ELISA is the common acronym for Enzyme-Linked-Immunosorbent Assay. It’s a quick plate based technique for detecting an antigen from a solution. This antigen could be a peptide, protein, antibody, or small molecule. In general, for an ELISA, an antigen is first immobilized on a surface (Step 1 below). Next, an antibody specific to the antigen is flowed over the surface (Step 2). This antibody, is also attached to a chemiluminescence-related enzyme. Treatment with the chemiluminescent substrate facilitates detection of the antibody and the antigen (Step 3). Take a look at these pictures to get an overview of the strategy:
Conjugated proteins may require different antibodies in ELISAs. However you can easily track the ELISA process by labeling your protein with a fluorescent probe.
There are a few different types of ELISA assays but they all follow the basic strategy outlined above. Essentially, one can choose how to immobilize the antigen on the surface and how the antigen is detected via the antibody.
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96 well polystyrene plate | |
Plate shaker | |
Pipettes | |
Coating buffer | 0.2 M sodium carbonate/bicarbonate buffer, pH 9.4 |
Wash buffer | 0.1 M phosphate, 0.15 M sodium chloride, pH 7.2 with 0.05% Tween 20 |
Blocking buffer | 2% w/v Bovine Serum Albumin in Wash Buffer |
Diluent buffer | 2% w/v BSA in Wash buffer or a more appropriate buffer such as cell culture media |
Stop buffer | 2 M Sulfuric Acid |
Capture Antibody Solution | 15 ug/ml antibody in coating buffer |
Detection Antibody Solution | 10 ug/ml in (20% Diluent buffer/80% Wash Buffer) |
Enzyme Conjugated Antibody Solution | 200 ng/ml in (20% Diluent buffer/80% Wash Buffer) |
HRP Substrate | TMB (3,3′,5,5′-tetramethylbenzidine). 1 mg/ml. Usually commercially available as a solution. |
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