Your search keyword '"Factor XIIa analysis"' showing total 71 results

1. Development of an updated assay for prekallikrein activator in albumin and immunoglobulin therapeutics.

Author

Roberts G, Fox B, and Longstaff C

Subjects

Factor XIIa metabolism, Humans, Prekallikrein metabolism, Reproducibility of Results, Albumins, Factor XIIa analysis, Immunoglobulins

Abstract

Background: Prekallikrein activator (PKA) is a contaminating enzyme found in therapeutic albumin and immunoglobulin products. The level is commonly measured using methods such as that defined by the European Pharmacopoeia (Ph Eur) with traceability to the WHO International Standard for PKA. This method generally works well, but problems are sometimes observed., Materials and Methods: A simplified one-step method has been developed to replace the existing Ph Eur two-step method which consists of kallikrein generation followed by kallikrein measurement using a chromogenic substrate. Analysis of data from the one-stage method is simplified by the use of a dedicated online app., Results: The one-stage method was validated against the current Ph Eur method using batches of albumin and immunoglobulins. Problem batches of immunoglobulins were investigated using the one-stage method. Improved methodology using true initial rate determinations and use of acid-treated prekallikrein substrate (PKS) helped understand and reduce artefactual results., Conclusions: The one-stage method and associated app streamline real-time determination of PKA and promote good principles of enzyme assays to limit substrate depletion, while also conserving expensive PKS. Blanking steps and reproducibility are simplified., (© 2020 Crown copyright. Vox Sanguinis published by John Wiley & Sons Ltd on behalf of International Society of Blood Transfusion. This article is published with the permission of the controller of HMSO and the Queen’s Printer for Scotland.)

Published

2021

2. Contact system activation and high thrombin generation in hyperthyroidism.

Author

Kim N, Gu JY, Yoo HJ, Han SE, Kim YI, Nam-Goong IS, Kim ES, and Kim HK

Subjects

Adult, Blood Coagulation, Blood Coagulation Factors analysis, Bradykinin blood, DNA blood, DNA metabolism, Factor XIIa analysis, Female, Histones blood, Histones metabolism, Humans, Kininogen, High-Molecular-Weight blood, Leukocyte Elastase blood, Male, Middle Aged, Prekallikrein analysis, Thyroxine blood, Extracellular Traps physiology, Hyperthyroidism metabolism, Thrombin biosynthesis

Abstract

Background: Hyperthyroidism is associated with increased thrombotic risk. As contact system activation through formation of neutrophil extracellular traps (NET) has emerged as an important trigger of thrombosis, we hypothesized that the contact system is activated along with active NET formation in hyperthyroidism and that their markers correlate with disease severity., Subjects and Methods: In 61 patients with hyperthyroidism and 40 normal controls, the levels of coagulation factors (fibrinogen, and factor VII, VIII, IX, XI and XII), D-dimer, thrombin generation assay (TGA) markers, NET formation markers (histone-DNA complex, double-stranded DNA and neutrophil elastase) and contact system markers (activated factor XII (XIIa), high-molecular-weight kininogen (HMWK), prekallikrein and bradykinin) were measured., Results: Patients with hyperthyroidism showed higher levels of fibrinogen (median (interquartile range), 315 (280-344) vs 262 (223-300), P  = 0.001), D-dimer (103.8 (64.8-151.5) vs 50.7 (37.4-76.0), P  < 0.001), peak thrombin (131.9 (102.2-159.4) vs 31.6 (14.8-83.7), P  < 0.001) and endogenous thrombin potential (649 (538-736) vs 367 (197-1147), P  = 0.021) in TGA with 1 pM tissue factor, neutrophil elastase (1.10 (0.39-2.18) vs 0.23 (0.20-0.35), P  < 0.001), factor XIIa (66.9 (52.8-87.0) vs 73.0 (57.1-86.6), P  < 0.001), HMWK (6.11 (4.95-7.98) vs 3.83 (2.60-5.68), P  < 0.001), prekallikrein (2.15 (1.00-6.36) vs 1.41 (0.63-2.22), P  = 0.026) and bradykinin (152.4 (137.6-180.4) vs 118.3 (97.1-137.9), P  < 0.001) than did normal controls. In age- and sex-adjusted logistic regression analysis, fibrinogen, factor VIII, IX and XIIa, D-dimer, peak thrombin, neutrophil elastase, HMWK and bradykinin showed significant odds ratios representing hyperthyroidism's contribution to coagulation and contact system activation. Free T4 was significantly correlated with factors VIII and IX, D-dimer, double-stranded DNA and bradykinin., Conclusion: This study demonstrated that contact system activation and abundant NET formation occurred in the high thrombin generation state in hyperthyroidism and were correlated with free T4 level., (© 2017 European Society of Endocrinology.)

Published

2017

3. Evidence of contact activation in patients suffering from ST-elevation myocardial infarction.

Author

Christensen K, Kozarcanin H, Ekdahl KN, and Nilsson B

Subjects

Aged, Antithrombin Proteins analysis, Complement C1 Inactivator Proteins analysis, Complement C1 Inhibitor Protein, Female, Humans, Male, Middle Aged, Blood Coagulation, Factor XIIa analysis, Myocardial Infarction blood

Abstract

Introduction: Factor (F) XIIa is an attractive target for anticoagulation in arterial thrombosis. The aim of this study is to investigate the degree of involvement of the contact system in cardiac infarctions., Methods and Patients: 165 patients suffering from ST-elevation myocardial infarction (STEMI) and 100 healthy controls were included in the study. Samples were drawn at admission before percutaneous intervention (PCI), 1-3days post-percutaneous intervention (PCI) and, in one-third of the patients, 3months after PCI. In order to investigate the degree of Factor XII (FXII) activation, changes in FXIIa/AT and FXIIa/C1INH complex levels were quantified by ELISA., Results: FXIIa/AT levels at admission (0.89±0.50; p<0.01) were significantly higher than those in normal individuals (0.39±0.28), but the levels after 1-3days (0.33±0.33; p<0.05) were essentially normalized. In contrast, the FXII/C1INH levels at admission (1.40±0.72; p<0.001) and after 1-3days (0.83±0.59; p<0.001) were both significantly higher than those in normal individuals (0.40±0.30). FXIIa/AT and FXIIa/C1INH complexes at admission (p<0.001; p<0.001) and after 1-3days (p<0.02; p<0.001) were significantly different from those at 3months. No significant differences were observed when the data were stratified for patency (open/closed culprit lesions)., Conclusion: Both FXIIa/AT and FXIIa/C1INH complexes were significantly increased and reflected the activation of FXII in STEMI patients at admission. In particular, FXIIa/AT complex elevations support the hypothesis that clot propagation-mediated FXII activation had occurred, and this activation may be a target for anticoagulation in patients with cardiac infarction. Based on previous studies, the FXIIa/C1INH complex levels were primarily interpreted to reflex endothelial cell activation., (Copyright © 2016. Published by Elsevier Ltd.)

Published

2016

4. Factor XII-mediated contact activation related to poor prognosis in disseminated intravascular coagulation.

Author

Park HS, Gu J, You HJ, Kim JE, and Kim HK

Subjects

Adult, Aged, Factor XIIa analysis, Female, Humans, Male, Middle Aged, Prognosis, Blood Coagulation, Disseminated Intravascular Coagulation blood, Disseminated Intravascular Coagulation diagnosis, Factor XII analysis

Abstract

Background: The contact system that initiates the intrinsic coagulation pathway plays a role in thrombus formation. Since neutrophil extracellular traps (NET), which are mainly composed of histone and DNA, are actively formed in disseminated intravascular coagulation (DIC) and the NET can activate factor XII, it is plausible that a NET component strongly activates the contact system in patients with DIC., Methods: In 146 patients suspected of having DIC, the plasma levels of contact system factors including factor XII, activated factor XII (XIIa), prekallikrein, high-molecular-weight kininogen (HMWK), bradykinin, extrinsic factor VII and histone–DNA complex were measured. In an in vitro plasma clotting assay, factor XII–deficient plasma was stimulated with silica or histone., Results: The levels of not only extrinsic coagulation factor VII but also intrinsic coagulation factors including factors XI and XII were significantly decreased in patients with overt DIC in comparison with those with no overt DIC. Factor XIIa and histone-DNA complex were also significantly increased in patients with overt DIC. However,HMWK, prekallikrein and bradykin inw ere not significantly different between patients with and without overt DIC. Interestingly, factors XII and XIIa were revealed as significantly independent potential prognostic markers for DIC. The histone-DNA complex level significantly contributed to the factor XIIa level (20.6%). In an in vitro clotting assay, histone, a major component of NET, activated coagulation that was dependent, in part, on the presence of factor XII., Conclusion: These findings suggest that active NET formation can induce factor XII-mediated coagulation activation in patients with DIC with poor prognosis. The resulting factor XIIa release can be used as an independent potential prognostic marker for DIC. Activation of factor XII-mediated coagulation may be a potential therapeutic target in DIC,

Published

2016

5. Hypercoagulability and the risk of myocardial infarction and ischemic stroke in young women.

Author

Siegerink B, Maino A, Algra A, and Rosendaal FR

Subjects

Adult, Age Factors, Brain Ischemia etiology, Case-Control Studies, Comorbidity, Confidence Intervals, Contraceptives, Oral adverse effects, Diabetes Mellitus epidemiology, Factor XIII genetics, Factor XIIa analysis, Factor XIa analysis, Female, Hospital Mortality, Humans, Hypercholesterolemia epidemiology, Hypertension epidemiology, Kallikreins analysis, Lupus Coagulation Inhibitor blood, Middle Aged, Myocardial Infarction etiology, Netherlands epidemiology, Odds Ratio, Risk, Risk Factors, Sex Factors, Smoking epidemiology, Thrombophilia blood, Thrombophilia chemically induced, Thrombophilia complications, Young Adult, Brain Ischemia epidemiology, Myocardial Infarction epidemiology, Thrombophilia epidemiology

Abstract

Background: Myocardial infarction (MI) and ischemic stroke (IS) are acute forms of arterial thrombosis and share some, but not all, risk factors, indicating different pathophysiological mechanisms., Objective: This study aims to determine if hypercoagulability has a differential effect on the risk of MI and IS., Patients and Methods: We reviewed the results from the Risk of Arterial Thrombosis in Relation to Oral Contraceptives study, a population-based case-control study involving young women (< 50 years) with MI, non-cardioembolic IS and healthy controls. From these data, relative odds ratios (ORIS /ORMI ) and their corresponding confidence intervals for all prothrombotic factors that were studied in both subgroups were calculated., Results: Twenty-nine prothrombotic risk factors were identified as measures of hypercoagulability. Twenty-two of these risk factors (21/29, 72%) had a relative odds ratios > 1; for 12 (41%), it was > 2; and for 5 (17%), it was > 2.75. The five risk factors with the largest differences in associations were high levels of activated factor XI (FXI) and FXII, kallikrein, the presence of lupus anticoagulans, and a genetic variation in the FXIII gene., Conclusion: In young women, prothrombotic factors are associated more with the risk of IS than with MI risk, suggesting a different role of hypercoagulability in the mechanism leading to these two diseases., (© 2015 International Society on Thrombosis and Haemostasis.)

