An Affinity Chromatography Technique for the Purification of Monoclonal Antibodies
An Affinity Chromatography Technique for the Purification of Monoclonal Antibodies
Trascrizione
Take an affinity chromatography column containing agarose beads conjugated to Protein A, an antibody-binding protein.
Add a binding buffer with a neutral pH to equilibrate the column.
Load the culture supernatant from an antibody-producing cell culture, containing monoclonal antibodies and contaminating cellular proteins.
The neutral pH facilitates protein A binding to the Fc region of the antibodies while the contaminants flow through.
Measure the UV absorbance of the flow through to create a chromatogram. A high absorbance during sample loading indicates unbound proteins in the flow through.
Wash the column with the binding buffer to remove non-specifically bound contaminants.
Add an elution buffer with a low pH to disrupt the Protein A-antibody interaction. Collect the eluted antibodies by monitoring the peak in absorbance.
Neutralize the pH to prevent antibody degradation and transfer into a centrifugal filter.
Centrifuge to concentrate the antibodies and resuspend in a buffer for downstream assays.