For reference only. Please follow the manual included in your kit for instructions.
For the quantitative detection of Ochratoxin A (OTA) concentration in cereal and feed samples.
This kit uses Competitive-ELISA as the method for the quantitative detection. It can detect Ochratoxin A (OTA) in samples, such as cereals, feed, etc. This kit is composed of ELISA Microtiter plate, HRP conjugate, antibody working solution, standard and other supplementary reagents. The microtiter plate provided in this kit has been pre-coated with coupled antigen. During the reaction, OTA in the samples or standard competes with coupled antigen on the solid phase supporter for sites of anti-OTA antibody. Then Horseradish Peroxidase (HRP) conjugate is added to each microtiter plate well, and substrate reagent is added for color development. There is a negative correlation between the OD value of samples and the concentration of OTA. The concentration of OTA in the samples can be calculated by comparing the OD of the samples to the standard curve.
Reagent | Quantity |
---|---|
ELISA Microtiter plate | 96 wells |
Standard Liquid | 1 mL each (ppb=ng/mL=ng/g) (0 ppb, 1 ppb, 3 ppb, 9 ppb, 27 ppb, 81 ppb) |
HRP Conjugate | 11 mL |
Antibody Working Solution | 5.5 mL |
Substrate Reagent A | 6 mL |
Substrate Reagent B | 6 mL |
Stop Solution | 6 mL |
20×Concentrated Wash Buffer | 40 mL |
Plate Sealer | 3 |
Sealed Bag | 1 |
Manual | 1 |
All reagent bottle caps should be tightly closed to prevent evaporation and microbial contamination.
Bring all reagents and samples to room temperature (25℃) before use. All reagents should be mixed thoroughly by gently swirling before pipetting. Avoid foaming. Any unused Microtiter plate wells should be resealed as soon as possible and stored at 2-8℃.
Absorbance (%) = A/A₀×100%