Development of an optical immunosensor based on the fluorescence of Cyanine-5 for veterinarian diagnostics

Development of an optical immunosensor based on the fluorescence of Cyanine-5 for veterinarian diagnostics

A model optical immunosensor was developed to quantify an antibody present in a sample by measuring the fluorescence of Cyanine-5 conjugated with the antibody, using a competitive and a sandwich immunoreaction configuration, with the antigen immobilised in controlled pore glass beads. At pH 2, 94% o...

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Veröffentlicht in:Biotechnology letters 2004-06, Vol.26 (12), p.993-997
Hauptverfasser: Silva, M, Cruz, H, Rossetti, O, Arese, A, Oliva, A
Format: Artikel
Sprache:eng
Schlagworte:
animal pathogenic bacteria
Animals
Antibodies
antibody detection
Biological and medical sciences
Biosensing Techniques - instrumentation
Biosensing Techniques - methods
Biosensing Techniques - veterinary
Biosensors
Biotechnology
Brucella
Brucella - immunology
Brucella - isolation & purification
Brucellosis, Bovine - blood
Brucellosis, Bovine - diagnosis
Brucellosis, Bovine - microbiology
Carbocyanines
Cattle
Diagnostic agents
diagnostic techniques
Diagnostics
Equipment Design
Equipment Failure Analysis
Fluorescence
Fluorescent Dyes
Fluoroimmunoassay - instrumentation
Fluoroimmunoassay - methods
Fluoroimmunoassay - veterinary
Fundamental and applied biological sciences. Psychology
Glass beads
Immunology
infection
Membrane Proteins - immunology
Microchemistry - instrumentation
Microchemistry - methods
optical immunosensors
Optical properties
Optics
Optics and Photonics - instrumentation
pH effects
Photobleaching
Q1
Q2
Reproducibility of Results
Sensitivity and Specificity
Sensors
Sheep
Spectrometry, Fluorescence - instrumentation
Spectrometry, Fluorescence - methods
Spectrometry, Fluorescence - veterinary
Stains
Veterinarians
Veterinary medicine
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Zusammenfassung:A model optical immunosensor was developed to quantify an antibody present in a sample by measuring the fluorescence of Cyanine-5 conjugated with the antibody, using a competitive and a sandwich immunoreaction configuration, with the antigen immobilised in controlled pore glass beads. At pH 2, 94% of the antigen-antibody complex was dissociated, allowing reutilisation. Photobleaching had no effect on the fluorescence. This model system was used to detect Brucella sp. infection and could quantify anti-Brucella sp. antibodies in ovine serum samples in the range from 0.005 to 0.11 mg ml-1.
ISSN:0141-5492
1573-6776
DOI:10.1023/B:BILE.0000030046.96039.e8