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- Dilute 5X Antibody Coating Buffer 1:5 with deionized water and mix for 15 minutes. As Antibody Coating Buffer is a 5X concentrate, crystalline precipitates may form in the bottle, especially when refrigerated. If this happens, gently warm the buffer until all crystals are dissolved. Do not let it boil.
- Dilute your antibody into the coating buffer. Optimal coating concentration varies significantly from 0.1 µg/mL to 10 µg/mL.
- Let the solution stir 10-15 minutes and pipette onto the plate. Optimal coating volume generally ranges between 50-200 µL per well. ICT recommends coating antibodies onto Costar 96-Well EIA/RIA Stripwell plate.
- Once added to the plate, incubate the coating solution from 8-24 hours at room temperature protected from light. Minimize evaporation by individually covering each plate with a plate sealing cover, wrapping a stack in plastic wrap, or placing plates in a humidified storage box and covering.
- Aspirate the coating solution.
- Wash each well twice with 1X ELISA Wash Buffer (catalog #652).
- Block the uncoated regions of the microplate wells by pipetting 300 μL of blocking buffer (such as catalog #640, 64, or 643) into each well.
- Incubate 8-24 hours at room temperature.
- Aspirate the blocking buffer.
- The assay can be run at this point, or the plate can be dried and packaged for later use.
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- Dry the plate by letting it sit on the bench top from 8-24 hours while protected from light, or dry in a drying chamber under vacuum from 3 – 6 hours at room temperature. When dry, seal the plate in an air-tight foil pouch with a desiccant packet and store at RT or 2-8°C protected from light.
Product Specific References
PMID | Publication |
39771980 | Hernández, J, et al. 2024. Dynamics of PCV2 and PCV3 in the Serum and Oral Fluids of Pigs After PCV2 Vaccination in a Commercial Farm. Vaccines, . |
28637884 | Heit, A., et al. 2017. Vaccination establishes clonal relatives of germinal center T cells in the blood of humans. The Journal of Experimental Medicine, 2139-2152. |
28716975 | Boraschi-Diaz, I., et al. 2017. Metabolic phenotype in the mouse model of osteogenesis imperfecta. Journal of Endocrinology, 279-289. |