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Wiley InterScience

Journal of Thrombosis and Haemostasis

Journal of Thrombosis and Haemostasis

Volume 6 Issue 4, Pages 654 - 659

Published Online: 17 Jan 2008

© 2010 International Society on Thrombosis and Haemostasis



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ORIGINAL ARTICLE
Common genetic variants associated with plasma fibrin D-dimer concentration in older European- and African-American adults
L. A. LANGE*, A. P. REINER, C. L. CARTY, N. S. JENNY, M. CUSHMAN and E. M. LANGE
  *Department of Genetics and the Carolina Center for Genome Sciences, University of North Carolina, Chapel Hill, NC ;   Department of Epidemiology, University of Washington, Seattle, WA ;   Departments of Pathology and Medicine, University of Vermont College of Medicine, Burlington, VT ; and   §Department of Biostatistics and the Carolina Center for Genome Sciences, University of North Carolina, Chapel Hill, NC, USA
Correspondence to Leslie A. Lange, Department of Genetics, University of North Carolina, 4300c Medical Biomolecular Research Building, Chapel Hill, NC 27599-7264, USA.
Tel.: +1 919 966 9562; fax: +1 919 843 4682.
E-mail: leslie_lange@med.unc.edu
Copyright © 2008 International Society on Thrombosis and Haemostasis
KEYWORDS
D-dimer • fibrinogen • genetics • plasminogen activator inhibitor • urokinase

ABSTRACT

Summary.  Background and Objectives: D-dimer is a hemostasis marker that reflects ongoing fibrin formation and degradation. There is significant inter-individual and inter-population variability in D-dimer concentration, but whether genetic factors underlie these differences is largely unknown. We hypothesized that common coagulation gene variants contribute to differences in circulating D-dimer concentration. Methods: The setting was European-American (EA; = 1858) and African-American (AA; = 327) unrelated older adults from the Cardiovascular Health Study (CHS), in which we genotyped SNPs in 42 genes related to blood coagulation and fibrinolysis. Results: Several fibrinogen gene polymorphisms, including the Thr312Ala Aα chain variant and the FGG-10034 C/T variant, were associated with ∼20% higher plasma D-dimer levels in EA (false discovery rate < 5% for covariate-adjusted model). There was also some evidence that a Pro41Leu variant of the PLAU gene encoding urinary plasminogen activator and non-coding polymorphism of the plasminogen activator inhibitor type 1 gene (SERPINE1) were associated with higher plasma D-dimer in EA. There were no significant associations between the studied coagulation or fibrinolysis gene SNPs and plasma D-dimer levels in the smaller AA sample. However, each standard deviation increase in European ancestry assessed by ancestry-informative gene markers was associated with ∼10% lower mean D-dimer levels in AA. Conclusions: Together, common coagulation/fibrinolysis gene SNPs explained only ∼2% of the variance in plasma D-dimer levels in EA. These findings suggest that the association of D-dimer with risk of vascular outcomes may be mediated largely by environmental factors, other genes, and/or genetic interactions.


Received 15 November 2007, accepted 9 January 2008

DIGITAL OBJECT IDENTIFIER (DOI)
10.1111/j.1538-7836.2008.02906.x About DOI

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