Published

2015

6. Heparan sulfate proteoglycans mediate factor XIIa binding to the cell surface.

Author

Wujak L, Didiasova M, Zakrzewicz D, Frey H, Schaefer L, and Wygrecka M

Subjects

Cells, Cultured, Factor XIIa analysis, Fibroblasts metabolism, Heparan Sulfate Proteoglycans analysis, Humans, Lung metabolism, Protein Binding, Factor XIIa metabolism, Fibroblasts pathology, Heparan Sulfate Proteoglycans metabolism, Lung pathology, Pulmonary Fibrosis metabolism, Pulmonary Fibrosis pathology

Abstract

Hageman factor (FXIIa) initiates the intrinsic coagulation pathway and triggers the kallikrein-kinin and the complement systems. In addition, it functions as a growth factor by expressing promitogenic activities toward several cell types. FXIIa binds to the cell surface via a number of structurally unrelated surface receptors; however, the underlying mechanisms are not yet fully understood. Here, we demonstrate that FXIIa utilizes cell membrane-bound glycosaminoglycans to interact with the cell surface of human lung fibroblasts (HLF). The combination of enzymatic, inhibitory, and overexpression approaches identified a heparan sulfate (HS) component of proteoglycans as an important determinant of the FXIIa binding capacity of HLF. Moreover, cell-free assays and competition experiments revealed preferential binding of FXIIa to HS and heparin over dextran sulfate, dermatan sulfate, and chondroitin sulfate A and C. Finally, we demonstrate that fibroblasts isolated from the lungs of the patients suffering from idiopathic pulmonary fibrosis (IPF) exhibit enhanced FXIIa binding capacity. Increased sulfation of HS resulting from elevated HS 6-O-sulfotransferase-1 expression in IPF HLF accounted, in part, for this phenomenon. Application of RNA interference technology and inhibitors of intracellular sulfation revealed the cooperative action of cell surface-associated HS and urokinase-type plasminogen activator receptor in the accumulation of FXIIa on the cell surface of IPF HLF. Moreover, FXIIa stimulated IPF HLF migration, which was abrogated by pretreatment of cells with heparinase I. Collectively, our study uncovers a novel role of HS-type glycosaminoglycans in a local accumulation of FXIIa on the cell membrane. The enhanced association of FXIIa with IPF HLF suggests its contribution to fibrogenesis., (© 2015 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2015

7. Human plasma-derived immunoglobulin G fractionated by an aqueous two-phase system, caprylic acid precipitation, and membrane chromatography has a high purity level and is free of detectable in vitro thrombogenic activity.

Author

Vargas M, Segura Á, Wu YW, Herrera M, Chou ML, Villalta M, León G, and Burnouf T

Subjects

Caprylates chemistry, Enzyme-Linked Immunosorbent Assay, Factor XIIa analysis, Humans, Immunoglobulin G chemistry, Oligopeptides chemistry, Thrombin biosynthesis, Chemical Fractionation methods, Chromatography methods, Immunoglobulin G isolation & purification, Plasma chemistry

Abstract

Background and Objectives: Instituto Clodomiro Picado has developed an immunoglobulin G (IgG) plasma fractionation process combining a polyethylene glycol/phosphate aqueous two-phase system (ATPS), caprylic acid precipitation and anion-exchange membrane chromatography. We evaluated the purity and in vitro thrombogenicity of such IgG, in line with current international requirements., Materials and Methods: Contributions of the different production steps to reduce thrombogenicity were assessed at 0·2 l-scale, and then the methodology was scaled-up to a 10 l-scale and final products (n = 3) were analysed. Purity, immunoglobulin composition, and subclass distribution were determined by electrophoretic and immunochemical methods. The in vitro thrombogenic potential was determined by a thrombin generation assay (TGA) using a Technothrombin fluorogenic substrate. Prekallikrein activator (PKA), plasmin, factor Xa, thrombin and thrombin-like activities were assessed using S-2302, S-2251, S-2222, S-2238 and S-2288 chromogenic substrates, respectively, and FXI by an ELISA., Results: The thrombogenicity markers were reduced mostly during the ATPS step and were found to segregate mostly into the discarded liquid upper phase. The caprylic acid precipitation eliminated the residual procoagulant activity. The IgG preparations made from the 10 l-batches contained 100% gamma proteins, low residual IgA and undetectable IgM. The IgG subclass distribution was not substantially affected by the process. TGA and amidolytic activities revealed an undetectable in vitro thrombogenic risk and the absence of proteolytic enzymes in the final product., Conclusions: Fractionating human plasma by an ATPS combined with caprylic acid and membrane chromatography resulted in an IgG preparation of high purity and free of a detectable in vitro thrombogenic risk., (© 2014 International Society of Blood Transfusion.)

Published

2015

8. C1-esterase inhibitor treatment: preclinical safety aspects on the potential prothrombotic risk.

Author

Schürmann D, Herzog E, Raquet E, Nolte MW, May F, Müller-Cohrs J, Björkqvist J, Dickneite G, and Pragst I

Subjects

Animals, Blood Coagulation Tests, Complement C1 Inhibitor Protein administration & dosage, Complement C1 Inhibitor Protein pharmacokinetics, Complement C1 Inhibitor Protein therapeutic use, Disease Models, Animal, Dose-Response Relationship, Drug, Drug Evaluation, Preclinical, Factor XIIa analysis, Factor XIa analysis, Femoral Artery, Fibrinolysis drug effects, Humans, Infusions, Intravenous, Kallikrein-Kinin System drug effects, Kallikrein-Kinin System physiology, Platelet Aggregation drug effects, Rabbits, Thrombelastography, Thrombin biosynthesis, Arterial Occlusive Diseases chemically induced, Complement C1 Inhibitor Protein toxicity, Venous Thrombosis chemically induced

Abstract

Human plasma-derived C1-esterase inhibitor (C1-INH) is an efficacious and safe treatment for hereditary angioedema. However, thrombotic events in subjects treated with C1-INH at recommended or off-label, high doses have been reported. In this study, we addressed the potential prothrombotic risk of C1-INH treatment in high doses using a non-clinical rabbit model. Following intravenous infusion of C1-INH to rabbits at doses up to 800 IU/kg, the exposure and the pharmacodynamic efficacy of C1-INH in rabbits were confirmed by activity measurements of C1-esterase, and coagulation factors XIa and XIIa, respectively. Potential prothrombotic effects were assessed following induction of venous and arterial thrombosis using in vivo models of venous and arterial stasis, complemented by various in vitro assays of coagulation markers. Administration of C1-INH at doses up to 800 IU/kg did not potentiate thrombus formation during venous stasis. In contrast, inhibition of arterial occlusion was observed upon C1-INH administration when compared with isotonic saline treatment, indicating antithrombotic rather than prothrombotic activity of high dose C1-INH treatment in vivo. This was further confirmed in vitro by decreased thrombin generation, increased activated partial thromboplastin time, clotting time and clot formation time, and inhibition of platelet aggregation. No relevant changes in fibrinolysis or in the levels of thrombin-antithrombin complexes, and prothrombin fragment 1+2 were observed upon high dose C1-INH treatment. The data suggest that treatment of healthy rabbits with high doses of C1-INH could potentially inhibit coagulation and thrombus formation rather than induce a prothrombotic risk.

Published

2014

9. Assessment of immunoglobulin concentrates on thrombogenic activity by thrombin generation assay, prekallikrein activator assay, and size-exclusion chromatography.

Author

Seifner A, Beck G, Bayer P, Eichmeir S, Lackner F, Rögelsperger O, Weber K, and Wollein G

Subjects

Austria, Drug Contamination, Factor XIIa analysis, Humans, Immunoglobulin G adverse effects, Immunoglobulin G blood, Immunoglobulins, Intravenous blood, Molecular Weight, Osmolar Concentration, Thrombin analysis, Thrombosis blood, Thrombosis immunology, Chromatography, Gel methods, Factor XIIa metabolism, Immunoglobulins, Intravenous adverse effects, Thrombin biosynthesis, Thrombosis etiology

Abstract

Background: Immunoglobulin G (IgG) concentrates have recently been found to be contaminated with procoagulant impurities causing thromboembolic events (TEEs) in vivo. In this study the question was raised whether a thrombin generation assay (TGA) will be able to characterize IgG samples from the Austrian market with regard to their thrombogenic potential., Study Design and Methods: A total of 44 IgG concentrates have been assayed by TGA employing pooled normal plasma and Factor (F)XI-deficient plasma (FXIdp). Furthermore, the prekallikrein activator assay including determination of blank values, size-exclusion chromatography, and further test systems required for batch release testing of IgG concentrates according to the European Pharmacopeia (Pharm. Eur.) were carried out., Results: All samples complied with acceptance criteria stated in the Plarm. Eur. and/or prescribed by the marketing approval. One intravenous immunoglobulin (IVIG) involved in TEEs exceeded a threshold level of 350 nmol peak thrombin, which was not exceeded after change of manufacture and by all the other IVIGs tested. Two hyperimmune globulins revealed elevated peak thrombin levels of up to 810 nmol in FXI and up to 285 nmol in FXIdp., Conclusion: The study indicates that the TGA is able to reliably predict procoagulant activities probably associated with the presence of FXIa and potential thrombogenicity. Comparison of thrombin generation with product-specific acceptance criteria as well as variables from other test systems as amidolytic activity and molecular size can help to monitor IgG quality and manufacturing changes with regard to thrombogenicity., (© 2013 American Association of Blood Banks.)

Published

2014

10. A new enzyme-linked immunosorbent assay recognizing both rat and human activated coagulation Factor XII (FXIIa).

Author

Papageorgiou PC, Yeo EL, Backx PH, and Floras JS

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal immunology, Base Sequence, Blotting, Western, Cardiovascular Diseases blood, Cardiovascular Diseases diagnosis, Epitopes immunology, Factor XIIa analysis, Humans, Male, Molecular Sequence Data, Rats, Antibodies, Monoclonal chemistry, Cardiovascular Diseases immunology, Enzyme-Linked Immunosorbent Assay methods, Factor XIIa immunology

Abstract

We describe the first sandwich enzyme-linked immunosorbent assay (ELISA) capable of recognizing both rat and human activated coagulation Factor XII (FXIIa). Increased plasma concentrations of FXIIa have been associated with adverse outcomes in several cardiovascular disease states. In humans, the FXIIa antigen in plasma is quantified by a direct sandwich ELISA employing an antibody (mAb 2/215) raised against its β-fragment (β-FXIIa), but this assay is unable to detect rat β-FXIIa antigen. Thus, experimental models are at present limited in their capacity to reveal mechanisms by which FXIIa might contribute to cardiovascular pathology. Consistent with overlap between human and rat FXIIa protein epitope sequences, Western blot analysis and ELISA demonstrate that another previously developed antibody against human FXIIa (mAb 201/9) detects β-FXIIa in both human and rat plasma, with no evidence for cross-reactivity with the FXII zymogen or FXIIa complexed with its endogenous inhibitor. The mAb 201/9 based ELISA identified similar elevations in FXIIa in plasma from rats and humans with chronic renal failure. The capacity of this ELISA to identify rat plasma FXIIa has potential application to a wide range of experimental models of human cardiovascular disease., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

11. Identification of kallikrein and FXIa as impurities in therapeutic immunoglobulins: implications for the safety and control of intravenous blood products.

