An immunoproteomic approach revealed antigenic proteins enhancing serodiagnosis performance of bird fancier's lung

Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were...

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Published in:	Journal of immunological methods Vol. 450; pp. 58 - 65
Main Authors:	Rouzet, Adeline, Reboux, Gabriel, Dalphin, Jean-Charles, Gondouin, Anne, De Vuyst, Paul, Balliau, Thierry, Millon, Laurence, Valot, Benoit, Roussel, Sandrine
Format:	Journal Article
Language:	English
Published:	Netherlands Elsevier B.V 01.11.2017 Elsevier
Subjects:	2D electrophoresis Adult Aged Aged, 80 and over Allergens - immunology Animals Area Under Curve Avian Proteins - immunology Biochemistry, Molecular Biology biomarkers Bird fancier's lung Bird Fancier's Lung - blood Bird Fancier's Lung - diagnosis Bird Fancier's Lung - immunology Birds - immunology breathing Case-Control Studies Chromatography, Liquid Ecology, environment Electrophoresis, Agar Gel Electrophoresis, Gel, Two-Dimensional ELISA Endopeptidases - immunology Enzyme Precursors - immunology Enzyme-Linked Immunosorbent Assay Escherichia coli Feces Female Genomics Health Human health and pathology Humans hypersensitivity Hypersensitivity pneumonitis immune system immunoblotting Immunoelectrophoresis Immunoglobulin Light Chains, Surrogate - immunology immunoglobulins Inhalation Exposure Life Sciences Male Middle Aged patients pigeons pneumonia Predictive Value of Tests proteomics Proteomics - methods Pulmonology and respiratory tract Recombinant antigens recombinant proteins Reproducibility of Results ROC Curve Serodiagnosis Serologic Tests Tandem Mass Spectrometry DD HVs Hypersensitivity pneumonitis Recombinant antigens HP BFL AECs 2-DE PDE LC-MS/MS Bird fancier's lung IEP IGLL1 Serodiagnosis 2D electrophoresis ProE ELISA
ISSN:	0022-1759, 1872-7905, 1872-7905
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Abstract	Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were (i) to identify antigenic proteins from pigeon droppings (ii) to provide information about their location in avian matrices and (iii) to produce them in recombinant proteins to evaluate their diagnostic performances. Antigenic proteins of pigeon dropping extracts were investigated using 2-dimensional immunoblotting with sera from patients with BFL, asymptomatic exposed controls and healthy volunteers. We investigated the origin of these antigenic proteins by analyzing droppings, blooms and sera using a shotgun proteomic analysis. BFL-associated proteins were produced as recombinant antigens in E. coli and were assessed in ELISA with sera from patients (n=25) and subject exposed controls (n=30). These diagnostic performances were compared with those obtained by precipitin techniques (agar gel double diffusion, immunoelectrophoresis). We identified 14 antigenic proteins mainly located in droppings and blooms. These proteins were involved in either the digestive or immune systems of pigeons. Using the recombinant BFL-associated proteins: Immunoglobulin lambda-like polypeptide-1 (IGLL1: sensitivity: 76%; specificity: 100%; AUC: 0.93) and Proproteinase E (ProE: sensitivity: 84%; specificity: 80%; AUC: 0.85), the ELISA test showed better performance than precipitin assays with pigeon dropping extracts (sensitivity: 60%; specificity: 93.3%; AUC: 0.76). IGLL1 and ProE were identified as the biomarkers of the disease. The use of these highly standardized antigens discriminates BFL cases from exposed subjects in serological assays. The results of this study offer new possibilities for the serological diagnosis of the disease. Clinical trial registration: ClinicalTrials.gov: Identifier NCT03056404. •Droppings and blooms contain 14 antigenic proteins.•These proteins are involved in either the digestive or immune systems of pigeons.•ELISA tests with recombinant IGLL1 and ProE improve and standardize serological diagnosis of BFL.
