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Immunomagnetic protein isolation using Dynabeads® Protein A provides a fast and reliable method for capturing Ig for small scale purification or downstream immunoprecipitation. Ig can be isolated directly from ascites, serum, tissue culture supernatants or other samples.
An Ig-containing sample is added to a tube containing pre-washed Dynabeads® Protein A. During a short incubation, the immunoglobulins will bind to Dynabeads® Protein A via their Fc part. Place the test tube on a magnet (Dynal® MPC™) to collect the Dynabeads® Protein A - Ig complex at the tube wall, and discard the supernatant.
The purified and concentrated Ig can be eluted off in a small volume for downstream use such as antibody labelling or epitope mapping. The Dynabeads® Protein A - Ig complex can also be used directly to immunoprecipitate a target antigen, or for immunodepletion (see References). Add the Dynabeads® Protein A - Ig complex directly to a sample (cell lysate or other) containing your target antigen and incubate for antibody-antigen complex formation. Place the test tube on a magnet to collect the complex at the tube wall, and discard the supernatant. Resuspend the beads in a small volume for further use, or elute off your target protein directly e.g. in an acidic buffer or boil in a small volume of SDS-PAGE application buffer. If your downstream application involves purification of your target protein, you might want to cross-link the Ig to the protein A on the Dynabeads® before immunoprecipitation to prevent co-elution of the Ig. This is not necessary for downstream SDS-PAGE followed by autoradiography or Western blotting, and optional for Silver or Coomassie staining.
Dynabeads® Protein A are uniform, magnetizable polystyrene beads covalently coupled with recombinant
protein A. Typical characteristics for any given lot of this product:
Protein A
Protein A has a high specificity for immunoglobulins (Table 1) and is therefore suitable for the one-step capture of Ig (1). The native bacterial cell wall protein is a single polypeptide chain of 42 kDa with four Ig Fc binding sites, two of which are active (2). The protein A employed in this product is a 45 kDa recombinant protein containing all four binding sites for the Fc region of Ig, but without any albumin binding sites.
Ig origin | Protein A |
Human IgG1,2,4
|
Strong
|
Human IgD
|
No binding
|
Human IgG3,A,E,M
|
Weak
|
Mouse IgG1
|
Weak
|
Mouse IgG2a,2b, 3
|
Strong
|
Mouse IgM
|
Weak
|
Rat IgG1
|
Weak
|
Rat IgG2a
|
No binding
|
Rat IgG2b
|
No binding
|
Rat IgG2c
|
Strong
|
Bovine IgG1
|
Weak
|
Bovine IgG2
|
Strong
|
Chicken IgY
|
No binding
|
Dog IgG
|
Strong
|
Goat IgG1
|
Weak
|
Goat IgG2
|
Strong
|
Guinea pig IgG
|
Strong
|
Hamster
|
Weak
|
Horse IgG
|
Weak
|
Monkey IgG
|
Strong
|
Porcine IgG
|
Strong
|
Rabbit IgG
|
Strong
|
Sheep IgG1
|
Weak
|
Sheep IgG2
|
Strong
|
Table 1: Binding strength of protein A to different species of immunoglobulins (Ig) and their subclasses. Monoclonal antibodies will vary in their affinity towards protein A.
Binding Capacity
Binding of Ig to protein A in solution is an equilibrium reaction. In order to capture as many Ig as possible, it is important to keep the reaction volume low to maintain high concentrations of beads and Ig. There is no need to pre-treat or dilute the sample (even viscous samples). For both the immobilization of Ig and downstream immunoprecipitation procedures, it is recommended to keep the concentration of beads in the sample close to its original concentration in the Dynabeads® Protein A vial. The binding efficiency will decrease if the Dynabeads® are suspended in more than 5 times the original volume of Dynabeads® initially added. The amount of Ig captured is dependent on the concentration of Ig in the starting sample. 100 µl Dynabeads® Protein A will isolate approximately 25-30 µg human IgG from a sample containing 20-200 µg IgG/ml. A higher volume of Dynabeads® is recommended to avoid waste of Ig when working with concentrated samples or the Ig is precious. Keep all other parameters fixed as described below. Maximum amount of Ig-binding is obtained after 10 minutes
Dynabeads® Protein A should be washed prior to use. Washed Dynabeads® Protein A are resuspended in a basic phosphate buffer (e.g. pH 8.1) to facilitate binding of Ig to beads. The pH in the sample containing Ig might be adjusted for the same reason using a basic 5 x stock solution. The procedure described below is for the isolation of approximately 25 µg IgG from 10 µl human serum (or similar sample). The use of polypropylene tubes is recommended for washing and Ig capture.
Washing Procedure
The washing procedure is facilitated by the use of a magnet (Dynal® MPC).
Ig Capture Procedure
In this example, the Dynabeads® volume is much larger than the sample volume. In cases where the sample volume is as large as 1/4 the Dynabeads® volume, add 0.5 M Na-phosphate 5 x stock solution to raise the pH in the sample to 8 (with a final molarity of 0.1) before adding to the Dynabeads® (i.e. ad 10 µl stock solution to each 40 µl sample). Dynabeads® are resuspended in an adjusted volume so that sample and Dynabeads® volumes together is the same as the bead-volume originally pipetted from the vial.
Ig Elution Procedure
Eluting Ig off the Dynabeads® Protein A is, in this example, performed by lowering pH using 0.1 M citrate (pH 2-3) as the elution buffer. The degree of acidity needed depends on the species and Ig sub-class, but at pH 3 most Ig will be eluted.
Immunoprecipitation
When isolating antigens for SDS-PAGE followed by Western blotting or autoradiography the presence of Ig will not disturb your detection system. For other applications (e.g. protein purification, amino acid sequencing or when the Dynabeads® Protein A with bound Ig is to be reused) co-elution of the Ig is not desired. To prevent this, the captured Ig can be crosslinked to the protein A on the Dynabeads®. Cross-linking is also necessary if the Dynabeads® - Ig complex is reused for immunoprecipitation.
Crosslinking
The protocol presented below is an example using one of several commercially available cross-linkers.
Binding of Antigen
Trace amounts of Ig not cross-linked to Dynabeads® Protein A can be removed prior to binding by following the elution procedure described in 2.3 above. Binding of protein or other antigen to the Dynabeads® - Ig complex is dependent on the concentration of the Dynabeads®, antigen concentration, the affinity of the immobilized Ig and incubation time. Binding is performed at 2-8°C from 10 minutes to 1 hour. Equilibrium antibody-antigen is reached at approximately 1 hour.
Target Protein Elution Procedure
Conventional elution methods can be applied for the elution of target antigen from the Dynabeads® -Ig complex. Low pH (2-3), change in ionic strength, affinity elution, electrophoresis, polarity reducing agents, deforming eluents can be applied, or even boiling the beads in SDS-PAGE application buffer for direct characterization of protein on SDS-PAGE. The method of choice depends on the Ig’s affinity for the antigen, stability of target protein and downstream applications and detection methods. Most antigens will be eluted at pH 3 following the procedure described under 2.3 above. If the Dynabeads® - Ig complex is to be reused, mild elution methods should be employed. To prevent aggregation of the beads with immobilized Ig, 0.01-0.1% Tween-20 can be added to the storage buffer.
Re-use of Dynabeads® Protein A
For re-use after elution, the Dynabeads® Protein A should be brought to neutral pH using a Na-phosphate buffer, pH 7.
Additional Material Required