Article

Involvement of Amino Acid Residues 423–429 of Human Protein S in Binding to C4b-Binding Protein

Department of Molecular and Experimental Medicine, The Scripps Research Institute, La Jolla, California; Department of Haematology, University Hospital Utrecht, The Netherlands; Department of Haematology, Thrombosis and Haemostasis Research Center, Leiden University Hospital, The Netherlands
Blood Cells, Molecules, and Diseases DOI:10.1006/bcmd.1998.0175 pp.101-112

ABSTRACT ABSTRACT: Human protein S binds to C4b-binding protein (C4BP) both in plasma and in a system using purified proteins. Amino acid residues 420-434 of the first disulfide loop of the sex hormone binding globulinlike domain of protein S are involved in the interaction of protein S with C4BP. To define the involvement of specific polar amino acids within residues 420-434, we studied in parallel synthetic protein S peptides and recombinant protein S variants containing the same amino acid replacements, K423E, E424K, Q427E and K429E. Synthetic peptide analogs of peptide PSP-420 (residues 420-434) were assayed for binding C4BP and as inhibitors of complex formation. The PSP-420 peptide and the analogous peptide with the substitution E424K, but not the peptides containing the substitutions K423E and K429E, were able to bind C4BP. Recombinant proteins with mutations of K423E, Q427E and K429E showed reduced affinity for C4BP compared to plasma protein S, recombinant wild type protein S, or E424K-protein S. These results suggest that Lys-423, Gln-427 and Lys-429 of protein S are important for normal binding to C4BP. The anti-protein S monoclonal antibody LJ-56, raised against peptide PSP-420, recognizes only free protein S and inhibits complex formation with C4BP. Antibody LJ-56 recognized the E424K and Q427E peptides but not the K423E or K429E peptides. Similarly, the E424K and Q427E protein S mutants were recognized by LJ-56, whereas the K423E and K429E protein S mutants were not recognized. This suggests that both in the peptide PSP-420 and in protein S, Lys-423 and Lys-429 significantly contribute to binding to antibody LJ-56. These results demonstrate that protein S residues 423, 427 and 429, but not residue 424, are involved in binding to both the antibody LJ-56 and to C4BP. When peptides PSP 420 and SL-6 (residues 447-460) with carboxyterminal amide or carboxylate moieties were compared to their ability to inhibit C4BP-protein S complexation, PSP-420-amide was the most potent. This finding together with the other results described here supports the hypothesis that the residues 420 and 434 in protein S provides a major binding site for C4BP

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Keywords

amino acid replacements
 
analogous peptide
 
anti-protein S monoclonal antibody LJ-56
 
antibody LJ-56
 
bind C4BP
 
binding C4BP
 
C4b-binding protein
 
C4BP-protein S complexation
 
Human protein S binds
 
K429E protein S mutants
 
major binding site
 
normal binding
 
protein S residues 423
 
PSP-420 peptide
 
purified proteins
 
Q427E protein S mutants
 
Recombinant proteins
 
specific polar amino acids
 
substitution E424K
 
Synthetic peptide analogs