Author

Etscheid M, Breitner-Ruddock S, Gross S, Hunfeld A, Seitz R, and Dodt J

Subjects

Blood Coagulation, Dose-Response Relationship, Drug, Drug Contamination, Drug-Related Side Effects and Adverse Reactions, Enzyme-Linked Immunosorbent Assay methods, Factor XIIa analysis, Fibrinolysin analysis, Humans, Immunoglobulins, Intravenous chemistry, Partial Thromboplastin Time, Prekallikrein analysis, Thrombin analysis, Thromboembolism immunology, Factor XIa analysis, Immunoglobulins chemistry, Immunoglobulins therapeutic use, Immunoglobulins, Intravenous therapeutic use, Kallikreins analysis

Abstract

Background and Objectives: The occurrence of thromboembolic events (TEEs) with intravenous immunoglobulin lots (IVIGs) raised the question of the causative agent for these adverse events. We investigated the predominant plasma proteases in 19 IVIG lots from five manufacturers including three lots associated with adverse events., Material and Methods: The inhibitor profile of the amidolytic activity in IVIG lots was investigated with substrates S-2302 and S-2288. In immunocapture assays, prekallikrein and FXI antigen and respective active proteases were quantified. Non-activated partial thromboplastin time (NAPTT) and a modified FXIa PTT served as global and FXIa-specific clotting assays, respectively., Results: Kallikrein was identified as one major contaminant activity in IVIGs. A second activity was seen in some IVIGs with substrate S-2288, but not with S-2302. Inhibition studies excluded FXIIa, thrombin or plasmin as contaminant activity. FXI antigen was seen in all 19 IVIG lots, and FXIa activity was found as second major impurity in some IVIGs, including all lots involved in TEEs. FXIa highly correlated with a short clotting time in NAPTT., Conclusions: Kallikrein and FXIa are the major contaminants in IVIGs. FXIa was highly procoagulant, with highest level in TEE-associated IVIGs. Since the NAPTT unambiguously identified FXIa procoagulant activity in IVIGs, its implementation as a release test would improve the safety of IVIGs., (© 2011 The Author(s). Vox Sanguinis © 2011 International Society of Blood Transfusion.)

Published

2012

12. A collaborative study to establish the 1st national standard of prekallikrein activator in Korea.

Author

Shin IS, Hong CM, Ban SJ, and Hong SH

Subjects

Calibration, Factor XIIa analysis, Factor XIIa chemistry, Female, Humans, Male, Reference Standards, Reproducibility of Results, Republic of Korea, Biological Assay standards, Factor XIIa standards

Abstract

The aim of this study was to establish the first national standard for prekallikrein activator (PKA) calibrating to the first international standard PKA. A collaborative study among five laboratories, including three manufacturers and two national control laboratories, was carried out to evaluate the suitability of a candidate to serve as a national standard of PKA. The candidate was manufactured in GMP facility following approved human serum albumin fractionation procedure and freeze-dried 5% albumin solution containing PKA. Participants were provided with sufficient samples and asked to use lab-made prekallikrein substrate prepared in accordance with European Pharmacopeia and also to use a commercial prekallikrein provided as part of the study. The PKA concentration of the candidate was 61.8 IU per vial using lab-made prekallikrein. However, the concentration was 54.2 IU per vial using commercial prekallikrein. The variability obtained at each laboratory ranged from 1.9% to 5.1% for within-a-day and from 5.6% to 9.0% for day-to-day. The candidate showed excellent stability from accelerated degradation study and real-time stability study. As a conclusion, the candidate preparation was suitable to serve as a Korean National Standard for PKA., (Copyright © 2011 The International Alliance for Biological Standardization. Published by Elsevier Ltd. All rights reserved.)

Published

2012

13. The effect of salt concentration on the prekallikrein activator assay.

Author

Georgakopoulos T, Bertolini J, and Hayes TK

Subjects

Biological Assay methods, Buffers, Dose-Response Relationship, Drug, Drug Contamination, Factor XIIa metabolism, Humans, Osmolar Concentration, Sensitivity and Specificity, Biological Assay standards, Factor XIIa analysis, Salts pharmacology

Published

2010

14. Activated factor XII type A and B-type natriuretic peptide are complementary and incremental predictors of mortality in patients following admission with acute coronary syndrome.

Author

Pönitz V, Brügger-Andersen T, Pritchard D, Grundt H, Staines H, and Nilsen DW

Subjects

Biomarkers blood, Mortality, Multivariate Analysis, Myocardial Infarction, Prospective Studies, Troponin T, Acute Coronary Syndrome diagnosis, Acute Coronary Syndrome mortality, Factor XIIa analysis, Natriuretic Peptide, Brain blood, Predictive Value of Tests

Abstract

The aim of this analysis was to assess the predictive value of activated factor XII type A (XIIaA) and B-type natriuretic peptide (BNP) in acute coronary syndrome patients stratified according to troponin release and to evaluate their complementary utility as predictors of all-cause mortality and recurrent troponin T (TnT)-positive events. Multivariable analysis in 870 patients admitted with suspected myocardial infarction was performed using the Cox proportional hazard ratio model. Variables in the model included XIIaA and BNP as well as conventional risk factors for mortality. Although both XIIaA and BNP were identified as independent predictors for all-cause mortality in the total group of patients, only BNP was found to be an independent predictor for all-cause mortality in patients with a confirmed myocardial infarction (TnT > 0.05 ng/ml) at admission (hazard ratio 4.24, 95% confidence interval 1.28-14.07), whereas only XIIaA was an independent predictor for all-cause mortality in patients with low TnT release (0.01 < TnT < or = 0.05 ng/ml) at admission (hazard ratio 10.37, 95% confidence interval 2.89-37.21). The combination of these two biomarkers provided complementary prognostic information for all-cause mortality as compared with each of the biomarkers alone in the total patient material. XIIaA is particularly useful in predicting mortality in acute coronary syndrome patients with low troponin release, whereas BNP is effective in predicting mortality in patients with confirmed myocardial infarction and more substantial troponin release. The combination of these two biomarkers improves outcome prediction in unselected patients with chest pain and acute coronary syndrome.

Published

2009

15. Adult cystic fibrosis patients with and without infective exacerbations and their factor XII levels.

Author

Davidson SJ, Paramothayan S, and Hodson ME

Subjects

Acute-Phase Proteins analysis, Adult, Antithrombin III analysis, Blood Coagulation Factors analysis, Cystic Fibrosis complications, Disease Susceptibility, Factor VIII analysis, Factor XII Deficiency blood, Factor XIIa analysis, Female, Fibrinogen analysis, Hemostasis, Humans, Inflammation blood, Inflammation complications, Interleukin-6 blood, Liver metabolism, Male, Cystic Fibrosis blood, Factor XII analysis, Factor XII Deficiency etiology, Infections complications

Abstract

We investigated haemostatic and inflammatory parameters in patients with cystic fibrosis in an attempt to understand a previous finding of low factor XII levels in this patient population. We selected two groups of patients, adults attending outpatient annual review clinic who were well, chronically inflammed and adult patients with an infective exacerbation requiring antibiotics or admission to hospital, acutely inflammed. We measured known positive acute phase haemostatic factors, fibrinogen and factor VIII. Antithrombin and factor XII were also measured as both these factors have been proposed to be negative acute phase proteins in in-vitro cell models. Interleukin-6 was also measured as the proposed modulator of these factors during inflammation. Activated factor XII was measured to exclude XII activation as a cause of the low XII activity levels. Cystic fibrosis patients admitted to hospital with infective exacerbations, showed significantly more evidence of inflammation than the annual review patients. Fibrinogen and factor VIII were higher and factor XII was lower in these patients. This work suggests that factor XII behaves as a negative acute phase protein with no signs of elevated activated XII levels in either group. This supports similar findings from in-vitro cell culture. This study also shows low antithrombin levels in both patient populations, although there was no statistical difference between groups, which is probably related to their liver disorder.

Published

2009

16. Activated factor XII type A predicts long-term mortality in patients admitted with chest pain.

Author

Pönitz V, Brügger-Andersen T, Pritchard D, Grundt H, Staines H, and Nilsen DW

Subjects

Aged, Female, Humans, Male, Middle Aged, Mortality, Prognosis, Proportional Hazards Models, Risk Factors, Survival Analysis, Survivors, Chest Pain mortality, Factor XIIa analysis, Predictive Value of Tests

Abstract

Background: We assessed the relation between admission levels of activated factor XII type A (XIIaA), and long-term all-cause and cardiac mortality and recurrent troponin T (TnT) positive cardiovascular events in a consecutive cohort of 870 patients admitted with a clinically strongly suspected acute coronary syndrome (ACS)., Methods and Results: After a 24-month follow-up period, 138 patients (15.8%) had died and 155 (17.8%) had suffered from a recurrent TnT positive (TnT > 0.05 ng mL(-1)) event. XIIaA levels were significantly lower in long-term survivors than in patients who died (22.9 (17.7-32.1) vs. 27.2 (20.0-39.7) pmol L(-1) [median, 25 and 75% percentiles], P < 0.001). The unadjusted hazard ratio for death within 2 years in patients with XIIaA in the highest quartile was 2.49 (95% confidence interval (CI), 1.52-4.06) as compared with patients with XIIaA in the lowest quartile. In a stepwise Cox regression model for death within 2 years, XIIaA added prognostic information for all-cause mortality (HR 2.05; 95% CI, 1.21-3.47) above and beyond age, a history of heart failure, ST-segment elevation, TnT and B-type natriuretic peptide (BNP). In the subgroup of patients with an admission TnT < or = 0.05 ng mL(-1), XIIaA provided independent prognostic information for all-cause mortality (HR 3.88; 95% CI, 1.66-9.08) and for the combined endpoint of death or recurrent TnT positive event (HR 2.46; 95% CI, 1.34-4.50)., Conclusion: XIIaA, a recently identified in vivo form of activated factor XII is an independent indicator of long-term all-cause mortality in patients admitted with chest pain, providing prognostic information above and beyond conventional risk factors.

Published

2009

17. Establishment of replacement batches for prekallikrein activator in albumin biological reference preparation.

Author

Lackner F, Daas A, Terao E, and Behr-Gross ME

Subjects

Chemistry, Pharmaceutical methods, Chemistry, Pharmaceutical standards, Humans, International Cooperation, Pharmacopoeias as Topic standards, Reference Standards, Serum Albumin analysis, Serum Albumin chemistry, Factor XIIa analysis, Factor XIIa standards, Serum Albumin standards

Abstract

A collaborative study was run by the European Directorate for the Quality of Medicines and HealthCare (EDQM) under the aegis of the Biological Standardisation Programme (BSP) to establish replacement batches of the current Prekallikrein activator in albumin Biological Reference Preparation (BRP) batch 1, the stocks of which were dwindling. Candidate BRP replacement batch 2 and batch 3 were assayed against the 2nd World Health Organization International Standard for Prekallikrein activator, human (2nd IS) and the Prekallikrein activator in albumin BRP batch 1. The candidate batches were manufactured from the same starting material as the current Biological Reference Preparation and the 2nd IS. They consisted of a 20 % solution of albumin lyophilised under the same conditions as the Prekallikrein activator in albumin BRP batch 1. Sixteen laboratories participated in the collaborative study and were requested to assay the candidates by their routine method, complying with the European Pharmacopoeia (Ph. Eur.) general method 2.6.15 for the determination of prekallikrein activator content. A central statistical analysis was performed at the EDQM using in-house calculations of prekallikrein activator contents provided by the participating laboratories. On the basis of the results of this study, which confirmed the assigned potency of 29 IU/vial of Prekallikrein activator in albumin BRP batch 1, the 2 candidate materials were assigned a potency of 30 IU/vial. The 2 candidates were adopted by the Ph. Eur. Commission in March 2008 as Ph. Eur. Prekallikrein activator in albumin Biological Reference Preparation batch 2 and batch 3.

Published

2008

18. Lower factor XII activity is a risk marker rather than a risk factor for cardiovascular disease: a rebuttal.

Author

Kanaji T

Subjects

Cardiovascular Diseases epidemiology, Case-Control Studies, Factor XII analysis, Factor XIIa analysis, Gene Frequency, Genetic Predisposition to Disease, Genotype, Humans, Hypercholesterolemia epidemiology, Hypertension epidemiology, Risk, Coronary Disease epidemiology, Factor XII physiology, Factor XII Deficiency epidemiology, Factor XIIa physiology, Polymorphism, Single Nucleotide

Published

2008

19. Coagulation factor XII (FXII) activity, activated FXII, distribution of FXII C46T gene polymorphism and coronary risk.

