Components
1.Vial 1 (yellow top):Anti-IgG capture antibody (1.2 ml);Concentration: 0.5 mg/ml.
2.Vial 2 (green top):Anti-IgG biotinylated detection antibody (100 ul);Concentration: 0.5 mg/ ml.
3.Vial 3 (white top):Streptavidin Alkaline Phosphatase (500 ul).
4.Vial 4 (black top):Polyclonal activator: R848 (100 μl), Concentration: 1 mg/ml.
5.Vial 5 (blue top):Lyophilised recombinant human IL-2(1 ug).
6.Antibodies are supplied in sterile filtered (0.2 um)PBS with 0.02% sodium azide.Strepta-vidin-ALP is supplied in 0.1 M Tris buffer with 0.002% Kathon CG.R848 is supplied insterile filtered (0.2 um)PBS containing 1% DMSO.Vials have been overfilled to ensurerecovery of the specified amount.
Assay Procedure
1.Dilute the coating antibodies (anti-IgG) to 15 ug/ml in sterile PBS, pH 7.4.
2.Remove the ELISpot plate from the package and if using a PVDF plate, pre-wet the membrane by adding ethanol.
3.Wash plate 5 times with sterile water, 200 ul/well.
4.Add 100 ul/well of the antibody solution and incubate overnight at 48°C.
5.Remove excess antibody and wash plate 5 times with sterile PBS, 200 ul/well.
6.Add 200 ul/well of medium containing 10% of the same serum as used for the cell suspensions Incubate for at least 30 minutes at room temperature.
7.Remove the medium and add the stimuli followed by the cell suspension. Alternatively cells and stimuli can be mixed before addition to the plate.
8.Put the plate in a 37°C humidified incubator with 5% CO, and incubate for 18-48 hours.
9.Remove the cells by emptying the plate and wash 5 times with PBS, 200 ul/well.
10.Dilute the detection antibody(anti-IgG-biotin) to 0.05 ug/ml in PBS containing 0.5% fetal calfserum(PBS-O.5%FCS).Add 100 ul/well and incubate for 2 hours at room temperature.
11.Wash plate as above (step C1).
12.Dilute the Streptavidin-ALP(1:1000) in PBS-0.5% FCS and add 100 ul/well. Incubate for 1 hour at room temperature.
13.Wash plate as above (step C1).
14.Filter the ready-to-use substrate solution(BCIP/NBT-plus) through a 0.45 um filter and add100 ul/well. Develop until distinct spots emerge.
15.Stop color development by washing extensively in tap water. If desirable, remove the underd-rain (the soft plastic under the plate) and rinse the underside of the membrane.
16.Leave the plate to dry.Inspect and count spots in an ELISpot reader or in a dissection micro-scope.
17. Store plate in the dark at room temperature.
Format
Capture Ab (anti-IgG),Biotinylated detection Ab (anti-IgG),Streptavidin-ALP,R848,Recombinant mouse IL-2
Precaution of Use
We recommend the use of PVDF-based membrane plates. Maximal antibody binding capacity of these platesis obtained by a brief treatment with ethanol.
Handling Advice
PBS for washing and dilution should be filtered (0.3 um) for optimal results.Although possible to use, we donot recommend the inclusion of Tween or other detergents in the washing and incubation buffers.
Storage Comment
Plates should be kept at room temperature.
Expiry Date
The expiry date indicates how long unopened products, stored according to instructions, are recommended for use.
Note
The serum should be selected to support cell culture and give low background staining. We recom-mend the use of fetal calf serum. Alternatively serum-free medium evaluated for cell culture can beused.
Restrictions
For Research Use Only. Not for use in diagnostic procedures.
Datasheet