Lignosulfonic Acid Sodium Is a Noncompetitive Inhibitor of Human Factor XIa

Srabani Kar; Page Bankston; Daniel K Afosah; Rami A Al-Horani

doi:10.3390/ph14090886

Lignosulfonic Acid Sodium Is a Noncompetitive Inhibitor of Human Factor XIa

Pharmaceuticals (Basel). 2021 Aug 31;14(9):886. doi: 10.3390/ph14090886.

Authors

Srabani Kar¹, Page Bankston¹, Daniel K Afosah², Rami A Al-Horani¹

Affiliations

¹ Division of Basic Pharmaceutical Sciences, College of Pharmacy, Xavier University of Louisiana, New Orleans, LA 70125, USA.
² Department of Chemistry and Biochemistry, Washington and Lee University, Lexington, VA 24450, USA.

Abstract

The anticoagulant activity of lignosulfonic acid sodium (LSAS), a non-saccharide heparin mimetic, was investigated in this study. LSAS is a relatively safe industrial byproduct with similar polyanionic characteristics to that of heparin. Human plasma clotting assays, fibrin polymerization testing, and enzyme inhibition assays were exploited to investigate the anticoagulant activity of LSAS. In normal human plasma, LSAS selectively doubled the activated partial thromboplastin time (APTT) at ~308 µg/mL. Equally, LSAS doubled APTT at ~275 µg/mL in antithrombin-deficient plasma. Yet, LSAS doubled APTT at a higher concentration of 429 µg/mL using factor XI-deficient plasma. LSAS did not affect FXIIIa-mediated fibrin polymerization at 1000 µg/mL. Enzyme assays revealed that LSAS inhibits factor XIa (FXIa) with an IC₅₀ value of ~8 μg/mL. LSAS did not inhibit thrombin, factor IXa, factor Xa, factor XIIIa, chymotrypsin, or trypsin at the highest concentrations tested and demonstrated significant selectivity against factor XIIa and plasmin. In Michaelis-Menten kinetics, LSAS decreased the V_MAX of FXIa hydrolysis of a tripeptide chromogenic substrate without significantly changing its K_M indicating an allosteric inhibition mechanism. The inhibitor also disrupted the generation of FXIa-antithrombin complex, inhibited factor XIIa-mediated and thrombin-mediated activation of the zymogen factor XI to FXIa, and competed with heparin for binding to FXIa. Its action appears to be reversed by protamine sulfate. Structure-activity relationship studies demonstrated the advantageous selectivity and allosteric behavior of LSAS over the acetylated and desulfonated derivatives of LSAS. LSAS is a sulfonated heparin mimetic that demonstrates significant anticoagulant activity in human plasma. Overall, it appears that LSAS is a potent, selective, and allosteric inhibitor of FXIa with significant anticoagulant activity in human plasma. Altogether, this study introduces LSAS as a promising lead for further development as an anticoagulant.

Keywords: allosteric inhibitor; anticoagulant; factor XIa; lignin; sulfonate.

Abstract

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