Author

Bach J, Endler G, Winkelmann BR, Boehm BO, Maerz W, Mannhalter C, and Hellstern P

Subjects

Aged, Cardiovascular Diseases epidemiology, Comorbidity, Factor XII analysis, Factor XII genetics, Factor XIIa analysis, Female, Follow-Up Studies, Gene Frequency, Genetic Predisposition to Disease, Genotype, Germany epidemiology, Humans, Hypercholesterolemia epidemiology, Hypertension epidemiology, Male, Middle Aged, Prospective Studies, Risk, White People genetics, Coronary Disease epidemiology, Factor XII physiology, Factor XII Deficiency epidemiology, Factor XIIa physiology, Polymorphism, Single Nucleotide

Abstract

Background: Whether factor XII (FXII) activity, its 46C>T polymorphism and activated FXII (FXIIa) are associated with coronary heart disease (CHD) remains to be determined., Methods: FXII, FXIIa and the FXII 46C>T polymorphism were determined in a hospital-based cohort of 2615 patients undergoing coronary angiography., Results: Fifty-seven per cent of the participants were identified as wild-type (46CC), 38% as heterozygous (46CT) and 5% as homozygous (46TT) for FXII 46C>T. FXII and FXIIa levels were significantly lower in carriers of the T-allele: 132 (97-151) U dL(-1) FXII in 46CC, 87 (77-99) U dL(-1) FXII in 46CT and 53 (42-67) U dL(-1) FXII in 46TT carriers (P < 0.001), and 2.8 (2.3-3.5) microg L(-1) FXIIa in CC, 2.1 (1.6-2.6) microg L(-1) FXIIa in CT and 1.2 (0.9-1.5) microg L(-1) FXIIa in TT carriers (P < 0.001; medians, lower and upper quartiles). Patients with stable CHD (n = 935), a history of myocardial infarction (n = 785) or who were suffering from acute coronary syndromes (ACS; n = 323) had significantly lower FXII levels than controls (n = 572). The differences remained statistically significant after adjustments for age, sex, diabetes mellitus, smoking, hypercholesterolemia and hypertension. Significantly reduced FXIIa levels in ACS patients lost significance once adjusted for covariates. FXII genotype was not associated with any clinical phenotype., Conclusion: Lower FXII activity represents an independent risk for CHD and ACS. This is not the case for FXIIa levels or the FXII 46C>T variation.

Published

2008

20. Impact of manufacturing improvements on clinical safety of albumin: Australian pharmacovigilance data for 1988-2005.

Author

Che Y, Wilson FJ, Bertolini J, Schiff P, and Maher DW

Subjects

Albumins adverse effects, Albumins chemistry, Australia, Factor XIIa analysis, Product Surveillance, Postmarketing, Retrospective Studies, Albumins standards

Abstract

Objective: To evaluate the impact of manufacturing improvements on the clinical safety of human albumin solutions in Australia., Methods: This retrospective study examined the incidence of spontaneously reported post-market adverse drug reactions (ADRs) in Australia associated with successive generations of albumin products manufactured by the Bioplasma Division of CSL Limited (CSL Bioplasma) over 18 years (1988-2005). Key characteristics of each product generation which could affect clinical safety, such as purity, aggregates and prekallikrein activator (PKA) levels, were also identified from CSL batch release records., Results: A total of 3.7 million bottles of iso-oncotic and hyperoncotic albumin products were distributed in Australia over the period. Improvements to manufacturing processes resulted in products with increased albumin purity, lower levels of impurities such as aggregates and PKA, and reduced batch-to-batch variation. The total ADR incidence (number of ADRs per 100 000 bottles distributed) associated with the products currently supplied was 1.5 and 1.7 for Albumex 4 (2VI) and Albumex 20 (2VI), respectively. This was a significant reduction compared with the earlier generation products Stable Plasma Protein Solution (14.1) and 20% Normal Serum Albumin (11.5), respectively (P<0.0001). In particular, hypotensive reactions declined substantially., Conclusion: Post-market pharmacovigilance data collected for successive generations of human albumin products supplied in Australia over 18 years indicates that manufacturing improvements have significantly improved the clinical safety profile of this product.

Published

2006

21. Specific types of activated Factor XII increase following thrombolytic therapy with tenecteplase.

Author

Pönitz V, Pritchard D, Grundt H, and Nilsen DW

Subjects

Aged, Enzyme-Linked Immunosorbent Assay methods, Factor XIIa analysis, Female, Humans, Male, Middle Aged, Myocardial Infarction blood, Tenecteplase, Factor XIIa drug effects, Fibrinolytic Agents pharmacology, Myocardial Infarction drug therapy, Thrombolytic Therapy, Tissue Plasminogen Activator pharmacology

Abstract

Background: Activated Factor XII (XIIa) is believed to participate in a number of pathophysiological processes including inflammation, thrombosis and fibrinolysis. Increasing XIIa levels following thrombolytic therapy have previously been reported. In contrast to other thrombolytics, tenecteplase (TNK-tpa) does not show paradoxical thrombin activation, indicating a lower procoagulant effect of this fibrin-selective thrombolytic agent. Recent research has demonstrated that in-vivo XIIa exists in a number of different types, and the aim of this study was to investigate plasma variations of different types of XIIa following thrombolytic treatment with TNK-tpa., Methods: Citrated blood samples were obtained from 34 patients admitted with acute ST-elevation myocardial infarction (STEMI) treated with TNK-tpa. Samples were taken immediately prior to treatment, 30-90 min after and 4 days post-treatment. XIIa measurements were performed using 2 ELISA assays designed to preferentially measure different types of XIIa; XIIaA and XIIaR. Both assays utilised a monoclonal antibody 2/215, which is highly specific for XIIa, as the solid phase capture antibody. The assay for XIIaA used a conjugate based on a polyclonal antibody against the entire XIIa molecule, whilst the assay for XIIaR incorporated a reagent to release otherwise unavailable XIIa and used a conjugate based on a monoclonal antibody against beta-XIIa., Results: Changes in plasma XIIaA concentration as a result of therapy were more evident than changes in XIIaR concentration. XIIaA showed a significant increase from 67.1 (49.0-84.4) pM to 97.8 (75.5-133.1) pM [median and 25 and 75% percentiles] in the 30-90 min sample (P < 0.001), returning to pre-intervention levels 61.5 (47.5-81.0) pM by day 4. In contrast, no significant change in XIIaR concentration was observed following thrombolytic therapy with TNK-tpa., Conclusion: In patients admitted with STEMI, thrombolytic therapy with TNK-tpa resulted in a significant short-lasting increase in specific types of XIIa (namely XIIaA), whereas other types of XIIa (XIIaR) were largely unaffected by this intervention.

Published

2006

22. Effect of varying the ratio of n-6 to n-3 fatty acids by increasing the dietary intake of alpha-linolenic acid, eicosapentaenoic and docosahexaenoic acid, or both on fibrinogen and clotting factors VII and XII in persons aged 45-70 y: the OPTILIP study.

Author

Sanders TA, Lewis F, Slaughter S, Griffin BA, Griffin M, Davies I, Millward DJ, Cooper JA, and Miller GJ

Subjects

Aged, Area Under Curve, Dietary Fats, Unsaturated administration & dosage, Dietary Fats, Unsaturated blood, Docosahexaenoic Acids administration & dosage, Docosahexaenoic Acids blood, Eicosapentaenoic Acid administration & dosage, Eicosapentaenoic Acid blood, Fasting blood, Fatty Acids, Omega-3 blood, Fatty Acids, Omega-6 blood, Female, Hemostasis drug effects, Humans, Male, Middle Aged, Myocardial Ischemia blood, Myocardial Ischemia epidemiology, Postprandial Period, Risk Factors, alpha-Linolenic Acid administration & dosage, alpha-Linolenic Acid blood, Factor VII analysis, Factor XIIa analysis, Fatty Acids, Omega-3 administration & dosage, Fatty Acids, Omega-6 administration & dosage, Fibrinogen analysis, Triglycerides blood

Abstract

Background: Elevated fibrinogen, activated factor XII (FXIIa), and factor VII coagulant activity (FVIIc) are associated with higher risk of fatal ischemic heart disease. This study tested the hypothesis that lowering the dietary ratio of n-6 to n-3 polyunsaturated fatty acids (n-6:n-3) would modify these risk factors in older men and women., Objective: The objective of the study was to measure fasting hemostatic risk factors and postprandial changes in activated FVII (FVIIa) concentrations after a 6-mo alteration in dietary n-6:n-3., Design: In a randomized, parallel design in 258 subjects aged 45-70 y, we compared 4 diets providing 6% of energy as polyunsaturated fatty acids at an n-6:n-3 between 5:1 and 3:1 with a control diet that had an n-6:n-3 of 10:1. The diets were enriched in alpha-linolenic acid, eicosapentaenoic (EPA) and docosahexaenoic (DHA) acid, or both., Results: Fasting and 3-h plasma triacylglycerol concentrations were 11.1% and 7.2% lower with the diet that had an n-6:n-3 of approximately 3:1 and that was enriched with EPA and DHA than with the other diets. Fasting fibrinogen, FXIIa, FVIIc, FVIIa, and FVII antigen and postprandial FVIIa were not influenced by the diets. Avoiding foods high in fat the day before measurement decreased FVIIc and FVIIa by 8% and 19.2%, respectively. A test meal containing 50 g fat resulted in a mean 47% (95% CI: 42%, 52%) increase in FVIIa 6 h later, but the response did not differ by n-6:n-3., Conclusion: Decreasing the n-6:n-3 to approximately 3:1 by increasing the intake of EPA and DHA lowers fasting and postprandial plasma triacylglycerol concentrations in older persons but does not influence hemostatic risk factors.

Published

2006

23. Effects on blood compatibility in vitro by combining a direct P2Y12 receptor inhibitor and heparin coating of stents.

Author

Christensen K, Larsson R, Emanuelsson H, Elgue G, and Larsson A

Subjects

Adenosine Monophosphate pharmacology, Analysis of Variance, Anticoagulants adverse effects, Anticoagulants pharmacology, Antithrombin III analysis, CD11b Antigen drug effects, Complement Activation drug effects, Drug Delivery Systems, Factor XIIa analysis, Factor XIa analysis, Flow Cytometry, Heparin administration & dosage, Heparin pharmacology, Humans, In Vitro Techniques, Membrane Proteins antagonists & inhibitors, Membrane Proteins drug effects, Peptide Hydrolases analysis, Platelet Activation physiology, Purinergic P2 Receptor Antagonists, Receptors, Purinergic P2 drug effects, Receptors, Purinergic P2Y12, Adenosine Monophosphate analogs & derivatives, Blood Platelets metabolism, CD11b Antigen metabolism, Platelet Activation drug effects, Platelet Aggregation Inhibitors pharmacology, Stents

Abstract

The effect of the direct platelet P2Y12 receptor inhibitor, AR-C69931MX, on activation of blood induced by stents with and without heparin coating was investigated using a whole blood Chandler loop model in vitro. Stents were deployed in Chandler loops. Fresh human blood with heparin and AR-C69931MX was rotated for 1 h at 37 degrees C and used for measurements of platelets, microparticles, thrombin-antithrombin complex (TAT), fibrinogen binding to platelets, P-selectin expression by platelets, CD11b, Prothrombin Fragment F1+2, FXIa-AT, FXIIa-AT, C3a, sC5b-9 and stent score. In the first experiment there were four study groups with unmodified stents: 1a, no AR-C69931MX; 1b, 250 nmol/L; 1c, 750 nmol/L; 1d, 2250 nmol/L of AR-C69931MX. In the second experiment the concentration of AR-C69931MX was 500 nmol/L: 2a; tubings without stent; 2b; tubings with heparin-coated stent; 2c; tubings with unmodified stents. Heparin-coated stents were used in the third experiment: 3a; no AR-C69931MX; 3b; 500 nmol/L of AR-C69931MX. In the first experiment there were significant differences in all parameters analysed except for C3a, and stent score when the group with no AR-C69931MX was compared to all the groups with AR-C69931MX. In the second experiment there were significant differences in platelet count, TAT, FXIa-AT, FXIIa-AT and stent score when unmodified stents were compared to loops with no stents and partly to loops with heparin-coated stents. In the third experiment there was a significant reduction in generation of TAT, stent score and better preservation of platelet number by combining the platelet inhibitor and heparin-coated stents as compared to heparin-coated stents alone. The conclusion is that the direct P2Y12 receptor inhibitor AR-C69931MX reduced the different aspects of activation of blood induced by both unmodified and heparin-coated stents.

