MHC complexes to the cell surface and consequently T cell recognition. Recent data suggest that E3/19K also sequesters MHC class I like ligands intracellularly to suppress natural killer (NK) cell recognition. While the mechanism of ER retention is well understood, the structure of E3/19K remains elusive. To further dissect the structural and antigenic topography of E3/19K we carried out site-directed mutagenesis and raised monoclonal antibodies (mAbs) against a recombinant version of Ad2 E3/19K comprising the lumenal domain followed by a C-terminal histidine tag. Using peptide scanning, the epitopes of three mAbs were mapped to different regions of the lumenal domain, comprising amino acids 3–13, 15–21 and 41–45, respectively. Interestingly, mAb 3F4 reacted only weakly with wild-type E3/19K, but showed drastically increased binding to mutant E3/19K molecules, e.g. those with disrupted disulfide bonds, suggesting that 3F4 can sense unfolding of the protein. MAb 10A2 binds to an epitope apparently buried within E3/19K while that of 3A9 is exposed. Secondary structure prediction suggests that the lumenal domain contains six β-strands and an α-helix adjacent to the transmembrane domain. Interestingly, all mAbs bind to non-structured loops. Using a large panel of E3/19K mutants the structural alterations of the mutations were determined. With this knowledge the panel of mAbs will be valuable tools to further dissect structure/function relationships of E3/19K regarding down regulation of MHC class I and MHC class I like molecules and its effect on both T cell and NK cell recognition

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