Instruction manual for rat major basic protein (MBP) ELISA kit
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Explanation
Experimental principle
Kit composition and reagent preparation
Reagents and equipment needed but not provided
Collection and preservation of specimens
Note: Hemolysis of specimens will affect the final test results, so hemolysis specimens should not be tested.
Dilution principle of specimens:
Standard dilution principle: 2 bottles, each bottle is diluted with sample diluent to 1ml before use, and then left to stand for more than 10 minutes after being capped, and then repeatedly inverted / rubbed to help dissolve. After serial dilution, dilute 800 ng / ml, 400 ng / ml, 200 ng / ml, 100 ng / ml, 50 ng / ml, 25 ng / ml, 12.5 ng / ml, and the sample dilution is directly used as the standard concentration 0 ng / ml, prepared within 15 minutes before use.
Dilution principle of biotinylated antibody:
Dilution principle of horseradish peroxidase-labeled avidin:
Steps
1. Add sample: set blank hole, standard hole and sample hole to be tested respectively. Add 100μl of sample diluent to blank wells, and add 100μl of standard or test sample to the remaining wells. Be careful not to have air bubbles. Add samples to the bottom of the wells of the microtiter plate. Try not to touch the well walls. The target plate is covered with a cover or film and reacted at 37 ° C for 120 minutes.
Note:
Plate washing method Manual plate washing method: suck (do not touch the wall) or shake off the liquid in the microplate; place a few layers of absorbent paper on the experimental table, and force the microplate down several times; pat the recommended wash buffer Inject at least 0.3ml of solution into the hole and soak for 1-2 minutes. Repeat this process several times as needed.
Automatic plate washing: If there is an automatic plate washing machine, it should be used in the formal experiment process after being used skillfully.
Calculation
Precautions
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