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LAReferencia - Red Federada de Repositorios Institucionales de Publicaciones Científicas Latinoamericanas

A disordered region retains the full protease inhibitor activity and the capacity to induce CD8+ T cells in vivo of the oral vaccine adjuvant U-Omp19

Author: Bruno Laura
Cassataro Juliana
Cerutti María Laura
Chemes Lucía B.
Coria Lorena M.
Darriba María Laura
Klinke Sebastián
Otero Lisandro H.
Pasquevich Karina A.
Pueblas Castro Celeste
Rasia Rodolfo M.
Publication venue: 'Elsevier BV'
Publication date: 01/01/2022
Field of study

U-Omp19 is a bacterial protease inhibitor from Brucella abortus that inhibits gastrointestinal and lysosomal proteases, enhancing the half-life and immunogenicity of co-delivered antigens. U-Omp19 is a novel adjuvant that is in preclinical development with various vaccine candidates. However, the molecular mechanisms by which it exerts these functions and the structural elements responsible for these activities remain unknown. In this work, a structural, biochemical, and functional characterization of U-Omp19 is presented. Dynamic features of U-Omp19 in solution by NMR and the crystal structure of its C-terminal domain are described. The protein consists of a compact C-terminal beta-barrel domain and a flexible N-terminal domain. The latter domain behaves as an intrinsically disordered protein and retains the full protease inhibitor activity against pancreatic elastase, papain and pepsin. This domain also retains the capacity to induce CD8+ T cells in vivo of U-Omp19. This information may lead to future rationale vaccine designs using U-Omp19 as an adjuvant to deliver other proteins or peptides in oral formulations against infectious diseases, as well as to design strategies to incorporate modifications in its structure that may improve its adjuvanticity.Fil: Darriba, María Laura. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Pueblas Castro, Celeste. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Coria, Lorena M. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Bruno, Laura. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Cerutti, María Laura. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Chemes, Lucía B. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Cassataro, Juliana. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Pasquevich, Karina A. Universidad Nacional de San Martín. Instituto de Investigaciones Biotecnológicas. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Darriba, María Laura. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Pueblas Castro, Celeste. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Coria, Lorena M. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Bruno, Laura. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Cerutti, María Laura. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Chemes, Lucía B. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Cassataro, Juliana. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Pasquevich, Karina A. Universidad Nacional de San Martín. Escuela de Bio y Nanotecnologías (EByN); Argentina.Fil: Otero, Lisandro H. Fundación Instituto Leloir. Plataforma Argentina de Biología Estructural y Metabolómica. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Klinke, Sebastián. Fundación Instituto Leloir. Plataforma Argentina de Biología Estructural y Metabolómica. Consejo Nacional de Investigaciones Científicas y Técnicas; Argentina.Fil: Rasia, Rodolfo M. Universidad Nacional de Rosario. Facultad de Ciencias Bioquímicas y Farmacéuticas. Instituto de Biología Molecular y Celular de Rosario. Plataforma Argentina de Biología Estructural y Metabolómica; Argentina

Repositorio Hipermedial de la Universidad Nacional de Rosario

Unlipidated Outer Membrane Protein Omp16 (U-Omp16) from Brucella spp. as Nasal Adjuvant Induces a Th1 Immune Response and Modulates the Th2 Allergic Response to Cow's Milk Proteins

Author: Cassataro Juliana
Coria Lorena M.
Delpino María V.
Docena Guillermo Horacio
Fossati Carlos Alberto
Giambartolomei Guillermo H.
Ibáñez Andrés Esteban
Oliveira Sergio C.
Pacífico Lucila G. G.
Pasquevich Karina A.
Risso Gabriela S.
Smaldini Paola Lorena
Publication venue
Publication date: 14/11/2019
Field of study