Published

2006

24. Adhesion of thrombotic components to the surface of a clinically used oxygenator is not affected by Trillium coating.

Author

van den Goor JM, van Oeveren W, Rutten PM, Tijssen JG, and Eijsman L

Subjects

Aged, Elective Surgical Procedures, Female, Humans, Leukocyte Count, Male, Microscopy, Electron, Scanning, Middle Aged, Platelet Count, Surface Properties, Blood Platelets ultrastructure, Coated Materials, Biocompatible, Coronary Artery Bypass, Factor XIIa analysis, Fibrin analysis, Leukocytes ultrastructure, Oxygenators, Platelet Adhesiveness

Abstract

The Trillium coating is designed to minimize adsorption of protein and the attachment of cells and other particles. The present study was undertaken to investigate the effect of surface coating on the adhesion of thrombotic components (activated platelets, white blood cells and fibrin) to the surface of a clinically used oxygenator. Twenty patients undergoing elective coronary artery bypass grafting (CABG) were randomized to one of the two oxygenator groups: non-coated (NC, n = 10) or Trillium-coated (TC, n = 10). Platelet and white blood cell counts and factor XIIa concentrations were determined prior to the induction of anesthesia and at the end of cardiopulmonary bypass (CPB). Binding of activated platelets, white blood cells and fibrin to the artificial surfaces was quantified by means of antibody binding and histological validation was achieved by scanning electron microscopy. Patient demographic and CPB data were similar for the two groups. No significant differences between the groups were found for any of the tested thrombotic components. However, observations from our scanning electron microscopy suggested a release of formed particles from the Trillium-coated surface. Primary adhesion of activated platelets, white blood cells and fibrin to the artificial surface of the venous blood inlet from an oxygenator is not affected by the Trillium surface coating under conditions of full systemic heparinization.

Published

2006

25. Impaired bradykinin response to ischaemia and exercise in patients with mild congestive heart failure during angiotensin-converting enzyme treatment. Relationships with endothelial function, coagulation and inflammation.

Author

Cugno M, Agostoni P, Mari D, Meroni PL, Gregorini L, Bussotti M, Anguissola GB, Donatelli F, and Nussberger J

Subjects

Adult, Biomarkers blood, Blood Coagulation Factors analysis, Brachial Artery diagnostic imaging, Case-Control Studies, Endothelium, Vascular physiopathology, Factor XIIa analysis, Heart Failure physiopathology, Humans, Interleukin-6 blood, Ischemia physiopathology, Male, Middle Aged, Receptors, Tumor Necrosis Factor, Type II blood, Tissue Plasminogen Activator analysis, Ultrasonography, Vasodilation, von Willebrand Factor analysis, Angiotensin-Converting Enzyme Inhibitors therapeutic use, Bradykinin blood, Exercise, Heart Failure blood, Heart Failure drug therapy, Lisinopril therapeutic use

Abstract

Inflammation and endothelial dysfunction play important roles in the pathophysiology of congestive heart failure (CHF), and the peptide bradykinin, generated during inflammation, may act as a defence mechanism by inducing vasodilation. Plasma bradykinin levels are increased in experimental heart failure but low in patients with advanced chronic CHF despite treatment with angiotensin-converting enzyme (ACE) inhibitors. It is not currently known how bradykinin behaves in less severe phases of CHF controlled by long-term ACE inhibitor treatment. We studied 10 male patients with clinically stable chronic CHF [New York Heart Association (NYHA) class II] on long-term ACE inhibitor treatment and 10 normal sex- and age-matched control subjects. High performance liquid chromatography/radioimmunoassay methods were used to evaluate plasma levels of bradykinin in relation to an array of parameters of endothelial function, coagulation and inflammation before and after stimuli of forearm arterial occlusion and physical exercise. CHF patients had higher levels of bradykinin (P = 0.008), activated factor XII (P = 0.049), interleukin-6 (P = 0.050) and tumour necrosis factor receptor II (sTNFRII) (P = 0.026) than controls. Arterial occlusion and exercise significantly increased bradykinin and von Willebrand factor levels in controls but not in CHF patients. The increase in brachial artery diameter after arterial occlusion was less in CHF patients (P = 0.036) and inversely related to baseline plasma levels of bradykinin (r = -0.855, P = 0.002) and sTNFRII (r = -0.780, P = 0.008). NYHA class II CHF patients during long-term treatment with ACE inhibitors have increased bradykinin levels and signs of inflammation. They are unable to respond adequately to stimuli of ischaemia and physical exercise which both require vasodilation.

Published

2005

26. Acute coronary syndromes do not promote prolonged in vivo FXII-dependent prothrombotic activity.

Author

Altieri P, Devoto E, Spallarossa P, Rossettin P, Garibaldi S, Bertero G, Balbi M, Barsotti A, Brunelli C, and Ghigliotti G

Subjects

Acute Disease, Adolescent, Adult, Aged, Aged, 80 and over, Angina Pectoris blood, Case-Control Studies, Coronary Artery Disease blood, Humans, Middle Aged, Myocardial Infarction blood, Risk Factors, Triglycerides blood, Coronary Disease blood, Factor XIIa analysis, Thrombophilia etiology

Abstract

Background: Coagulation FXII is activated on contact with lipoprotein particles. It has been suggested that contact with subendothelial tissue provides an alternative biological surface for FXII activation. Our aim was to investigate whether activated FXII (FXIIa) is elevated in patients with coronary atherosclerosis, and whether disease status (acute phase or stable state) affects circulating levels of FXIIa., Methods: Circulating FXIIa levels were measured in the peripheral blood of 122 patients with coronary atherosclerosis (32, stable angina; 54, unstable angina; 36, nQ myocardial infarction) and in 45 age-matched subjects (Contr)., Results: FXIIa levels (median, first and third quartiles; ng/ml) were higher in patients than in Contr: 1.61 (1.26-2.02) vs. 1.34 (1.13-1.81) (p<0.01). FXIIa levels were similar among patients with stable angina [1.66 (1.23-1.91)], unstable angina [1.53 (1.21-2.04)], and nQ myocardial infarction [1.75 (1.34-2.03)]. The three groups of patients had similar prevalence for most atherothrombotic risk factors; patients with stable angina had an increased severity of coronary disease, which did not explain the different levels of FXIIa. Fasting levels of triglycerides were the best predictor of FXIIa levels in our patients., Conclusions: The finding of similar FXIIa levels among patients in either acute or chronic phases of coronary atherosclerosis suggests that the initial arterial denudation and the acute-phase response associated to acute coronary syndromes are not major determinants for prolonged FXII activation.

Published

2005

27. [Activated factor XII in patients with hyperglycaemia and dyslipidaemia].

Author

Průsa R, Zadina J, and Bronský J

Subjects

Adolescent, Adult, Aged, Arteriosclerosis blood, Child, Diabetes Complications, Female, Humans, Hyperlipidemias drug therapy, Male, Middle Aged, Risk Factors, Diabetes Mellitus blood, Factor XIIa analysis, Hyperglycemia blood, Hyperlipidemias blood

Abstract

Background: Increased plasma levels of activated factor FXII (FXIIa) are associated with increased risk of atherosclerosis and coronary heart disease. There are increased levels of FXIIa in patients with dyslipidaemia and also elevated levels of FXIIa have been reported in patients with diabetes mellitus. No studies were reported whether FXIIa correlates rather with plasma glucose levels or with other metabolic markers like hypertriacylglycerolemia., Methods: We measured plasma FXIIa levels, triacylglycerols, uric acid and glucose in a group of 158 hyperglycaemic patients with P-glucose more than 8 mmol/l and variable serum lipid parameters [cholesterol, triacylglycerols, HDL-cholesterol, LDL-cholesterol, lipoprotein (a), apolipoprotein AI, apolipoprotein B] in a group of 55 patients of lipid clinic on hypolipidaemic treatment (statins, fibrates)., Results and Conclusion: The comparison of FXIIa with the age in the group of hyperglycaemic patients has shown that the number of patients with FXIIa more than 2.5 microg/l is growing with increasing age. Low concentration of FXIIa was observed in the youngest age group (10-30 years), where all values are within the reference ranges. We proved positive correlation between plasma FXIIa levels and age, triacylglycerols, uric acid. No correlation was found between plasma FXIIa and glucose in both groups.

Published

2004

28. Interleukin-6, fibrin D-dimer, and coagulation factors VII and XIIa in prediction of coronary heart disease.

Author

Lowe GD, Rumley A, McMahon AD, Ford I, O'Reilly DS, and Packard CJ

Subjects

Angioplasty, Balloon, Coronary statistics & numerical data, Biomarkers, Case-Control Studies, Coronary Disease epidemiology, Fibrinogen analysis, Humans, Hydroxymethylglutaryl-CoA Reductase Inhibitors therapeutic use, Hypercholesterolemia blood, Hypercholesterolemia drug therapy, Hypercholesterolemia epidemiology, Hypertension epidemiology, Incidence, Inflammation, Interleukin-6 metabolism, Male, Middle Aged, Monocytes metabolism, Myocardial Infarction epidemiology, Myocardial Revascularization statistics & numerical data, Pravastatin therapeutic use, Predictive Value of Tests, Risk Factors, Scotland epidemiology, Thrombophilia epidemiology, Triglycerides blood, Coronary Disease blood, Factor VII analysis, Factor XIIa analysis, Fibrin Fibrinogen Degradation Products analysis, Interleukin-6 blood

Abstract

Objective: Activated inflammation and activated blood coagulation are believed to increase the risk of coronary thrombosis and are related. We therefore compared plasma IL-6 (a key cytokine in the inflammatory process), fibrin D-dimer (a marker of fibrin turnover), and coagulation factors VII and XIIa (initiators of extrinsic and intrinsic blood coagulation, respectively) as predictors of coronary risk in the West of Scotland Coronary Prevention Study of pravastatin in men with hypercholesterolemia., Methods and Results: 485 men who had had a coronary event (nonfatal myocardial infarction, death from coronary heart disease, or revascularization) were matched for age and smoking status with 934 controls. Baseline IL-6 and D-dimer were strong univariate predictors of coronary risk (relative risk in the highest quintile approximately twice that in the lowest quintile) and were associated with each other and with C-reactive protein. On multivariate analyses, D-dimer retained a significant association with coronary risk (relative risk, 1.86; 95% CI, 1.24 to 2.80), whereas IL-6 (1.47; 0.95 to 2.28) and C-reactive protein (1.33; 0.85 to 2.08) did not. Neither factor VII nor factor XIIa antigens were predictors of coronary events., Conclusions: Fibrin D-dimer may be a stronger predictor of coronary risk than inflammatory markers, perhaps through its ability to stimulate monocyte release of IL-6.

