Measurement of factor XIII activity in plasma.

Clin Chem Lab Med

Clinical Research Center, University of Debrecen, Medical and Health Science Center, Debrecen, Hungary.

Published: February 2012

AI Article Synopsis

  • Coagulation factor XIII (FXIII) is activated by thrombin and calcium, playing a crucial role in stabilizing fibrin clots and preventing their breakdown.
  • FXIII deficiency can lead to severe bleeding issues, highlighting the importance of accurate FXIII activity testing for diagnosis.
  • This review evaluates FXIII activity assays, noting that while incorporation assays are sensitive but complex, ammonia release assays are quicker, standardized, and recommended for screening FXIII deficiency.

Article Abstract

Coagulation factor XIII (FXIII) is converted by thrombin and Ca(2+) into an active transglutaminase (FXIIIa) in the final phase of coagulation cascade. Its main function is the mechanical stabilization of fibrin clot and its protection from fibrinolysis by cross-linking of fibrin chains and α(2)-plasmin inhibitor to fibrin. In non-substituted patients FXIII deficiency is a severe hemorrhagic diathesis, not infrequently with fatal consequences. The main reason for using FXIII assays is the diagnosis of FXIII deficiency. The aim of this review is to provide a comprehensive critical evaluation of the methods reported for the determination of FXIII activity in the plasma. Such methods are based on two principles: 1) measurement of labeled amines incorporated by FXIIIa into a glutamine residue of a substrate protein, 2) monitoring ammonia released from a peptide bound glutamine residue by FXIIIa using NAD(P)H dependent glutamate dehydrogenase indicator reaction. The incorporation assays are sensitive, but cumbersome and time-consuming, they are difficult to standardize and cannot be automated. The ammonia release assays are less sensitive, but quick, well standardized, and can be automated; this type of assay is recommended for the screening of FXIII deficiency. The traditional clot solubility assay should not be used for this purpose.

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Source
http://dx.doi.org/10.1515/cclm-2011-0730DOI Listing

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