First, let's take a brief look at IL-8: L-8 is a polypeptide with a molecular weight of 8-10 kD, which has chemotactic effects on neutrophils, T lymphocytes and eosinophils, and activates neutrophils, which is an important inflammation. medium. High levels of IL-8 can be detected in serum of severely infected patients and in local exudates of inflammation. In addition, recent studies have shown that IL-8 may be involved in the development of various tissue ischemia-reperfusion injury. We used two self-made monoclonal antibodies to establish a sandwich ELISA for the detection of IL-8 with a sensitivity of 156 Pg/ml. The method is simple and reproducible, and can be used for basic and clinical research of IL-8. Its principle: two strains of anti-IL-8 monoclonal antibodies recognizing different epitopes, one of which (4D7) is used as a coating antibody to recognize and bind IL-8 in the specimen to be tested, and the other strain as an enzyme label The antibody binds to another epitope that binds to the antibody-coated IL-8 and catalyzes the development of the substrate. Steps: 1. Coating: pH 9.5 carbonate slow solution diluted 4D7 monoclonal antibody crude gamma globulin to 1 μg / ml, added to a 96-well plate, 100 μl / well, placed at 4 ° C, 36 hours. 2. Blocking: 0.1% Tween PBS (Buffer A) was rinsed three times with 96-well plates, 3% BSA Buffer A (Buffer B) 200 μl/well, and placed at 37 ° C for 1 hour. 3. Add the sample to be tested: Buffer A. Rinse the 96-well plate three times, add 100 μl/well of the sample to be tested and Buffer B diluted, and put it at 37 ° C for 3 hours. 4. Add enzyme labeling antibody: Buffer A was rinsed five times in 96-well plate, 3% PEG Buffer A diluted enzyme-labeled antibody to 1:800, added to 96-well plate, 100 μl/well, and placed at 37 ° C for 1 hour. 5. Color development: Buffer A rinse 96-well plate five times, pH5.4 citrate buffer solution substrate (ABTS), 0.2mg/ml, add 3%H2O2, 2μl/ml, add 96-well plate, 100μ/well , develop color at room temperature or 37 ° C. Reagent equipment: 1. The kit provides coated antibody, enzyme-labeled antibody, standard, substrate (ABTS), 96-well elisa plate. 2. The coating buffer, PBS, and substrate buffer were prepared in the same manner as the conventional ELISA method. Precautions: 1. If the specimen to be tested is serum, a disposable container should be used, and serum should be separated as soon as possible after blood collection (within 6 hours). 2. The blocking solution or antibody dilution should be freshly prepared or frozen. Stainless Steel Hexagonal Bar,420 Stainless Steel Hexagonal Bar,Stainless Steel Bar Metal Rod,Stainless Steel Bar Top ShenZhen Haofa Metal Precision Parts Technology Co., Ltd. , https://www.haofametals.com
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