Published

2004

29. Activated factor 12 (FXIIa) predicts recurrent coronary events after an acute myocardial infarction.

Author

Grundt H, Nilsen DW, Hetland Ø, Valente E, and Fagertun HE

Subjects

Angina, Unstable blood, Angina, Unstable epidemiology, Biomarkers blood, C-Reactive Protein analysis, Female, Fibrin Fibrinogen Degradation Products analysis, Humans, Male, Prognosis, Proportional Hazards Models, Prospective Studies, Recurrence, Risk Factors, Troponin T blood, Factor XIIa analysis, Myocardial Infarction blood

Abstract

Background: Activated factor XII (FXIIa) is involved in vascular injury and repair, participating in inflammation, thrombosis, and fibrinolysis. We wanted to test the hypothesis that FXIIa may predict an acute coronary syndrome (ACS) after a myocardial infarction (MI) and to evaluate whether FXIIa is related to global markers of end-stage coagulation and inflammation, including fibrin monomer (FM) and ultrasensitive C-reactive protein (microCRP)., Methods: In a prospective study of 300 patients with acute MI, we evaluated the predictive value of FXIIa in blood samples drawn 4 to 6 days after admission. Cardiac death, re-MI, and troponin-T-positive unstable angina pectoris were registered during a median follow-up period of 1.5 years., Results: In the upper quartile of FXIIa (Q4) (> or =2.23 ng/mL) 32.0% of patients had an ACS as compared with 16.9% of patients with FXIIa in the three lower quartiles (Q1-3, P =.008). Relative risk of recurrent ACS for patients with FXIIa in the Q4 as compared with Q1-3 was 1.89 (95% CI, 1.22 to 2.93). A secondary ACS occurred earlier in patients with FXIIa in the Q4 as compared with those with FXIIa in the Q1-3 (P =.0039). Conventional risk factors as potential confounders were not associated with time to event. FXIIa did not correlate with FM or microCRP, and the FM and microCRP levels were of a similar magnitude in the Q4 as compared with the Q1 and the Q1-3 of FXIIa., Conclusions: FXIIa predicts recurrent coronary events after MI. The prognostic ability of FXIIa was not reflected by markers of hypercoagulability or inflammation.

Published

2004

30. Activated factor XII in rheumatoid arthritis.

Author

McLaren M, Alkaabi J, Connacher M, Belch JJ, and Valenete E

Subjects

Adult, Aged, Arthritis, Rheumatoid complications, Arthritis, Rheumatoid diagnosis, Biomarkers analysis, Case-Control Studies, Coronary Disease physiopathology, Enzyme-Linked Immunosorbent Assay, Factor XIIa analysis, Female, Humans, Male, Middle Aged, Probability, Prognosis, Reference Values, Rheumatoid Factor analysis, Risk Assessment, Sensitivity and Specificity, Severity of Illness Index, Statistics, Nonparametric, Arthritis, Rheumatoid blood, Coronary Disease etiology, Factor XIIa metabolism

Abstract

Rheumatoid arthritis (RA) is associated with premature mortality, with approximately 50% of deaths being due to cardiovascular disease. It has been shown that the increased incidence of cardiovascular disease is independent of traditional risk factors. Previous studies have shown an increased risk of coronary heart disease with increased levels of activated factor XII (FXIIa). The aim of this study was to investigate levels of FXIIa in patients with RA. We studied 32 patients with RA and 30 age- and sex-matched control subjects. We found FXIIa levels significantly increased in the patient group, with 56% of the patients and 6.7% of controls having levels greater than or equal to 2 ng/ml. A previous study has shown that individuals with levels of 2 ng/ml or more have an increased risk of coronary heart disease. Measurement of FXIIa could perhaps help to identify an 'at risk' group of patients, allowing early intervention therapy.

Published

2002

31. Juvenile xanthogranuloma of the oral cavity in children: a clinicopathologic study.

Author

Flaitz C, Allen C, Neville B, and Hicks J

Subjects

Antigens, CD analysis, Antigens, Differentiation, Myelomonocytic analysis, Carrier Proteins analysis, Child, Child, Preschool, Diagnosis, Differential, Factor XIIa analysis, Female, Histiocytosis, Langerhans-Cell diagnosis, Humans, Immunohistochemistry, Infant, Male, Microfilament Proteins analysis, S100 Proteins analysis, alpha 1-Antitrypsin analysis, Mouth Diseases pathology, Xanthogranuloma, Juvenile pathology

Abstract

Purpose: This clinicopathologic study describes the histopathologic, immunocytochemical, and electron microscopic features of oral juvenile xanthogranuloma (JXG) in children., Design: The study population consisted of 5 children (5 months to 10 years of age) with biopsy-proven JXGs obtained for consultation., Results: Lesion sites were gingiva, buccal mucosa, and tongue and were described by the clinicians as (1). irritation fibroma; (2). granulation tissue; (3). pedunculated granular nodule; (4). papilloma-like lesion; and (5). brown-red umbilicated papule. Tissue was available for histopathologic (n = 5), immunocytochemical (n = 5), and ultrastructural (n = 3) studies. Three cases showed early JXG lesions possessing abundant histiocytes, but lacking Touton giant cells. The other 2 cases had classic JXG lesions with vacuolated histiocytes and Touton giant cells. Immunocytochemical findings were (1). CD68 (KP1, PGM1), moderate to diffuse; (2). fascin, moderate to diffuse; (3). factor XIIIa, focal to diffuse; (4). alpha-1-antitrypsin, moderate to diffuse; (5). S-100 protein, focal to diffuse; and (6). CD1a, negative in all cases. Ultrastructural examination displayed histiocytic and dendritic cells lacking pentalaminar structures (Birbeck granules)., Conclusion: JXGs of the oral cavity vary in their clinical and histopathologic appearances and necessitate that Langerhans' cell disease (LCD) be excluded. JXG and Langerhans' cell disease may occur concurrently, before or after each other, in some children.

Published

2002

32. An improved, reliable and practical kinetic assay for the detection of prekallikrein activator in blood products.

Author

Shin IS, Shim YB, Hong CM, Koh HC, Lee SH, and Hong SH

Subjects

Amidohydrolases analysis, Blood Chemical Analysis, Dose-Response Relationship, Drug, Humans, Hydrogen-Ion Concentration, Indicators and Reagents, Kinetics, Reference Standards, Reproducibility of Results, Sodium Chloride, Factor XIIa analysis

Abstract

An improved kinetic assay for prekallikrein activator (PKA), a potential vasodilator, has been developed to be used as an indicator for quality control during production of human albumin preparations. It consists of two reaction stages. In the first stage, PKA and prekallikrein are incubated at 37 degrees C for 45 min to allow the transformation into kallikrein. Kallikrein, a serine protease, catalyzes the splitting of p-nitroaniline (pNA) from its substrate H-D-Pro-Phe-Arg-pNA (S-2302). The rate at which pNA is released was measured spectrophotometrically at 405 nm. Prekallikrein, a substrate of PKA was purified by DEAE ion-exchange chromatography and the major potential variations in the assay were optimized; pH 8.0 and 150 mM sodium chloride were chosen to give a proper ionic strength. Reaction times in the range of 10 to 360 min provided linear dose-response curves. The concentration of prekallikrein was adjusted to fall between 1:1 and 1:3 dilutions to generate a linear standard calibration curve. Under the optimized conditions, reproducibility was checked. In a precision test, the coefficient of variation (CV) stayed within +/-4% and the dose-response curve showed a good correlation (r2=0.999). An accuracy test with an international standard of PKA afforded a mean recovery of 97.5%.

Published

2002

33. Activated factor XII levels and factor XII 46C>T genotype in relation to coronary artery calcification in patients with type 1 diabetes and healthy subjects.

Author

Colhoun HM, Zito F, Norman Chan N, Rubens MB, Fuller JH, and Humphries SE

Subjects

Adult, Biomarkers analysis, Coronary Artery Disease etiology, Diabetes Mellitus, Type 1 complications, Endothelium, Vascular physiopathology, Factor XIIa analysis, Factor XIIa metabolism, Female, Humans, Male, Nitric Oxide metabolism, Polymorphism, Genetic, Random Allocation, Risk, Calcinosis etiology, Coronary Disease etiology, Diabetes Mellitus, Type 1 metabolism, Factor XIIa genetics, Genotype

Abstract

The relationship of activated factor XII (FXIIa) and FXII 46C>T genotype to coronary atherosclerosis and endothelial function was examined in 192 randomly sampled subjects from the general population and 190 type 1 diabetic subjects (mean age 38+/-4 years). Coronary artery calcification (CAC) was measured using Electron beam CT. von Willebrand factor (vWF), a marker of endothelial function, and FXIIa were measured by ELISA. Endothelial nitric oxide production was quantified as the forearm blood flow response to intra-brachial infusion of bradykinin and N(G) monomethyl-L-arginine (L-NMMA). A higher FXIIa was independently associated with higher triglycerides (P<0.001), BMI (P=0.001), alcohol consumption (P=0.003) and vWF (P<0.001) in non-diabetic subjects and with insulin dose (P=0.009), total cholesterol (P=0.02) and alcohol (P<0.001) in diabetic subjects. Diabetic subjects had lower FXIIa (1.55 ng/ml) than non-diabetic subjects (1.92 ng/ml, P<0.001). Higher FXIIa was associated with lower response to bradykinin (P=0.048) and to L-NMMA (P=0.029). FXIIa was positively associated with CAC (odds ratio=1.57 for every 1 ng/ml higher FXIIa, P=0.005) but not independently of other risk factors (odds ratio=1.1 on adjustment). 46C>T genotype explained 18% of the variance in FXIIa (P<0.001) but was not associated with CAC (P=0.6). We conclude that plasma FXIIa is under strong genetic control but also reflects plasma triglycerides and endothelial activation or dysfunction. FXIIa appears unlikely to be directly atherogenic but may be a useful marker of coronary atherosclerosis because of its association with these other factors. Type 1 diabetes is associated with lower levels of FXIIa despite a greater prevalence of atherosclerosis.

Published

2002

34. Plasma markers of hypercoagulability in patients with serious infections and risk of septic shock.

Author

Psuja P, Zozulińska M, Turowiecka Z, Cieślikowski W, Vinazzer H, and Zawilska K

Subjects

Adult, Aged, Aged, 80 and over, Antithrombin III, Bacterial Infections blood, Biomarkers blood, Blood Coagulation Tests, Factor XIIa analysis, Female, Fibrin Fibrinogen Degradation Products analysis, Humans, Male, Middle Aged, Peptide Fragments blood, Peptide Hydrolases blood, Prothrombin, Risk Factors, Shock, Septic etiology, Bacterial Infections complications, Thrombophilia diagnosis, Thrombophilia etiology

Abstract

Hyperthrombinogenesis due to bacterial septicemia may aggravate the risk of irreversible septic shock. In 22 patients with septicemia complicating urinary or alimentary infections, daily assessment of hemostasis was performed throughout 1 week. Standard screening of hemostasis revealed significantly increased mean values of prothrombin time, fibrinogen, and fibrinogen degradation product (FDP) concentration. However, platelet counts, activated partial thromboplastin times (APTT), thrombin times, ethanol gelation tests, and antithrombin activity remained within the normal range. By contrast, except for insignificant changes in protein C activity and activated factor VII content, specific markers of plasma hypercoagulability, that is, thrombin-antithrombin (TAT) complexes, prothrombin activating factor F 1+2, activated factor XII (XIIa), and dimer D were all markedly increased. Pathologic levels of TAT and Xlla were found in 82% and 73% of all plasma samples, respectively. The augmentation of TAT correlated with prolongation of thrombin time and increases in F 1+2 levels. The increase in XIIa correlated with thrombocytopenia, prolongation of APTT, exhaustion of antithrombin, and accumulation of F 1+2 and FDP in the plasma. Moreover, a significant increase in XIIa, stronger positivity of the ethanol gelation test, a greater increase in FDP, and a more pronounced decrease in protein C activity were observed in 8 patients with fatal septic shock. This study suggests the usefulness of TAT and XIIa measurements in the early recognition of plasma hypercoagulation in serious infections.

