ELISA Protocol

• 6 steps
• 6 hours
• 8 reagents required

The use of enzyme-linked immunosorbent assay, or ELISA, provides an economical, rapid and highly sensitive method for screening a large number of samples. ELISA can be used to detect and quantitate peptides, proteins, or antibodies. The assay is based upon an antigen-antibody interaction and subsequent enzymatic action on a substrate yielding a soluble colored product. Variations of the basic method exist for specialized applications. A basic method is outlined below.

Reagents Required

Procedure

Prepare antigen at 5.0 ug/mL in carbonate buffer. Load 200 µL per well. Cover plate to minimize evaporation. Allow antigen to bind at 4° C. The time required to bind antigens varies and may range from a few hours to overnight. Remove antigen. Wash 3 times with PBS.
Add 300 µL blocking solution per well. Allow blocking to occur at room temperature for 2 hours. Remove blocking solution and wash 3 times with PBS
Prepare serial dilutions of antibody to be titered in antibody diluent. Load 100 µL of diluted antibody per well. Allow the antibody to bind at room temperature for 1 hour. Remove antibody and wash 3 times with NP-40 solution.
Prepare enzyme-conjugated secondary antibody by dilution in antibody diluent. The optimum dilution may be lot-specific. Refer to back-cover inset for recommended dilution ranges. Load 100 µL of diluted enzyme-conjugated antibody per well. Allow the conjugate to bind at room temperature for 30 minutes. Remove conjugate and wash 3 times with NP-40 solution.
Add 100 µL of desired substrate solution per well. Allow color to develop at room temperature for 30 minutes.
Read absorbances on plate using microplate reader.