The discovery of novel mucosal adjuvants will help to develop new formulations to control infectious and allergic diseases. In this work we demonstrate that U-Omp16 from Brucella spp. delivered by the nasal route (i.n.) induced an inflammatory immune response in bronchoalveolar lavage (BAL) and lung tissues. Nasal co-administration of U-Omp16 with the model antigen (Ag) ovalbumin (OVA) increased the amount of Ag in lung tissues and induced OVA-specific systemic IgG and T helper (Th) 1 immune responses. The usefulness of U-Omp16 was also assessed in a mouse model of food allergy. U-Omp16 i.n. administration during sensitization ameliorated the hypersensitivity responses of sensitized mice upon oral exposure to Cow's Milk Protein (CMP), decreased clinical signs, reduced anti-CMP IgE serum antibodies and modulated the Th2 response in favor of Th1 immunity. Thus, U-Omp16 could be used as a broad Th1 mucosal adjuvant for different Ag formulations.Laboratorio de Investigaciones del Sistema Inmun

Unlipidated Outer Membrane Protein Omp16 (U-Omp16) from Brucella spp. as Nasal Adjuvant Induces a Th1 Immune Response and Modulates the Th2 Allergic Response to Cow's Milk Proteins

Author: Cassataro Juliana
Coria Lorena M.
Delpino María V.
Docena Guillermo Horacio
Fossati Carlos Alberto
Giambartolomei Guillermo H.
Ibáñez Andrés Esteban
Oliveira Sergio C.
Pacífico Lucila G. G.
Pasquevich Karina A.
Risso Gabriela S.
Smaldini Paola Lorena
Publication venue
Publication date: 14/11/2019
Field of study

Servicio de Difusión de la Creación Intelectual

An Oral Vaccine Based on U-Omp19 Induces Protection against B. abortus Mucosal Challenge by Inducing an Adaptive IL-17 Immune Response in Mice

Author: A Al-Mariri
A Cabrera
A Pashine
A Tibor
AN Sieve
Andrés E. Ibañez
Astrid Zwerdling
B Golding
CA Velikovsky
Christine Seither
CL Baldwin
CL Baldwin
Clara García Samartino
DA Ashford
DM Magnani
DS Pontes
EA Murphy
F Roth
F Sala
Fernanda S. Oliveira
G Matsuzaki
GG Schurig
GH Giambartolomei
GP Priebe
Guillermo H. Giambartolomei
Heribert Warzecha
HS Mason
J Cassataro
J Cassataro
J Cassataro
J Cassataro
J Cassataro
J Holmgren
J Rice
JP Gorvel
Juliana Cassataro
K Fujihashi
KA Pasquevich
KA Pasquevich
Karina A. Pasquevich
KD Meeks
KI Happel
L Lin
LC Freytag
LE Brown
Lorena M. Coria
M Raffatellu
M Umemura
MA Fiorentino
Mauricio Martins Rodrigues
MG Stevens
MJ Izadjoo
MM Curtis
MP Jimenez de Bagues
MR Neutra
MV Delpino
P Nicoletti
P Pasquali
P Ye
Paula Barrionuevo
PE Shewen
RA Bowden
S Kohler
S Liljeqvist
S Marillonnet
SA Khader
SA Khader
SA Khader
SC Higgins
SD Perkins
Sergio C. Oliveira
SG Reed
Silvia M. Estein
SJ Streatfield
SM Schulz
SM Schulz
T Korn
TJ Stabel
W Huang
Y Lin
Publication venue: Public Library of Science
Publication date: 01/01/2011
Field of study

As Brucella infections occur mainly through mucosal surfaces, the development of mucosal administered vaccines could be radical for the control of brucellosis. In this work we evaluated the potential of Brucella abortus 19 kDa outer membrane protein (U-Omp19) as an edible subunit vaccine against brucellosis. We investigated the protective immune response elicited against oral B. abortus infection after vaccination of mice with leaves from transgenic plants expressing U-Omp19; or with plant-made or E. coli-made purified U-Omp19. All tested U-Omp19 formulations induced protection against Brucella when orally administered without the need of adjuvants. U-Omp19 also induced protection against a systemic challenge when parenterally administered. This built-in adjuvant ability of U-Omp19 was independent of TLR4 and could be explained at least in part by its capability to activate dendritic cells in vivo. While unadjuvanted U-Omp19 intraperitoneally administered induced a specific Th1 response, following U-Omp19 oral delivery a mixed specific Th1-Th17 response was induced. Depletion of CD4+ T cells in mice orally vaccinated with U-Omp19 resulted in a loss of the elicited protection, indicating that this cell type mediates immune protection. The role of IL-17 against Brucella infection has never been explored. In this study, we determined that if IL-17A was neutralized in vivo during the challenge period, the mucosal U-Omp19 vaccine did not confer mucosal protection. On the contrary, IL-17A neutralization during the infection did not influence at all the subsistence and growth of this bacterium in PBS-immunized mice. All together, our results indicate that an oral unadjuvanted vaccine based on U-Omp19 induces protection against a mucosal challenge with Brucella abortus by inducing an adaptive IL-17 immune response. They also indicate different and important new aspects i) IL-17 does not contribute to reduce the bacterial burden in non vaccinated mice and ii) IL-17 plays a central role in vaccine mediated anti-Brucella mucosal immunity

