Chemiluminescence detection kit for Es (E-selectin) and preparation method of kit
A chemiluminescence detection and chemiluminescence technology, which is applied in chemiluminescence/bioluminescence, biological testing, and analysis through chemical reactions of materials, can solve problems such as complex reaction kinetics, unstable results, and many influencing factors. Achieve the effects of no reduction in photon yield, good reagent stability, and low background luminescence
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[0025] The invention provides a chemiluminescent detection kit for E-selectin and a preparation method thereof, a magnetic particle-coupled E-selectin (Es) capture antibody, and an acridinium ester-labeled E-selectin (Es) detection antibody. The kit also includes E-selectin calibrator, chemiluminescence pre-excitation solution A, chemiluminescence excitation solution B and cleaning solution.
[0026] Specifically, in the process of preparing the magnetic particle-coupled capture antibody in the present invention, the antibody-coupled buffer is a buffer with a pH value of 5.0-6.0 and a concentration of 20-200 mmol / L MES.
[0027] Specifically, in the process of preparing the magnetic particle-coupled capture antibody in the present invention, the blocking buffer is a buffer containing 1% BSA.
[0028] Specifically, in the process of preparing the acridinium ester-labeled detection antibody in the present invention, the buffer solution of the acridinium ester-labeled E-selectin ...
Embodiment 1
[0034] Example 1: The composition and preparation method of a chemiluminescent detection kit for E-selectin
[0035] 1. Assembly of the kit
[0036] Magnetic particle-coupled E-selectin monoclonal antibody;
[0037] E-selectin (Es) monoclonal antibody labeled with acridinium ester;
[0038] E-selectin series calibrator solution;
[0039] Chemiluminescence pre-excitation solution A and chemiluminescence excitation solution B;
[0040] Cleaning fluid.
[0041] 2. Preparation of Magnetic Microparticle Suspension Conjugated to E-selectin Monoclonal Antibody
[0042] (1) Take 1 mg of carboxyl magnetic particles in a 0.5 mL centrifuge tube, add 200 μL of MES buffer solution with a concentration of 0.1 mol / L, vortex and mix, place on a magnetic stand, and let it stand for 5 minutes to make the magnetic particles and liquid Separate, discard the supernatant, wash 3 times, then add 200 μL of MES (pH 6.0) buffer, and vortex.
[0043] (2) Add 15 μg E-selectin monoclonal antibody so t...
Embodiment 2
[0062] Embodiment 2: detection and result analysis with kit
[0063] (1) Add 50 μL of the sample to be tested into the cuvette, then add 150 μL of magnetic particle coupling suspension, shake and mix, and incubate at 37°C for 8 min.
[0064] (2) Separate and wash 3 times. Shake the washed reaction vessel sufficiently to disperse the magnetic particles. .
[0065] (3) Add 150 μL of acridinium ester marker into the cuvette, shake to mix, and incubate at 37°C for 7 min.
[0066] (4) Separate and wash 3 times. Shake the washed reaction vessel sufficiently to disperse the magnetic particles.
[0067] (5) Add 100 μL of chemiluminescence pre-excitation solution A, add 100 μL of chemiluminescence excitation solution B after 1 second, and measure its relative luminous intensity. The content of E-selectin in the sample is proportional to its relative luminous intensity.
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