Chemiluminiscence immunodetection reagent kit for detecting salbutamol
A chemiluminescent immunoassay and detection kit technology, which is applied in the field of immunological detection, can solve the problems of prolonging the detection time, and achieve the effects of increasing sensitivity, reducing incubation time, and simple instruments
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Embodiment 1
[0050] 1) Preparation of each component of the kit
[0051] Preparation of salbutamol hapten: acidify salbutamol, react with sodium nitrite in a low-temperature environment without light at 4°C, and generate intermediates containing diazonium cations. The diazotized albuterol was used as a hapten for subsequent synthesis of immune antigens and coating antigens.
[0052] Synthesis of bovine serum albumin-salbutamol immune antigen: the immune antigen was obtained by coupling salbutamol and bovine serum albumin (BSA) by diazotization method.
[0053] Synthesis of human serum albumin-salbutamol-coated antigen: the immune antigen was obtained by coupling salbutamol and human serum albumin (HSA) by diazotization.
[0054] Preparation of albuterol-peroxidase-labeled antibody: inject the above-mentioned immune antigen into Balb / C mice, and make it produce antibody serum after several booster immunizations. Take out the splenocytes of the immunized mice, add them to the centrifuge tu...
Embodiment 2
[0082] The chemiluminescent immunoassay kit for detecting salbutamol includes the following components:
[0083] (1) 48-well opaque white ELISA plates (6 strips x 8 wells) are coated with salbutamol-mouse serum albumin cross-linked complex, and are vacuum-sealed with aluminum film.
[0084] (2) 5 bottles of albuterol standard solution, the concentrations are respectively:
[0085] 0μg / L, 0.04μg / L, 0.36μg / L, 3.24μg / L, 29.16μg / L
[0086] (3) Salbutamol-horseradish peroxidase labeled antibody solution.
[0087] (4) Luminescence substrate A solution (luminol and enhancer), and luminescence substrate B solution (urea hydrogen peroxide).
[0088] (5) 50 times concentrated buffer. Diluted 50 times before use to become a working concentration buffer, the diluted working concentration buffer is 0.05mol / L Tris-HCl buffer, pH6.9, containing 0.1% (v / v) Tween-20.
Embodiment 3
[0090] The chemiluminescent immunoassay kit for detecting salbutamol includes the following components:
[0091] (1) 96-well opaque white ELISA plate (12 strips x 8 wells) is coated with albuterol-egg albumin cross-linked complex and vacuum-sealed with aluminum film.
[0092] (2) 6 bottles of albuterol standard solution, the concentrations are respectively:
[0093] 0μg / L, 0.05μg / L, 0.25μg / L, 1.25μg / L, 6.25μg / L, 31.25μg / L.
[0094] (3) Salbutamol-horseradish peroxidase labeled antibody solution.
[0095] (4) Luminescence substrate A solution (luminol and enhancer), and luminescence substrate B solution (urea hydrogen peroxide).
[0096] (5) 10 times concentrated buffer. Diluted 10 times before use to become a working concentration buffer, the diluted working concentration buffer is 0.05mol / L glycine-HCl buffer, pH6.9, containing 0.02% (v / v) Tween-20.
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