AbstractList	Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were (i) to identify antigenic proteins from pigeon droppings (ii) to provide information about their location in avian matrices and (iii) to produce them in recombinant proteins to evaluate their diagnostic performances. Antigenic proteins of pigeon dropping extracts were investigated using 2-dimensional immunoblotting with sera from patients with BFL, asymptomatic exposed controls and healthy volunteers. We investigated the origin of these antigenic proteins by analyzing droppings, blooms and sera using a shotgun proteomic analysis. BFL-associated proteins were produced as recombinant antigens in E. coli and were assessed in ELISA with sera from patients (n=25) and subject exposed controls (n=30). These diagnostic performances were compared with those obtained by precipitin techniques (agar gel double diffusion, immunoelectrophoresis). We identified 14 antigenic proteins mainly located in droppings and blooms. These proteins were involved in either the digestive or immune systems of pigeons. Using the recombinant BFL-associated proteins: Immunoglobulin lambda-like polypeptide-1 (IGLL1: sensitivity: 76%; specificity: 100%; AUC: 0.93) and Proproteinase E (ProE: sensitivity: 84%; specificity: 80%; AUC: 0.85), the ELISA test showed better performance than precipitin assays with pigeon dropping extracts (sensitivity: 60%; specificity: 93.3%; AUC: 0.76). IGLL1 and ProE were identified as the biomarkers of the disease. The use of these highly standardized antigens discriminates BFL cases from exposed subjects in serological assays. The results of this study offer new possibilities for the serological diagnosis of the disease. Clinical trial registration: ClinicalTrials.gov: Identifier NCT03056404. •Droppings and blooms contain 14 antigenic proteins.•These proteins are involved in either the digestive or immune systems of pigeons.•ELISA tests with recombinant IGLL1 and ProE improve and standardize serological diagnosis of BFL. Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were (i) to identify antigenic proteins from pigeon droppings (ii) to provide information about their location in avian matrices and (iii) to produce them in recombinant proteins to evaluate their diagnostic performances. Antigenic proteins of pigeon dropping extracts were investigated using 2-dimensional immunoblotting with sera from patients with BFL, asymptomatic exposed controls and healthy volunteers. We investigated the origin of these antigenic proteins by analyzing droppings, blooms and sera using a shotgun proteomic analysis. BFL-associated proteins were produced as recombinant antigens in E. coli and were assessed in ELISA with sera from patients (n=25) and subject exposed controls (n=30). These diagnostic performances were compared with those obtained by precipitin techniques (agar gel double diffusion, immunoelectrophoresis). We identified 14 antigenic proteins mainly located in droppings and blooms. These proteins were involved in either the digestive or immune systems of pigeons. Using the recombinant BFL-associated proteins: Immunoglobulin lambda-like polypeptide-1 (IGLL1: sensitivity: 76%; specificity: 100%; AUC: 0.93) and Proproteinase E (ProE: sensitivity: 84%; specificity: 80%; AUC: 0.85), the ELISA test showed better performance than precipitin assays with pigeon dropping extracts (sensitivity: 60%; specificity: 93.3%; AUC: 0.76). IGLL1 and ProE were identified as the biomarkers of the disease. The use of these highly standardized antigens discriminates BFL cases from exposed subjects in serological assays. The results of this study offer new possibilities for the serological diagnosis of the disease. ClinicalTrials.gov: Identifier NCT03056404. Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were (i) to identify antigenic proteins from pigeon droppings (ii) to provide information about their location in avian matrices and (iii) to produce them in recombinant proteins to evaluate their diagnostic performances.Antigenic proteins of pigeon dropping extracts were investigated using 2-dimensional immunoblotting with sera from patients with BFL, asymptomatic exposed controls and healthy volunteers. We investigated the origin of these antigenic proteins by analyzing droppings, blooms and sera using a shotgun proteomic analysis. BFL-associated proteins were produced as recombinant antigens in E. coli and