INSTRUCTION FOR USE

All operations are carried out at room temperature and gravity flow rate.

1. Equilibrate the column bIgG-AFF (Bovine IgG Activated Binding Gel) with 4 ml of Bovine IgG Binding & Coupling Buffer (bIgG-BCB).
2. Make up the sample with the purified bIgG (maximum 5 mg for monoclonal and 10 mg for polyclonal IgG) dissolved in the Bovine IgG Binding and Coupling Buffer (bIgG-BCB), at a concentration of 1-2 mg/ml.
3. - Apply the sample prepared in point 2. into the column prepared in point 1. at a flow rate of approx. 20 ml/cm²/hour.
   - Reload the flow through into the column at the same flow rate.
   - Repeat the same once more.
4. Wash the column with 20 ml of Bovine IgG Binding & Coupling Buffer (bIgG-BCB)
5. Load into the column 15 ml of Bovine IgG Saturation Reagent (Code : bIgG-SR) at a flow rate of approx. 20 ml/cm²/hour.
6. Wash the column with
   - 20 ml of Immuno Acid Washing Buffer (Code : IAf-WA).
   - then with 20 ml of Immuno Basic Washing Buffer (Code : IAf-WB).
7. The column is now ready for use. This immunoaffinity column can be re-used 10 times without loss of binding capacity for the corresponding antigen.
8. Storage : at 4°C in ¹PBS or ²TBS buffer pH 7.4 in the presence of NaN₃ 0.1% (w/v).

¹PBS : Phosphate buffered saline (K₂HPO₄ 50mM, NaCl 150mM).
²TBS : Tris buffered saline (Tris.HCl 50mM, NaCl 150mM).

It is not difficult to immobilize a protein on a solid support using any classic activation method such as the cyanogen bromide or N-hydroxysuccinimidylcarboxylate... However, if the protein of interest is a specific antibody, its biological activity will be affected if not entirely lost after the covalent linkage between the solid support with the active site H₂N of the antibody.

AFFILAND has developed an Antibody "Activated Binding Gel" for immobilizing the antibody at its Fc portion leaving free its Fab. The biological properties of immobilized antibody will be so conserved.

  IgG & IgM & IgY Immobilization Kits