Binding of C4b-Binding Protein to Porin

Author:

Ram Sanjay1,Cullinane Meabh1,Blom Anna M.2,Gulati Sunita1,McQuillen Daniel P.1,Monks Brian G.1,O'Connell Catherine1,Boden Ryan1,Elkins Christopher3,Pangburn Michael K.4,Dahlbäck Björn2,Rice Peter A.1

Affiliation:

1. Evans Biomedical Research Center, Boston Medical Center, Boston, Massachusetts 02118

2. Lund University, Malmö S-20502, Sweden

3. University of North Carolina, Chapel Hill, North Carolina 27599

4. University of Texas Health Sciences Center, Tyler, Texas 75708

Abstract

We screened 29 strains of Neisseria gonorrhoeae and found 16/21 strains that resisted killing by normal human serum and 0/8 serum sensitive strains that bound the complement regulator, C4b-binding protein (C4bp). Microbial surface–bound C4bp demonstrated cofactor activity. We constructed gonococcal strains with hybrid porin (Por) molecules derived from each of the major serogroups (Por1A and Por1B) of N. gonorrhoeae, and showed that the loop 1 of Por1A is required for C4bp binding. Por1B loops 5 and 7 of serum-resistant gonococci together formed a negatively charged C4bp-binding domain. C4bp–Por1B interactions were ionic in nature (inhibited by high salt or by heparin), whereas the C4bp–Por1A bond was hydrophobic. Only recombinant C4bp mutant molecules containing the NH2-terminal α-chain short consensus repeat (SCR1) bound to both Por1A and Por1B gonococci, suggesting that SCR1 contained Por binding sites. C4bp α-chain monomers did not bind gonococci, indicating that the polymeric form of C4bp was required for binding. Using fAb fragments against C4bp SCR1, C4bp binding to Por1A and Por1B strains was inhibited in a complement-dependent serum bactericidal assay. This resulted in complete killing of these otherwise fully serum resistant strains in only 10% normal serum, underscoring the importance of C4bp in mediating gonococcal serum resistance.

Publisher

Rockefeller University Press

Subject

Immunology,Immunology and Allergy

Reference86 articles.

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