Determination of background serum density for lipoprotein ultracentrifugation

It is necessary to know the density of serum exclusive of its macromolecules (background density) prior to density adjustment with solid potassium bromide for ultra‐centrifugal separation of lipoprotein fractions. To evaluate this, we compared the densities of the corresponding ultrafiltrates or dialysates of both human and equine sera produced by ultrafiltration and equilibrium dialysis methods for macromolecule removal. Excellent correlation is found between background densities determined following ultrafiltration or equilibrium dialysis. These data validate the use of ultrafiltration as a simple, direct method for determination of background serum densities but reveal equilibrium dialysis to be more time consuming and less precise. Using ultrafiltration, we find the background density for equine serum to be 1.004 g/ml, and initial investigation suggests this value may be altered by freezing, prolonged refrigeration (3 months), or heating to inactivate lecithin: cholesterol acyltransferase.