Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase

BACKGROUND: Protein-protein interactions are at the basis of many cellular processes, and they are also involved in the interaction between pathogens and their host(s). Many intracellular pathogenic bacteria translocate proteins called effectors into the cytoplasm of the infected host cell, and thes...

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Autores principales: Nkengfac, Bernard, Pouyez, Jenny, Bauwens, Emilie, Vandenhaute, Jean, Letesson, Jean-Jacques, Wouters, Johan, De Bolle, Xavier
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2012
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3527289/
https://www.ncbi.nlm.nih.gov/pubmed/22892012
http://dx.doi.org/10.1186/1471-2091-13-16
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author Nkengfac, Bernard
Pouyez, Jenny
Bauwens, Emilie
Vandenhaute, Jean
Letesson, Jean-Jacques
Wouters, Johan
De Bolle, Xavier
author_facet Nkengfac, Bernard
Pouyez, Jenny
Bauwens, Emilie
Vandenhaute, Jean
Letesson, Jean-Jacques
Wouters, Johan
De Bolle, Xavier
author_sort Nkengfac, Bernard
collection PubMed
description BACKGROUND: Protein-protein interactions are at the basis of many cellular processes, and they are also involved in the interaction between pathogens and their host(s). Many intracellular pathogenic bacteria translocate proteins called effectors into the cytoplasm of the infected host cell, and these effectors can interact with one or several host protein(s). An effector named RicA was recently reported in Brucella abortus to specifically interact with human Rab2 and to affect intracellular trafficking of this pathogen. RESULTS: In order to identify regions of the RicA protein involved in the interaction with Rab2, RicA was subjected to extensive random mutagenesis using error prone polymerase chain reaction. The resulting allele library was selected by the yeast two-hybrid assay for Rab2-interacting clones that were isolated and sequenced, following the “absence of interference” approach. A tridimensional model of RicA structure was used to position the substitutions that did not affect RicA-Rab2 interaction, giving a “negative image” of the putative interaction region. Since RicA is a bacterial conserved protein, RicA homologs were also tested against Rab2 in a yeast two-hybrid assay, and the C. crescentus homolog of RicA was found to interact with human Rab2. Analysis of the RicA structural model suggested that regions involved in the folding of the “beta helix” or an exposed loop with the IGFP sequence could also be involved in the interaction with Rab2. Extensive mutagenesis of the IGFP loop suggested that loss of interaction with Rab2 was correlated with insolubility of the mutated RicA, showing that “absence of interference” approach also generates surfaces that could be necessary for folding. CONCLUSION: Extensive analysis of substitutions in RicA unveiled two structural elements on the surface of RicA, the most exposed β-sheet and the IGFP loop, which could be involved in the interaction with Rab2 and protein folding. Our analysis of mutants in the IGFP loop suggests that, at least for some mono-domain proteins such as RicA, protein interaction analysis using allele libraries could be complicated by the dual effect of many substitutions affecting both folding and protein-protein interaction.
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spelling pubmed-35272892012-12-21 Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase Nkengfac, Bernard Pouyez, Jenny Bauwens, Emilie Vandenhaute, Jean Letesson, Jean-Jacques Wouters, Johan De Bolle, Xavier BMC Biochem Research Article BACKGROUND: Protein-protein interactions are at the basis of many cellular processes, and they are also involved in the interaction between pathogens and their host(s). Many intracellular pathogenic bacteria translocate proteins called effectors into the cytoplasm of the infected host cell, and these effectors can interact with one or several host protein(s). An effector named RicA was recently reported in Brucella abortus to specifically interact with human Rab2 and to affect intracellular trafficking of this pathogen. RESULTS: In order to identify regions of the RicA protein involved in the interaction with Rab2, RicA was subjected to extensive random mutagenesis using error prone polymerase chain reaction. The resulting allele library was selected by the yeast two-hybrid assay for Rab2-interacting clones that were isolated and sequenced, following the “absence of interference” approach. A tridimensional model of RicA structure was used to position the substitutions that did not affect RicA-Rab2 interaction, giving a “negative image” of the putative interaction region. Since RicA is a bacterial conserved protein, RicA homologs were also tested against Rab2 in a yeast two-hybrid assay, and the C. crescentus homolog of RicA was found to interact with human Rab2. Analysis of the RicA structural model suggested that regions involved in the folding of the “beta helix” or an exposed loop with the IGFP sequence could also be involved in the interaction with Rab2. Extensive mutagenesis of the IGFP loop suggested that loss of interaction with Rab2 was correlated with insolubility of the mutated RicA, showing that “absence of interference” approach also generates surfaces that could be necessary for folding. CONCLUSION: Extensive analysis of substitutions in RicA unveiled two structural elements on the surface of RicA, the most exposed β-sheet and the IGFP loop, which could be involved in the interaction with Rab2 and protein folding. Our analysis of mutants in the IGFP loop suggests that, at least for some mono-domain proteins such as RicA, protein interaction analysis using allele libraries could be complicated by the dual effect of many substitutions affecting both folding and protein-protein interaction. BioMed Central 2012-08-14 /pmc/articles/PMC3527289/ /pubmed/22892012 http://dx.doi.org/10.1186/1471-2091-13-16 Text en Copyright ©2012 Nkengfac et al.; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Research Article
Nkengfac, Bernard
Pouyez, Jenny
Bauwens, Emilie
Vandenhaute, Jean
Letesson, Jean-Jacques
Wouters, Johan
De Bolle, Xavier
Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase
title Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase
title_full Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase
title_fullStr Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase
title_full_unstemmed Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase
title_short Structural analysis of Brucella abortus RicA substitutions that do not impair interaction with human Rab2 GTPase
title_sort structural analysis of brucella abortus rica substitutions that do not impair interaction with human rab2 gtpase
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3527289/
https://www.ncbi.nlm.nih.gov/pubmed/22892012
http://dx.doi.org/10.1186/1471-2091-13-16
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