On the binding of complement to solid artificial surfaces in vitro

Since the realization of a complement activation capacity by artificial surfaces upon contact with blood. a common belief has evolved that charged nucleophilic surface groups such as amine (-NH2) and hydroxyl (-OH) react with and eventually bind to the internal thioester in complement factor 3 (C3). A covalent amide or ester linkage is thereby supposed to form between Ob and the surface itself. In this report, we present complement surface binding data by null-ellipsometry for two nucleophilic Surfaces (-NH2 and -OH), for surfaces with immunoglobulin G (IgG) covalently bound, and for IgG spontaneously pre-adsorbed to hydrophobic silicon. The results reveal that the plasma proteins that were deposited during complement activation became eluted by sodium dodecyl sulfate. Hence the direct covalent binding between C3 and solid nucleophilic surfaces seems to be only of moderate importance. at least during shorter serum incubations. This strongly suggests that the prevalent covalent linkage model between solid artificial Surfaces and C3b is not accurate. Instead we suggest a more pronounced role for C3 associations to other adsorbed proteins and/or electrostatic and hydrophobic protein-surface interactions. (C) 2001 Elsevier Science Ltd. All rights reserved.