for the isolation any GST-tagged cloned protein. It is possible to remove the GST tag
in a one-step process by adding PreScission™Protease to the matrix, as it will be
bound to the column and remove the tag as the protein is eluted.Practical procedure
The procedure for affinity chromatography is similar to that used in other forms of
liquid chromatography. The buffer used must contain any cofactors, such as metal
ions, necessary for ligand–macromolecule interaction. Once the sample has been applied
and the macromolecule bound, the column is eluted with more buffer to remove non-
specifically bound contaminants. The purified compound is recovered from the ligand
by eitherspecificornon-specific elution. Non-specific elution may be achieved by a
change in either pH or ionic strength. pH shift elution using dilute acetic acid or
ammonium hydroxide results from a change in the state of ionisation of groups in the
ligand and/or the macromolecule that are critical to ligand–macromolecule binding.
A change in ionic strength, not necessarily with a concomitant change in pH, also
causes elution due to a disruption of the ligand–macromolecule interaction; 1M NaCl
is frequently used for this purpose.Table 11.5Examples of group-specific ligands commonly used in affinity
chromatography
Ligand Affinity
Nucleotides
50 -AMP NADþ-dependent dehydrogenases, some kinases
2050 -ADP NADPþ-dependent dehydrogenasesCalmodulin Calmodulin-binding enzymes
Avidin Biotin-containing enzymes
Fatty acids Fatty-acid-binding proteins
Heparin Lipoproteins, lipases, coagulation factors, DNA polymerases, steroid receptor
proteins, growth factors, serine protease inhibitors
Proteins A and G Immunoglobulins
Concanavalin A Glycoproteins containinga-D-mannopyranosyl anda-D-glucopyranosyl residues
Soybean lectin Glycoproteins containingN-acetyl-a-(orb)-D-galactopyranosyl residues
Phenylboronate Glycoproteins
Poly(A) RNA containing poly(U) sequences, some RNA-specific proteins
Lysine rRNA
Cibacron Blue
F3G-A
Nucleotide-requiring enzymes, coagulation factors468 Chromatographic techniques