were assessed in ELISA with sera from patients (n=25) and subject exposed controls (n=30). These diagnostic performances were compared with those obtained by precipitin techniques (agar gel double diffusion, immunoelectrophoresis).We identified 14 antigenic proteins mainly located in droppings and blooms. These proteins were involved in either the digestive or immune systems of pigeons.Using the recombinant BFL-associated proteins: Immunoglobulin lambda-like polypeptide-1 (IGLL1: sensitivity: 76%; specificity: 100%; AUC: 0.93) and Proproteinase E (ProE: sensitivity: 84%; specificity: 80%; AUC: 0.85), the ELISA test showed better performance than precipitin assays with pigeon dropping extracts (sensitivity: 60%; specificity: 93.3%; AUC: 0.76).IGLL1 and ProE were identified as the biomarkers of the disease. The use of these highly standardized antigens discriminates BFL cases from exposed subjects in serological assays. The results of this study offer new possibilities for the serological diagnosis of the disease.Clinical trial registration: ClinicalTrials.gov: Identifier NCT03056404. Background: Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common fonn of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were (i) to identify antigenic proteins from pigeon droppings (ii) to provide information about their location in avian matrices and (iii) to produce them in recombinant proteins to evaluate their diagnostic performances. Method: Antigenic proteins of pigeon dropping extracts were investigated using 2-dimensional immunoblotting with sera from patients with BFL, asymptomatic exposed controls and healthy volunteers. We investigated the origin of these antigenic proteins by analyzing droppings, blooms and sera using a shotgun proteomic analysis. BFL-associated proteins were produced as recombinant antigens in E. coli and were assessed in ELISA with sera from patients (n = 25) and subject exposed controls (n = 30). These diagnostic performances were compared with those obtained by precipitin techniques (agar gel double diffusion, immunoelectrophoresis). Results: We identified 14 antigenic proteins mainly located in droppings and blooms. These proteins were involved in either the digestive or immune systems of pigeons. Using the recombinant BFL-associated proteins: Immunoglobulin lambda-like polypeptide-1 (IGLL1: sensitivity: 76%; specificity: 100%; AUC: 0.93) and Proproteinase E (ProE: sensitivity: 84%; specificity: 80%; AUC: 0.85), the ELISA test showed better performance than precipitin assays with pigeon dropping extracts (sensitivity: 60%; specificity: 93.3%; AUC: 0.76). Conclusion: IGLL1 and ProE were identified as the biomarkers of the disease. The use of these highly standardized antigens discriminates BFL cases from exposed subjects in serological assays. The results of this study offer new possibilities for the serological diagnosis of the disease. Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were (i) to identify antigenic proteins from pigeon droppings (ii) to provide information about their location in avian matrices and (iii) to produce them in recombinant proteins to evaluate their diagnostic performances.BACKGROUNDBird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact identification of proteins involved is unknown, and serological test use for diagnosis need to be standardized. The objectives of this study were (i) to identify antigenic proteins from pigeon droppings (ii) to provide information about their location in avian matrices and (iii) to produce them in recombinant proteins to evaluate their diagnostic performances.Antigenic proteins of pigeon dropping extracts were investigated using 2-dimensional immunoblotting with sera from patients with BFL, asymptomatic exposed controls and healthy volunteers. We investigated the origin of these antigenic proteins by analyzing droppings, blooms and sera using a shotgun proteomic analysis. BFL-associated proteins were produced as recombinant antigens in E. coli and were assessed in ELISA with sera from patients (n=25) and subject exposed controls (n=30). These diagnostic performances were compared with those obtained by precipitin techniques (agar gel double diffusion, immunoelectrophoresis).METHODAntigenic proteins of pigeon dropping extracts were investigated using 2-dimensional immunoblotting with sera from patients with BFL, asymptomatic exposed controls and healthy