Fullerene-Interfaced Porphyrin Ligand in Affinity Chromatography of Membrane Proteins

To purify the mammalian cell membrane porphyrin binding proteins (PBP), an original affinity chromatographic technique is proposed. The method is based on the application of an agarose attached fullerene-porphyrin ligand connected to a polysaccharide gel matrix through the epoxy-cyclohexyl residue interface. A selective PBP-stationary phase coupling has been managed in a single column chromatographic run leading to a complete purification of the 17.6 kDa monomer protein from the rat myocardium mitochondria membranes. A synchronous pH and ionic strength linear gradients were used to separate this protein with a high specific affinity to the porphyrin K related structures from all non-specific sorption retained membrane proteins.