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13817140470更新時(shí)間:2010-04-12 瀏覽次數(shù):3442
Immunoassays are a powerful technique for detecting and measuring antigens and antibodies. Immunoassays can be classified three ways based on the steps involved:
Many types of immunoassays can be used to detect and quantitate both antigens and antibodies, but there are differences in the avidity requirements for the antibodies, the signal strengths of the labels, and the amount of background for each of these types of assays. Antibody capture assays are the most appropriate for measuring the titer of the antisera you have generated.
In this type of ELISA (Enzyme-Linked Immunosorbant Assay), the antigen (peptide or protein) is bound to the polystyrene microtiter plate first. The antiserum containing the anti-peptide antibody is then added to the well and allowed to bind. Finally, a second antibody, specific for the first antibody and labeled for detection, is added to the well and allowed to bind. The second antibody usually has an enzyme conjugated to it. This enzyme catalyzes the formation of colored substance, e.g., p-nitrophenol, from a colorless substrate, p-nitrophenylphosphate (Figure 21). This colored substance is then quantified and the amount of antibody present can be calculated.
This procedure has two parts. Part 1 applies to any detection protocol. Part 2 describes two different detection methods. To measure an antibody titer, decide on the detection method first, then complete both Parts 1 and 2.
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Figure 21. Antibody detection in an Enzyme- Linked Immunosorbant Assay (ELISA) |
Part 1: Antigen and Antibody
Equipment Needed
Solutions to Prepare for the ELISA Procedure
ELISA Procedure
Run duplicates or triplicates of each of antiserum dilution. The ELISA template in Table 3 can be used to track the experiments.
Table 3. ELISA Template
1 | 2 | 3 | 4 | 5 | 6 | 7 | 8 | 9 | 10 | 11 | 12 | |
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Table 4. Serial Dilution Schedule | ||
Antiserum |
BSA/PBS-T (µL) |
Dilution (µL) |
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The next step (Part 2) is detection of the amount of antibodies bound to the plate. You can choose either of the procedures described.
Notes on ELISA Procedures
Detection Using Alkaline Phosphatase
Reagents for Alkaline Phosphatase Detection
For example, if the antibodies were raised in a rabbit, use goat anti-rabbit IgG whole molecule/alkaline phosphatase conjugate
Procedure for Alkaline Phosphatase Detection
Detection Using Horseradish Peroxidase
Reagents for Horseradish Peroxidase Detection
Procedure for Horseradish Peroxidase Detection
How to Calculate the Antibody Titer of the Sera
An example of a graph used to determine the titer of an antibody is shown in Figure 22.
The titer was estimated to be 1 in 2400.
Figure 22. Antibody titer graph (X = dilution corresponding to Ab titer) |
Further Methods for Evaluating Anti-peptide Antibodies
If the antibodies are to be used as a reagent to study a specific protein, it is important to learn whether they recognize the native protein. This can be done using the above ELISA procedure. Use the protein in place of the peptide or peptide conjugate. Additional information about the binding strength of the antibodies can be obtained by a competitive assay using the synthetic peptide in conjunction with the native protein. For further details, see Van Regenmor .
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