Published

2002

35. C1 inhibitor infusion modifies platelet activity in hereditary angioedema patients.

Author

Coppola L, Guastafierro S, Verrazzo G, Coppola A, De Lucia D, and Tirelli A

Subjects

Adenosine Diphosphate pharmacology, Adolescent, Adult, Angioedema blood, Angioedema genetics, Blood Platelets chemistry, Blood Platelets drug effects, Collagen pharmacology, Complement C1 Inactivator Proteins administration & dosage, Complement C1 Inactivator Proteins pharmacokinetics, Complement C1 Inhibitor Protein, Dose-Response Relationship, Drug, Factor XIIa analysis, Female, Humans, Infusions, Intravenous, Male, Middle Aged, Peptide Fragments blood, Platelet Aggregation drug effects, Prothrombin, Angioedema drug therapy, Blood Platelets metabolism, Complement C1 Inactivator Proteins therapeutic use

Abstract

Context: C1 inhibitor (C1-INH) is an alpha2-globulin that blocks esterolytic activity of the first component of the classic complement cascade. The alpha-granules of normal human platelets also contain C1-INH, which is expressed on the platelet surface during platelet secretion in healthy patients, but it is clearly reduced in patients with hereditary angioedema (HAE)., Objective: To evaluate the effects of in vivo C1-INH concentrate infusion on platelet responsiveness and coagulation system activity in patients with HAE., Design: Assessment of the platelet activity and plasma levels of C1-INH, activated factor XII (XIIa), and prothrombin fragment F1.2 (F1.2) before and after infusion of 15 U/kg of C1-INH concentrate., Patients: In 6 patients (4 men and 2 women), HAE was diagnosed according to the accepted clinical and laboratory criteria., Measurements: Platelet aggregation (final concentrations: adenosine diphosphate, 0.5, 1.25, and 2.5 microM; collagen, 5 microg/mL), C1-INH antigen (radial immunodiffusion), C1-INH activity (chromogenic substrates), and XIIa and F1.2 (enzyme-linked immunosorbent assay)., Results: After C1-INH infusion, we observed a prompt increase of C1-INH level and a slow return toward its plasma preinfusion values within 4 to 7 days, a significant decrease of both adenosine diphosphate- and collagen-induced platelet aggregation versus preinfusion values (maximum after 1-2 days; P <.001), and a rapid decrease of high basal values of XIIa and F1.2 in 30 and 120 minutes, respectively., Conclusions: These data show a role of C1-INH in the control of platelet activity and that its deficiency increases platelet aggregability and plasma levels of XIIa and F1.2 in patients with HAE.

Published

2002

36. Absence of paradoxical thrombin activation by fibrin-specific thrombolytics in acute myocardial infarction: comparison of single-bolus tenecteplase and front-loaded alteplase.

Author

Szabo S, Letsch R, Ehlers R, Walter T, Kazmaier S, Helber U, and Hoffmeister HM

Subjects

Aged, Anticoagulants administration & dosage, Anticoagulants therapeutic use, Antifibrinolytic Agents blood, Antithrombin III analysis, Aspirin administration & dosage, Aspirin therapeutic use, Biomarkers, Enzyme Activation drug effects, Factor XIIa analysis, Female, Fibrin Fibrinogen Degradation Products analysis, Fibrinolysin, Fibrinolysis drug effects, Hemostasis drug effects, Heparin administration & dosage, Heparin therapeutic use, Humans, Male, Middle Aged, Myocardial Infarction drug therapy, Peptide Fragments blood, Platelet Aggregation Inhibitors administration & dosage, Platelet Aggregation Inhibitors therapeutic use, Prothrombin, Recombinant Proteins administration & dosage, Recombinant Proteins pharmacology, Recombinant Proteins therapeutic use, Substrate Specificity, Tenecteplase, Tissue Plasminogen Activator administration & dosage, Tissue Plasminogen Activator blood, Tissue Plasminogen Activator therapeutic use, alpha-2-Antiplasmin, Fibrin drug effects, Fibrinolytic Agents pharmacology, Myocardial Infarction blood, Thrombin drug effects, Thrombolytic Therapy, Tissue Plasminogen Activator pharmacology

Abstract

Objectives: Thrombolytic therapy in patients with acute myocardial infarction is hampered by bleeding complications and procoagulant effects favoring early reocclusion. TNK-tPA was shown in vitro to have considerable fibrin specificity. We investigated the effects of tenecteplase (TNK-tPA) and alteplase (rt-PA) on the haemostasis and fibrinolytic system., Methods and Results: We enrolled 30 patients with AMI into the study. Twenty patients received front-loaded rt-PA up to 100 mg; 10 patients were given TNK-tPA in a single bolus up to 50 mg. All patients received aspirin and intravenous heparin. During the first 2 days, the following parameters were repetitively determined: thrombin-antithrombin III complexes (TAT), antithrombin III (ATIII), prothrombin fragment F 1 + 2 (F 1 + 2), kallikrein-like activity (KK), activated factor XII (FXIIa), plasmin alpha 2-antiplasmin complexes (PAP), fibrinogen, D-dimers (DD), tissue-type plasminogen activator (t-PA). A total of 75 healthy persons served as control group. TAT increased significantly after rt-PA but not after TNK-tPA (3 h: 38.1 +/- 29.4 versus 10.5 +/- 4.2 microg/l; p < 0.01), indicating paradoxical thrombin activation. F 1 + 2 increased transiently after rt-PA but not after TNK-tPA. Fibrinogen was significantly lower after rt-PA versus TNK-tPA (3 h: 163 +/- 27 versus 380 +/- 54 mg/dl; p < 0.05). KK activities in the rt-PA group were significantly (p < 0.01) increased over 48 h versus TNK-tPA. PAP and D-dimers were lower over the time course of 48 h in the tenecteplase group versus rt-PA., Conclusions: This study indicates that tenecteplase has higher fibrin specificity not only in vitro but also in vivo versus alteplase. TNK-tPA consecutively has no paradoxical systemic procoagulant effect due to the lower extent of activation of the kallikrein-factor XII system than alteplase., (Copyright 2002 Elsevier Science Ltd.)

Published

2002

37. Bradykinin in the ascitic fluid of patients with liver cirrhosis.

Author

Cugno M, Salerno F, Nussberger J, Bottasso B, Lorenzano E, and Agostoni A

Subjects

Adult, Aged, Electrophoresis, Polyacrylamide Gel, Factor XIIa analysis, Female, Fibrinolysin analysis, Humans, Immunoblotting, Kininogens analysis, Liver Cirrhosis blood, Male, Middle Aged, Peptide Fragments analysis, Renin blood, Serum Albumin analysis, alpha-2-Antiplasmin analysis, Ascitic Fluid chemistry, Bradykinin analysis, Liver Cirrhosis metabolism

Abstract

Bradykinin, a nonapeptide with vasodilatory and permeabilizing activity, is generated through the cleavage of high-M(r) ('high-molecular-weight') kininogen by kallikrein, and its generation is facilitated by plasmin. In the ascitic fluid of patients with cirrhosis, there is massive cleavage of high-M(r) kininogen and activation of fibrinolysis, but bradykinin has never been measured directly. In the ascitic fluid of 24 patients with cirrhosis, we measured bradykinin-(1-9)-nonapeptide levels by RIA after liquid-phase and subsequent HPLC extraction, and those of its catabolic product bradykininin-(1-5)-pentapeptide by ELISA after liquid-phase extraction. Cleaved high-M(r) kininogen, activated factor XII and plasmin-antiplasmin complexes were measured in ascitic fluid and plasma. Plasma renin activity (PRA) was also determined. As a control, we also analysed plasma from 24 healthy subjects matched for sex and age with the patients. In the ascitic fluid from patients with cirrhosis, the median bradykinin-(1-9) concentration was 3.3 fmol/ml (range 0.2-29.0 fmol/ml), and the median bradykinin-(1-5) concentration was 210 fmol/ml (range 58-7825 fmol/ml). The levels of bradykinin-(1-5) in ascitic fluid were higher in patients with refractory ascites [median 1091 fmol/ml (range 58-7825 fmol/ml)] than in patients with responsive ascites [134 fmol/ml (72-1084 fmol/ml)] (P=0.010). Ascitic fluid levels of bradykinin-(1-9) were not related to the severity of ascites. PRA was higher in patients with refractory ascites [23.0 ng x h(-1) x ml(-1) (7.9-80.0 ng.h(-1).ml(-1))] than in patients with responsive ascites [6.9 ng x h(-1) x ml(-1) (0.9-29.4 ng x h(-1) x ml(-1))] (P=0.002). In ascitic fluid, 48% (19-68%) of high-M(r) kininogen was cleaved, and plasmin-antiplasmin complexes were more concentrated than in plasma (P=0.0001). In conclusion, in the ascitic fluid of patients with cirrhosis, both bradykinin-(1-9) and bradykinin-(1-5) are present, with cleavage of high-M(r) kininogen and activation of fibrinolysis. The highest levels of the long-lived metabolite bradykinin-(1-5) were found in the ascitic fluid of patients with refractory ascites and high PRA. Activation of the kinin system may therefore be involved in decompensating cirrhosis, but a cause-effect relationship remains to be established.

Published

2001

38. Plasma levels of factor XIIa and factor VIIa are increased but not related in primary hyperlipidaemia.

Author

Cardigan RA, Crook M, Mackie IJ, and Machin SJ

Subjects

Adult, Aged, Aged, 80 and over, Antithrombin III analysis, Enzyme Activation, Fasting blood, Female, Humans, Hypercholesterolemia blood, Hypercholesterolemia complications, Hypertriglyceridemia blood, Hypertriglyceridemia complications, Lipolysis, Lipoproteins blood, Male, Middle Aged, Peptide Fragments analysis, Peptide Hydrolases analysis, Prothrombin analysis, Thrombin biosynthesis, Thrombophilia blood, Thrombophilia etiology, Triglycerides blood, Factor VIIa analysis, Factor XIIa analysis, Hyperlipidemias blood

Abstract

The lipolysis of triglyceride-rich lipoproteins may provide a surface that supports the activation of factor XII (FXII) with subsequent activation of factor VII (FVII). Plasma levels of activated FVII (FVIIa) but not activated FXII (FXIIa) are increased in the post-prandial state when there is a transient increase in triglyceride levels. We compared plasma levels of FXIIa antigen in control subjects (n = 33) and in patients with chronically elevated lipids (primary hyperlipidaemia, n = 49), with FVIIa and markers of thrombin generation. Results are given as median (first and third quartiles). Plasma levels of FXIIa [2.34 (1.68-3.32) ng/ml versus 1.53 (0.93-1.86) ng/ml, P = 0.0002], FVIIa [3.02 (2.15-4.64) ng/ml versus 2.20 (1.66-2.56) ng/ml, P = 0.0004], thrombin-antithrombin complexes [3.08 (2.16-5.54) microg/I versus 2.13 (1.46-2.84) microg/l, P = 0.005] and prothrombin fragment 1 + 2 (Pro F1 + 2) [1.28 (1.08-1.50) nmol/l versus 0.92 (0.65-1.08) nmol/l, P = 0.0001] were increased compared with controls irrespective of the type of hyperlipidaemia. In hyperlipdaemic subjects, levels of Pro F1 + 2 were correlated with FVIIa (r = 0.56, P = 0.0002) and FXIIa (r = 0.31, P = 0.03). These results suggest increased activation of both FVII and FXII in hyperlipidaemic subjects, which correlates with increased thrombin generation. Given the lack of correlation between levels of FXIIa and FVIIa, it remains to be established whether the increase in FXIIa is responsible for increased FVIIa activity in this subject group.