Public Library of Science (PLOS)

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Depletion of Dendritic Cells Enhances Innate Anti-Bacterial Host Defense through Modulation of Phagocyte Homeostasis

Author: AA Navarini
Ana Novakovic
AP Tittel
BD Corbin
C De Trez
C Elbim
C Summers
C Waskow
Cecilia Lucero Estrada
CJ Chen
CL Semerad
D Bell
Doreen Drechsler
DT Fearon
F Hayashi
F Sallusto
FL Craciun
GH Wabnitz
GH Wabnitz
GH Wabnitz
Guido H. Wabnitz
Günter J. Hämmerling
HJ McKenna
IB Autenrieth
IB Autenrieth
Ingo B. Autenrieth
J Banchereau
J Bohannon
JA Hoffmann
JE Galan
K Hochweller
K Hochweller
Karina A. Pasquevich
KJ Eash
Kristin Hochweller
KW Tinsley
L Mölne
M Kinoshita
Manina Günter
MF Oellerich
MH Kim
MJ Christopher
N Borregaard
N Onai
Natalio Garbi
NV Serbina
NV Serbina
NV Serbina
O Guisset
P Scapini
PA Efron
Philipp Warnke
PO Scumpia
PY Lee
R Medzhitov
R Taneja
RM Steinman
RS Hotchkiss
S Akira
S Jung
S Yona
Sabine Ehrt
Sandra Beer-Hammer
SE Autenrieth
SH Naik
Stella E. Autenrieth
T Birnberg
T De Smedt
TB Issekutz
TL Cover
Y Tsuda
Yvonne Samstag
Publication venue: Public Library of Science
Publication date: 01/02/2012
Field of study

Dendritic cells (DCs) as professional antigen-presenting cells play an important role in the initiation and modulation of the adaptive immune response. However, their role in the innate immune response against bacterial infections is not completely defined. Here we have analyzed the role of DCs and their impact on the innate anti-bacterial host defense in an experimental infection model of Yersinia enterocolitica (Ye). We used CD11c-diphtheria toxin (DT) mice to deplete DCs prior to severe infection with Ye. DC depletion significantly increased animal survival after Ye infection. The bacterial load in the spleen of DC-depleted mice was significantly lower than that of control mice throughout the infection. DC depletion was accompanied by an increase in the serum levels of CXCL1, G-CSF, IL-1α, and CCL2 and an increase in the numbers of splenic phagocytes. Functionally, splenocytes from DC-depleted mice exhibited an increased bacterial killing capacity compared to splenocytes from control mice. Cellular studies further showed that this was due to an increased production of reactive oxygen species (ROS) by neutrophils. Adoptive transfer of neutrophils from DC-depleted mice into control mice prior to Ye infection reduced the bacterial load to the level of Ye-infected DC-depleted mice, suggesting that the increased number of phagocytes with additional ROS production account for the decreased bacterial load. Furthermore, after incubation with serum from DC-depleted mice splenocytes from control mice increased their bacterial killing capacity, most likely due to enhanced ROS production by neutrophils, indicating that serum factors from DC-depleted mice account for this effect. In summary, we could show that DC depletion triggers phagocyte accumulation in the spleen and enhances their anti-bacterial killing capacity upon bacterial infection

LAReferencia - Red Federada de Repositorios Institucionales de Publicaciones Científicas Latinoamericanas

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Antibody Reactivity to Omp31 from Brucella melitensis in Human and Animal Infections by Smooth and Rough Brucellae