volunteers. We investigated the origin of these antigenic proteins by analyzing droppings, blooms and sera using a shotgun proteomic analysis. BFL-associated proteins were produced as recombinant antigens in E. coli and were assessed in ELISA with sera from patients (n=25) and subject exposed controls (n=30). These diagnostic performances were compared with those obtained by precipitin techniques (agar gel double diffusion, immunoelectrophoresis).We identified 14 antigenic proteins mainly located in droppings and blooms. These proteins were involved in either the digestive or immune systems of pigeons. Using the recombinant BFL-associated proteins: Immunoglobulin lambda-like polypeptide-1 (IGLL1: sensitivity: 76%; specificity: 100%; AUC: 0.93) and Proproteinase E (ProE: sensitivity: 84%; specificity: 80%; AUC: 0.85), the ELISA test showed better performance than precipitin assays with pigeon dropping extracts (sensitivity: 60%; specificity: 93.3%; AUC: 0.76).RESULTSWe identified 14 antigenic proteins mainly located in droppings and blooms. These proteins were involved in either the digestive or immune systems of pigeons. Using the recombinant BFL-associated proteins: Immunoglobulin lambda-like polypeptide-1 (IGLL1: sensitivity: 76%; specificity: 100%; AUC: 0.93) and Proproteinase E (ProE: sensitivity: 84%; specificity: 80%; AUC: 0.85), the ELISA test showed better performance than precipitin assays with pigeon dropping extracts (sensitivity: 60%; specificity: 93.3%; AUC: 0.76).IGLL1 and ProE were identified as the biomarkers of the disease. The use of these highly standardized antigens discriminates BFL cases from exposed subjects in serological assays. The results of this study offer new possibilities for the serological diagnosis of the disease.CONCLUSIONIGLL1 and ProE were identified as the biomarkers of the disease. The use of these highly standardized antigens discriminates BFL cases from exposed subjects in serological assays. The results of this study offer new possibilities for the serological diagnosis of the disease.ClinicalTrials.gov: Identifier NCT03056404.CLINICAL TRIAL REGISTRATIONClinicalTrials.gov: Identifier NCT03056404.
Author	Dalphin, Jean-Charles Reboux, Gabriel Rouzet, Adeline Roussel, Sandrine Balliau, Thierry Gondouin, Anne De Vuyst, Paul Millon, Laurence Valot, Benoit
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Keywords	DD HVs Hypersensitivity pneumonitis Recombinant antigens HP BFL AECs 2-DE PDE LC-MS/MS Bird fancier's lung IEP IGLL1 Serodiagnosis 2D electrophoresis ProE ELISA
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Snippet	Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common form of hypersensitivity pneumonitis. However, the exact... Background: Bird fancier's lung (BFL) caused by repeated inhalation of avian proteins is the most common fonn of hypersensitivity pneumonitis. However, the...
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SubjectTerms	2D electrophoresis Adult Aged Aged, 80 and over Allergens - immunology Animals Area Under Curve Avian Proteins - immunology Biochemistry, Molecular Biology biomarkers Bird fancier's lung Bird Fancier's Lung - blood Bird Fancier's Lung - diagnosis Bird Fancier's Lung - immunology Birds - immunology breathing Case-Control Studies Chromatography, Liquid Ecology, environment Electrophoresis, Agar Gel Electrophoresis, Gel, Two-Dimensional ELISA Endopeptidases - immunology Enzyme Precursors - immunology Enzyme-Linked Immunosorbent Assay Escherichia coli Feces Female Genomics Health Human health and pathology Humans hypersensitivity Hypersensitivity pneumonitis immune system immunoblotting Immunoelectrophoresis Immunoglobulin Light Chains, Surrogate - immunology immunoglobulins Inhalation Exposure Life Sciences Male Middle Aged patients pigeons pneumonia Predictive Value of Tests proteomics Proteomics - methods Pulmonology and respiratory tract Recombinant antigens recombinant proteins Reproducibility of Results ROC Curve Serodiagnosis Serologic Tests Tandem Mass Spectrometry
Title	An immunoproteomic approach revealed antigenic proteins enhancing serodiagnosis performance of bird fancier's lung
URI	https://dx.doi.org/10.1016/j.jim.2017.07.012 https://www.ncbi.nlm.nih.gov/pubmed/28760669 https://www.proquest.com/docview/1925273729 https://www.proquest.com/docview/2010208281 https://hal.science/hal-01664277
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