DNA and histones impair the mechanical stability and lytic susceptibility of fibrin formed by staphylocoagulase

Erzsébet Komorowicz; Veronika J Farkas; László Szabó; Sophie Cherrington; Craig Thelwell; Krasimir Kolev

doi:10.3389/fimmu.2023.1233128

DNA and histones impair the mechanical stability and lytic susceptibility of fibrin formed by staphylocoagulase

Front Immunol. 2023 Aug 17:14:1233128. doi: 10.3389/fimmu.2023.1233128. eCollection 2023.

Authors

Erzsébet Komorowicz¹, Veronika J Farkas¹, László Szabó^{1

2}, Sophie Cherrington³, Craig Thelwell³, Krasimir Kolev¹

Affiliations

¹ Institute of Biochemistry and Molecular Biology, Department of Biochemistry, Semmelweis University, Budapest, Hungary.
² Plasma Chemistry Research Group, Institute of Materials and Environmental Chemistry, Research Centre for Natural Sciences, Budapest, Hungary.
³ South Mimms Laboratories, Medicines and Healthcare Products Regulatory Agency, Potters Bar, United Kingdom.

Abstract

Background: Staphylocoagulase (SCG) is a virulence factor of Staphylococcus aureus, one of the most lethal pathogens of our times. The complex of SCG with prothrombin (SCG/ProT) can clot fibrinogen, and SCG/ProT-induced fibrin and plasma clots have been described to show decreased mechanical and lytic resistance, which may contribute to septic emboli from infected cardiac vegetations. At infection sites, neutrophils can release DNA and histones, as parts of neutrophil extracellular traps (NETs), which in turn favor thrombosis, inhibit fibrinolysis and strengthen clot structure.

Objectives: To characterize the combined effects of major NET-components (DNA, histone H1 and H3) on SCG/ProT-induced clot structure, mechanical and lytic stability.

Methods: Recombinant SCG was used to clot purified fibrinogen and plasma. The kinetics of formation and lysis of fibrin and plasma clots containing H1 or core histones+/-DNA were followed by turbidimetry. Fibrin structure and mechanical stability were characterized with scanning electron microscopy, pressure-driven permeation, and oscillation rheometry.

Results: Histones and DNA favored the formation of thicker fibrin fibers and a more heterogeneous clot structure including high porosity with H1 histone, whereas low porosity with core histones and DNA. As opposed to previous observations with thrombin-induced clots, SCG/ProT-induced fibrin was not mechanically stabilized by histones. Similarly to thrombin-induced clots, the DNA-histone complexes prolonged fibrinolysis with tissue-type plasminogen activator (up to 2-fold). The anti-fibrinolytic effect of the DNA and DNA-H3 complex was observed in plasma clots too. Heparin (low molecular weight) accelerated the lysis of SCG/ProT-clots from plasma, even if DNA and histones were also present.

Conclusions: In the interplay of NETs and fibrin formed by SCG, DNA and histones promote structural heterogeneity in the clots, and fail to stabilize them against mechanical stress. The DNA-histone complexes render the SCG-fibrin more resistant to lysis and thereby less prone to embolization.

Keywords: NET; extracellular DNA; fibrin; fibrinolysis; histone; staphylocoagulase.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Coagulase
DNA
Fibrin*
Fibrinogen
Hemostatics*
Histones
Thrombin

Substances

Fibrin
Histones
Coagulase
Thrombin
DNA
Fibrinogen
Hemostatics

Grants and funding

This work was supported by the Hungarian National Research, Development and Innovation Office (NKFIH) (#137563), Thematic Institutional Excellence funding scheme of the Ministry of Innovation and Technology in Hungary for the Molecular Biology thematic programme of Semmelweis University (TKP2021-EGA-24), and Central Europe Leuven Strategic Alliance CELSA research fund (CELSA/22/024).