Author: Baldi Pablo C.
Bruno Laura
Cassataro Juliana
Fossati Carlos A.
Pasquevich Karina
Wallach Jorge C.
Publication venue: American Society for Microbiology
Publication date: 01/01/2004
Field of study

Group 3 of outer membrane proteins (OMPs) of Brucella includes Omp25 and Omp31, which share 34% identity. Omp25 is highly conserved in Brucella species, and Omp31 is present in all Brucella species, except Brucella abortus. Antibodies to Brucella melitensis Omp31 have been sought only in infected sheep, and Western blotting of sera from infected sheep did not reveal anti-Omp31 reactivity. We obtained recombinant purified Omp31 (B. melitensis) and tested its recognition by sera from humans and animals suffering from brucellosis by an indirect enzyme-linked immunosorbent assay (ELISA). Serum samples from 74 patients, 57 sheep, and 47 dogs were analyzed; brucellosis was confirmed by bacteriological isolation in all ovine and canine cases and 31 human cases of brucellosis. Thirty-five patients (47%) were positive for antibodies to Omp31, including seven cases of Brucella suis infection, two cases of B. abortus infection, and three cases of B. melitensis infection. Of 39 sheep naturally infected with B. melitensis (biovars 1 and 3), 23 (59%) were positive for antibodies to Omp31. Anti-Omp31 antibodies were also detected in 12 of 18 rams (67%) in which Brucella ovis was isolated from semen. Antibodies to Omp31 were also found in 41 (87%) of the 47 dogs, including 13 with recent infection. These results suggest that an indirect ELISA using recombinant purified Omp31 from B. melitensis would be of limited value for the diagnosis of human and animal brucellosis. Nevertheless, the potential usefulness of this antigen in combination with other recombinant proteins from Brucella should not be dismissed.

Vaccination with the Recombinant Brucella Outer Membrane Protein 31 or a Derived 27-Amino-Acid Synthetic Peptide Elicits a CD4(+) T Helper 1 Response That Protects against Brucella melitensis Infection

Author: Bowden Raúl
Cassataro Juliana
de la Barrera Silvia
Estein Silvia M.
Fossati Carlos A.
Giambartolomei Guillermo H.
Pasquevich Karina A.
Velikovsky Carlos A.
Publication venue: American Society for Microbiology
Publication date: 01/12/2005
Field of study

The immunogenicity and protective efficacy of the recombinant 31-kDa outer membrane protein from Brucella melitensis (rOmp31), administered with incomplete Freund's adjuvant, were evaluated in mice. Immunization of BALB/c mice with rOmp31 conferred protection against B. ovis and B. melitensis infection. rOmp31 induced a vigorous immunoglobulin G (IgG) response, with higher IgG1 than IgG2 titers. In addition, spleen cells from rOmp31-immunized mice produced interleukin 2 (IL-2) and gamma interferon, but not IL-10 or IL-4, after in vitro stimulation with rOmp31, suggesting the induction of a T helper 1 (Th1) response. Splenocytes from rOmp31-vaccinated animals also induced a specific cytotoxic-T-lymphocyte activity, which led to the in vitro lysis of Brucella-infected macrophages. In vitro T-cell subset depletion indicated that rOmp31 immunization elicited specific CD4(+) T cells that secrete IL-2 and gamma interferon, while CD8(+) T cells induced cytotoxic-T-lymphocyte activity. In vivo depletion of T-cell subsets showed that the rOmp31-elicited protection against B. melitensis infection is mediated by CD4(+) T cells while the contribution of CD8(+) T cells may be limited. We then evaluated the immunogenicity and protective efficacy of a known exposed region from Omp31 on the Brucella membrane, a peptide that contains amino acids 48 to 74 of Omp31. Immunization with the synthetic peptide in adjuvant did not elicit a specific humoral response but elicited a Th1 response mediated by CD4(+) T cells. The peptide in adjuvant induced levels of protection similar to those induced by rOmp31 against B. melitensis but less protection than was induced by rOmp31 against B. ovis. Our results indicate that rOmp31 could be a useful candidate for the development of subunit vaccines against B. melitensis and B. ovis

Brucella abortus Inhibits Major Histocompatibility Complex Class II Expression and Antigen Processing through Interleukin-6 Secretion via Toll-Like Receptor 2▿

