Canine parvovirus colloidal gold immunochromatography test strip and preparation method
A technology for immunochromatographic detection and canine parvovirus, which is applied in measurement devices, analytical materials, biological material analysis, etc., can solve problems such as limitations, and achieve the effects of simple operation, rapid detection, and high detection accuracy.
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Embodiment 1
[0027] The schematic diagram of the structure of the canine parvovirus colloidal gold immunochromatographic detection test strip is as follows figure 1 As shown, the horizontal plane of the test strip is sequentially from right to left the sample absorption area 1, the gold label probe area 2, the immobilized antibody area 3 and the water absorption area 4, which are laid on the bottom plate 5 and partially overlap each other; the sample absorption area 1, The materials of gold standard probe area 2, immobilized antibody area 3, water absorption area 4 and bottom plate 5 are glass fiber membrane, polyester membrane, nitrocellulose membrane, water absorption filter paper and polyethylene plate respectively. The gold-labeled probe area 2 is coated with colloidal gold-labeled anti-canine parvovirus monoclonal antibody F1, and the labeling amount is 4 μg / mL; the solid-phase antibody area 3 (from the gold-labeled probe area to the water-absorbing area) has Detection line 31 and con...
Embodiment 2
[0035] Except that the amount of anti-canine parvovirus monoclonal antibody B6 coated on detection line 31 was 1.5 μg / cm; the amount of goat anti-mouse IgG coated on control line 32 was 1.5 μg / cm; the colloid coated with gold standard probe area 2 The labeling amount of gold-labeled anti-canine parvovirus monoclonal antibody F1 is 4 μg / mL, and colloidal gold-labeled anti-canine parvovirus monoclonal antibody F1 method: take 20 mL of colloidal gold solution with a radius of 25 nm and anti-canine parvovirus monoclonal antibody F180 μg , under the condition of pH 9.0, it was combined by magnetic stirring and shaking, PEG-20000 was added as a stabilizer, and the final mass concentration of PEG-20000 was 20%, and the unbound anti-canine parvovirus monoclonal antibody F1 was removed by centrifugation And unstabilized colloidal gold particles and aggregates thereof, except for the colloidal gold-F1 complex, the dark red precipitate at the bottom of the centrifuge tube is the same as i...
Embodiment 3
[0037] Except that the amount of anti-canine parvovirus monoclonal antibody B6 coated on detection line 31 was 4.8 μg / cm; the amount of goat anti-mouse IgG coated on control line 32 was 4.8 μg / cm; the colloid coated with gold standard probe area 2 The labeling amount of gold-labeled anti-canine parvovirus monoclonal antibody F1 is 10 μg / mL, and colloidal gold-labeled anti-canine parvovirus monoclonal antibody F1 method: take 20 mL of colloidal gold solution with a radius of 40 nm and anti-canine parvovirus monoclonal antibody F1 200 μg , under the condition of pH 9.0, it was combined by magnetic stirring and shaking, PEG-20000 was added as a stabilizer, and the final mass concentration of PEG-20000 was 10%, and the unbound anti-canine parvovirus monoclonal antibody F1 was removed by centrifugation And unstabilized colloidal gold particles and aggregates thereof, except for the colloidal gold-F1 complex, the dark red precipitate at the bottom of the centrifuge tube is the same a...
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