C4BP-IgM protein as a therapeutic approach to treat Neisseria gonorrhoeae infections
Serena Bettoni, Jutamas Shaughnessy, Karolina Maziarz, David Ermert, Sunita Gulati, Bo Zheng, Matthias Mörgelin, Susanne Jacobsson, Kristian Riesbeck, Magnus Unemo, Sanjay Ram, Anna M. Blom
Serena Bettoni, Jutamas Shaughnessy, Karolina Maziarz, David Ermert, Sunita Gulati, Bo Zheng, Matthias Mörgelin, Susanne Jacobsson, Kristian Riesbeck, Magnus Unemo, Sanjay Ram, Anna M. Blom
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Research Article Infectious disease Therapeutics

C4BP-IgM protein as a therapeutic approach to treat Neisseria gonorrhoeae infections

Abstract

Gonorrhea is a sexually transmitted infection with 87 million new cases per year globally. Increasing antibiotic resistance has severely limited treatment options. A mechanism that Neisseria gonorrhoeae uses to evade complement attack is binding of the complement inhibitor C4b-binding protein (C4BP). We screened 107 porin B1a (PorB1a) and 83 PorB1b clinical isolates randomly selected from a Swedish strain collection over the last 10 years and noted that 96/107 (89.7%) PorB1a and 16/83 (19.3%) PorB1b bound C4BP; C4BP binding substantially correlated with the ability to evade complement-dependent killing (r = 0.78). We designed 2 chimeric proteins that fused C4BP domains to the backbone of IgG or IgM (C4BP-IgG; C4BP-IgM) with the aim of enhancing complement activation and killing of gonococci. Both proteins bound gonococci (KD C4BP-IgM = 2.4 nM; KD C4BP-IgG 980.7 nM), but only hexameric C4BP-IgM efficiently outcompeted heptameric C4BP from the bacterial surface, resulting in enhanced complement deposition and bacterial killing. Furthermore, C4BP-IgM substantially attenuated the duration and burden of colonization of 2 C4BP-binding gonococcal isolates but not a non–C4BP-binding strain in a mouse vaginal colonization model using human factor H/C4BP–transgenic mice. Our preclinical data present C4BP-IgM as an adjunct to conventional antimicrobials for the treatment of gonorrhea.

Authors

Serena Bettoni, Jutamas Shaughnessy, Karolina Maziarz, David Ermert, Sunita Gulati, Bo Zheng, Matthias Mörgelin, Susanne Jacobsson, Kristian Riesbeck, Magnus Unemo, Sanjay Ram, Anna M. Blom

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Figure 4

C4BP-IgM promotes complement activation selectively on the bacterial surface.

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C4BP-IgM promotes complement activation selectively on the bacterial sur...
(A) C1q deposition on plates coated with C4BP-IgM fusion protein, human aggregated IgG (hAgg_IgG), human IgM (hIgM), α1AT, or BSA. (B and C) C3 deposition from either human serum (NHS) or mouse serum on C4BP-IgM fusion protein or hAgg_IgG, hIgM, α1AT, or BSA immobilized on plate. Each dot represents mean ± SEM of 3 independently performed experiments. (DF) C4BP binding and complement deposition on the surface of 5 laboratory strains of N. gonorrhoeae using 10% NHS with or without C4BP-IgM 20 μg/mL. Bars display mean ± SD, with circles indicating independent repeats. P values were performed by 2-way ANOVA with Sidak’s multiple-comparisons test. (G and H) C3 complement deposition on the surface of apoptotic Jurkat cells or human erythrocytes. Each bar represents the mean ± SD of 4 independently performed experiments. Differences were analyzed using 1-way ANOVA with Dunnett’s multiple-comparisons test. *P < 0.05, ***P < 0.005, and ****P < 0.0001 as indicated, or compared with NHS.