Rapid detection method based on gold magnetic particle-labeled immunochromatography
A technology of gold magnetic particles and detection methods, which can be used in measurement devices, analytical materials, biological tests, etc., and can solve the problems of complicated operations, subjective differences, and narrow application fields.
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Embodiment 1
[0050] Application of gold magnetic particle-labeled rapid immunochromatographic test strips for early pregnancy detection based on the sandwich method (in the field of health testing)
[0051] 1. The β-antibody of human chorionic gonadotropin HCG is labeled with gold magnetic particles, and dissolved in the chromatography working solution:
[0052] 1.1) Take the gold magnetic particles, equilibrate for 3 times with pH=7, 0.01M phosphate buffer, add the β-antibody of human chorionic gonadotropin HCG at the ratio of 200 μg / mg gold magnetic particles, and then pH=7, 0.01M phosphate buffer solution balance treated gold magnetic particles, placed in 35 ℃, 180rpm constant temperature oscillator fully reacted for 30min;
[0053] 1.2) After the reaction is completed, separate on the magnetic separator for 3 minutes, discard the supernatant, and wash with pH=7, 0.01M phosphate buffer containing 0.5% Tween20 to remove protein molecules that are not bound to the surface of the gold magn...
Embodiment 2
[0065] Detection of cardiac troponin by using gold magnetic particle-labeled rapid immunochromatographic test strips based on the sandwich method (in the field of disease detection)
[0066] 1. Gold magnetic particle-labeled cardiac troponin monoclonal antibody, and dissolved in the chromatography working solution:
[0067] 1.1) Take 1 mg of gold magnetic particles, equilibrate 3 times with pH=7, 0.01M phosphate buffer, add 1 mg / ml cardiac troponin monoclonal antibody mAb2-19C7, 200 μg, into the gold magnetic particles, and place at 35°C , 180rpm constant temperature oscillator fully reacted for 30min;
[0068] 1.2) After the reaction is completed, separate on a magnetic separator for 3 minutes, suck off the supernatant, wash with pH=7, 0.01M phosphate buffer containing 0.5% Tween20, and remove unlabeled cardiac troponin antibody I molecules; repeat the above steps three times.
[0069] 1.3) Blocking: Add 1ml of blocking agent to the gold magnetic particles immobilized with ...
Embodiment 3
[0080] Detection of aflatoxin in food using gold magnetic particles based on competition method (food safety detection field)
[0081] 1. Anti-aflatoxin monoclonal antibody clone 3A7 is labeled with gold magnetic particles and dissolved in the chromatography working solution:
[0082] 1.1) Take 1 mg of gold magnetic particles, equilibrate 3 times with pH=7, 0.01M phosphate buffer, add 1 mg / ml anti-aflatoxin monoclonal antibody clone 3A7, 200 μg, into the gold magnetic particles, place at 35 Fully react in a constant temperature oscillator at 180 rpm for 30 minutes;
[0083] 1.2) After the reaction is completed, separate on a magnetic separator for 3 minutes, suck off the supernatant, wash with pH=7, 0.01M phosphate buffer containing 0.5% Tween20, and remove the unlabeled anti-aflatoxin monoclonal antibody clone 3A7 ;Repeat the above steps three times;
[0084] 1.3) Blocking: Add 1ml of blocking agent to the gold magnetic particles immobilized with cardiac troponin antibody I...
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