Author: Barrionuevo Paula
Cassataro Juliana
Delpino M. Victoria
Fossati Carlos A.
Giambartolomei Guillermo H.
Pasquevich Karina A.
Samartino Clara García
Wallach Jorge C.
Zwerdling Astrid
Publication venue: American Society for Microbiology (ASM)
Publication date: 01/12/2008
Field of study

The strategies that allow Brucella abortus to survive inside macrophages for prolonged periods and to avoid the immunological surveillance of major histocompatibility complex class II (MHC-II)-restricted gamma interferon (IFN-γ)-producing CD4+ T lymphocytes are poorly understood. We report here that infection of THP-1 cells with B. abortus inhibited expression of MHC-II molecules and antigen (Ag) processing. Heat-killed B. abortus (HKBA) also induced both these phenomena, indicating the independence of bacterial viability and involvement of a structural component of the bacterium. Accordingly, outer membrane protein 19 (Omp19), a prototypical B. abortus lipoprotein, inhibited both MHC-II expression and Ag processing to the same extent as HKBA. Moreover, a synthetic lipohexapeptide that mimics the structure of the protein lipid moiety also inhibited MHC-II expression, indicating that any Brucella lipoprotein could down-modulate MHC-II expression and Ag processing. Inhibition of MHC-II expression and Ag processing by either HKBA or lipidated Omp19 (L-Omp19) depended on Toll-like receptor 2 and was mediated by interleukin-6. HKBA or L-Omp19 also inhibited MHC-II expression and Ag processing of human monocytes. In addition, exposure to the synthetic lipohexapeptide inhibited Ag-specific T-cell proliferation and IFN-γ production of peripheral blood mononuclear cells from Brucella-infected patients. Together, these results indicate that there is a mechanism by which B. abortus may prevent recognition by T cells to evade host immunity and establish a chronic infection

LAReferencia - Red Federada de Repositorios Institucionales de Publicaciones Científicas Latinoamericanas

LAReferencia - Red Federada de Repositorios Institucionales de Publicaciones Científicas Latinoamericanas

Immunization with Recombinant Brucella Species Outer Membrane Protein Omp16 or Omp19 in Adjuvant Induces Specific CD4+ and CD8+ T Cells as Well as Systemic and Oral Protection against Brucella abortus Infection▿

Author: Barrionuevo Paula
Cassataro Juliana
Coria Lorena M.
Estein Silvia M.
Fossati Carlos A.
Giambartolomei Guillermo H.
Pasquevich Karina A.
Samartino Clara García
Zwerdling Astrid
Publication venue: American Society for Microbiology (ASM)
Publication date: 01/01/2009
Field of study

Available vaccines against Brucella spp. are live attenuated Brucella strains. In order to engineer a better vaccine to be used in animals and humans, our laboratory aims to develop an innocuous subunit vaccine. Particularly, we are interested in the outer membrane proteins (OMPs) of B. abortus: Omp16 and Omp19. In this study, we assessed the use of these proteins as vaccines against Brucella in BALB/c mice. Immunization with lipidated Omp16 (L-Omp16) or L-Omp19 in incomplete Freund's adjuvant (IFA) conferred significant protection against B. abortus infection. Vaccination with unlipidated Omp16 (U-Omp16) or U-Omp19 in IFA induced a higher degree of protection than the respective lipidated versions. Moreover, the level of protection induced after U-Omp16 or U-Omp19 immunization in IFA was similar to that elicited by live B. abortus S19 immunization. Flow cytometric analysis showed that immunization with U-Omp16 or U-Omp19 induced antigen-specific CD4+ as well as CD8+ T cells producing gamma interferon. In vivo depletion of CD4+ or CD8+ T cells in mice immunized with U-Omp16 or U-Omp19 plus IFA resulted in a loss of the elicited protection, indicating that both cell types are mediating immune protection. U-Omp16 or U-Omp19 vaccination induced a T helper 1 response, systemic protection in aluminum hydroxide formulation, and oral protection with cholera toxin adjuvant against B. abortus infection. Both immunization routes exhibited a similar degree of protection to attenuated Brucella vaccines (S19 and RB51, respectively). Overall these results indicate that U-Omp16 or U-Omp19 would be a useful candidate for a subunit vaccine against human and animal brucellosis