Published

2001

39. A potentially improved approach to methylene blue virus inactivation of plasma: the Maco Pharma Maco-Tronic system.

Author

Hornsey VS, Drummond O, Young D, Docherty A, and Prowse CV

Subjects

Antithrombin III analysis, Blood Coagulation Factors analysis, Blood Transfusion standards, Complement C3a analysis, Complement C5a analysis, Factor XIIa analysis, Fibrinogen analysis, Humans, Leukocyte Count, Light, Platelet Count, PrPC Proteins blood, Viruses growth & development, Blood virology, Methylene Blue pharmacology, Viruses drug effects

Abstract

Plasma was subjected to methylene blue (MB) photochemical virus inactivation using the Maco Pharma Maco-Tronic system which allows three units to be illuminated together, thus reducing processing time. The plasma bag system used incorporates an integral membrane plasma filter and a dry MB pill which dissolves in the plasma to give a 1-microM concentration. There is computer-controlled processing and datalogging. In an assessment of 10 pools of Group A plasma, the losses of coagulation factors, following MB/light treatment, were 23% fibrinogen, 10% FV, 26% FVIII, 11% FIX and 13% FXI. Group O, Group B and Group AB plasmas were not tested. Von Willebrand factor (vWf) multimers showed no substantial change when treated with MB, and no losses were seen for antithrombin III (ATIII), protein C and vWf:Ag. Measurements of C3a, C5a, prothrombin fragment 1+2 and FXIIa indicated that there was no activation as a result of filtration.

Published

2001

40. Factor XIIa and triacylglycerol rich lipoproteins: responses to exercise intervention.

Author

Woolf-May K, Jones W, Kearney EM, Davison RC, and Bird S

Subjects

Cholesterol, HDL analysis, Cholesterol, LDL analysis, Female, Humans, Male, Middle Aged, Triglycerides analysis, Exercise physiology, Factor XIIa analysis, Lipoproteins analysis, Walking physiology

Abstract

Objectives: (a) To determine if factor XIIa (FXIIa) would be sensitive to change from exercise intervention in a group of previously sedentary/low active middle aged men and women; (b) to investigate further the previously reported relation between FXIIa and triacylglycerol (TAG) rich lipoproteins., Methods: Thirty seven men (mean (SD) age 57 (7) years) and 60 women (mean age 54 (7) years) completed the study. Before the intervention, these subjects were randomly allocated to a group of walkers (n = 81) or controls (n = 16). Before and after an 18 week walking intervention, fasted blood samples were collected and analysed for FXIIa, TAG, total cholesterol (TC), low density lipoprotein cholesterol (LDL-C), high density lipoprotein cholesterol (HDL-C), and apolipoprotein (apo) B., Results: Kruskal-Wallis analysis of data obtained before the intervention showed no significant differences (p>0.4) between the walking and control groups for age, height, body mass, gender, FXIIa, TAG, TC, HDL-C, or apo B, although the women did show significantly lower levels of TAG (p<0.04) and higher HDL-C (p<0.0001) than the men. General linear model analysis of data obtained after the intervention, using the baseline value as a covariate, showed significant reductions (p<0.0001) in FXIIa for the walkers compared with the controls. Pearson product-moment correlations also showed significant relations between the concentrations of FXIIa and TAG, TC, LDL-C, and apo B., Conclusions: The findings of this study suggest that FXIIa is sensitive to change from exercise intervention and support previous research showing an association between the concentrations of FXIIa and TAG rich lipoproteins.

Published

2000

41. The link between high-fat meals and postprandial activation of blood coagulation factor VII possibly involves kallikrein.

Author

Larsen LF, Marckmann P, Bladbjerg EM, Ostergaard PB, Sidelmann J, and Jespersen J

Subjects

Adult, Blood Coagulation drug effects, Blood Glucose, Enzyme Precursors blood, Factor VII analysis, Factor XII analysis, Factor XII metabolism, Factor XIIa analysis, Factor XIIa metabolism, Fasting, Humans, Insulin blood, Male, Monocytes metabolism, Peptide Fragments analysis, Prothrombin analysis, Triglycerides blood, Blood Coagulation physiology, Dietary Fats administration & dosage, Factor VII metabolism, Kallikreins blood, Postprandial Period

Abstract

Contrary to low-fat meals, high-fat meals are known to cause postprandial factor VII (FVII) activation, but the mechanism is unknown. To study the postprandial FVII activation in detail, 18 young men consumed in randomized order high-fat or low-fat test meals. Fasting and non-fasting blood samples were collected. The high-fat test was associated with an increase in plasma triglyceride and kallikrein concentrations and postprandial FVII activation (p<0.001). Plasma kallikrein was strongly associated with triglycerides in fasting and non-fasting samples (r2=0.74-0.87, p<0.0001), suggesting that triglyceride-rich lipoproteins may activate prokallikrein. Neither plasma triglycerides nor kallikrein and activated FVII were statistically associated. This may suggest that additional factors are involved in the postprandial FVII activation. No clear evidence for a role of tissue factor expression by monocytes, factor XII or insulin in postprandial FVII activation was observed. Tissue factor pathway inhibitor and prothrombin fragment 1+2, a marker of thrombin generation, were not affected postprandially after either the high-fat or the low-fat meals. Our findings indicate that triglyceride-rich lipoproteins activate prokallikrein postprandially, which might form an important initial event in FVII activation after consumption of high-fat meals.

Published

2000

42. Reduction of blood loss and transfusion requirement by aprotinin in posterior lumbar spine fusion.

Author

Lentschener C, Cottin P, Bouaziz H, Mercier FJ, Wolf M, Aljabi Y, Boyer-Neumann C, and Benhamou D

Subjects

Adult, Aprotinin adverse effects, Double-Blind Method, Factor VIIa analysis, Factor XIIa analysis, Female, Hematocrit, Hemostatics adverse effects, Humans, Intraoperative Period, Male, Middle Aged, Platelet Count drug effects, Postoperative Period, Prospective Studies, Prothrombin analysis, Aprotinin therapeutic use, Blood Loss, Surgical prevention & control, Blood Transfusion, Hemostatics therapeutic use, Spinal Fusion

Abstract

Unlabelled: Aprotinin reduces blood loss in many orthopedic procedures. In posterior lumbar spine fusion, blood loss results primarily from large vein bleeding and also occurs after the wound is closed. Seventy-two patients undergoing posterior lumbar spine fusion were randomly assigned to large-dose aprotinin therapy or placebo. All patients donated three units of packed red blood cells (RBCs) preoperatively. Postoperative blood loss was harvested from the surgical wound in patients undergoing two- and/or three-level fusion for reinfusion. The target hematocrit for RBC transfusion was 26% if tolerated. Total (intraoperative and 24 h postoperative) blood loss, transfusion requirements, and percentage of transfused patients per treatment group were significantly smaller in the aprotinin group than in the placebo group (1935 +/- 873 vs 2809 +/- 973 mL per patient [P = 0.007]; 42 vs 95 packed RBCs per group [P = 0.001]; 40% vs 81% per group [P = 0.02]). Hematological assessments showed an identically significant (a) intraoperative increase in both thrombin-antithrombin III complexes (TAT) and in activated factor XII (XIIa) and (b) decrease in activated factor VII (VIIa), indicating a similar significant effect on coagulation in patients of both groups (P = 0.9 for intergroup comparisons of postoperative VIIa, XIIa, and TAT). Intraoperative activation of fibrinolysis was significantly less pronounced in the aprotinin group than in the placebo group (P < 0.0001 for intergroup comparison of postoperative D-dimer levels). No adverse drug effects (circulatory disturbances, deep venous thrombosis, alteration of serum creatinine) were detected. Although administered intraoperatively, aprotinin treatment dramatically reduced intraoperative and 24-h postoperative blood loss and autologous transfusion requirements but did not change homologous transfusion in posterior lumbar spine fusion., Implications: In our study, aprotinin therapy significantly decreased autologous, but not homologous, transfusion requirements in posterior lumbar spine fusion.

Published

1999

43. Evaluation of markers of deep vein thrombosis in patients undergoing surgery for maxillofacial malignancies.

Author

Wendel HP, Scholpp J, Schulze HJ, Heller W, and Schwenzer N

Subjects

Antithrombin III analysis, Blood Coagulation Tests, Case-Control Studies, Factor XIIa analysis, Fibrinogen analysis, Head and Neck Neoplasms blood, Humans, Kallikrein-Kinin System, Monitoring, Intraoperative, Multivariate Analysis, Peptide Hydrolases analysis, Thromboembolism etiology, Tissue Plasminogen Activator blood, Venous Thrombosis diagnosis, Head and Neck Neoplasms surgery, Postoperative Complications, Venous Thrombosis blood, Venous Thrombosis etiology

Abstract

During and following significant surgical intervention, deep venous thrombosis prophylaxis by application of anticoagulants is routinely used. However, patients with malignant disorders are subject to an especially high risk of deep venous thrombosis progressing in severe cases to subsequent pulmonary embolism. The present study focuses on appraising modern markers of deep vein thrombosis in 34 patients undergoing major maxillofacial surgery, with some malignant disorders. No significant differences between the two patient groups were noted using the markers of the kallikrein-kinin-system. From the first postoperative day plasma levels of the coagulation indicator thrombin-antithrombin-III complexes were significantly higher in the group of tumour patients. Markers of fibrinolysis indicated corresponding results: on the first postoperative day tissue-plasminogen activator values rose to 18.9 +/- 3.2 micrograms/l in the group of malignant patients, but only to 7.4 +/- 1.1 micrograms/l (P < 0.05) in the control group. Also postoperative D-dimer concentrations in the malignancy group were significantly above those of the control group. In the present study it could be demonstrated that patients with malignant neoplasia undergoing major maxillofacial surgery are exposed postoperatively to a particularly high risk of developing thromboembolic complications. All in all, the status of anti-thrombotic therapy requires reappraisal with respect to the current treatment approach adopted in tumour patients.

Published

1999

44. Haemocompatibility of paediatric membrane oxygenators with heparin-coated surfaces.

Author

Wendel HP, Scheule AM, Eckstein FS, and Ziemer G

Subjects

Child, Factor XIIa analysis, Humans, Kallikreins analysis, Leukocyte Elastase metabolism, Neutrophils metabolism, Osmolar Concentration, Platelet Count, Platelet Factor 4 analysis, Surface Properties, alpha 1-Antitrypsin metabolism, Biocompatible Materials, Blood Physiological Phenomena, Heparin, Oxygenators, Membrane, Pediatrics instrumentation

Abstract

Extracorporeal circulation (ECC) in paediatric patients with heparin-coated oxygenation systems is rarely investigated. The objective of this study was to evaluate, preclinically, the haemocompatibility of paediatric membrane oxygenators with heparin-coated surfaces. We compared 16 paediatric membrane oxygenators (Minimax, Medtronic) in an in vitro heart-lung machine model with fresh human blood. Eight of these oxygenation systems had a covalent heparin coating (Carmeda bioactive surface). After 90 min simulated ECC, the heparin-coated systems showed significantly higher platelet count, lower platelet-factor 4 release, reduced contact activation (factor XIIa and kallikrein), and lower neutrophil elastase levels (p < 0.05), compared to the noncoated oxygenator group. More biocompatible materials for paediatric operations may ameliorate the various postperfusion syndromes arising from ECC procedures, particularly unspecific inflammation, hyperfibrinolysis and blood loss.

Published

1999

45. Clustering of haemostatic risk factors with FXIIIVal34Leu in patients with myocardial infarction.

Author

Kohler HP and Grant PJ

Subjects

Antifibrinolytic Agents analysis, Factor XIIa analysis, Gene Frequency, Genotype, Humans, Myocardial Infarction genetics, Plasminogen Activator Inhibitor 1 analysis, Plasminogen Activator Inhibitor 1 genetics, Polymorphism, Genetic, Promoter Regions, Genetic, Risk Factors, Tissue Plasminogen Activator analysis, White People genetics, Amino Acid Substitution, Factor XIII genetics, Myocardial Infarction epidemiology, Point Mutation, Thrombophilia epidemiology

Published

1998

46. Pathogenetic and clinical aspects of C1 inhibitor deficiency.

Author

Cicardi M, Bergamaschini L, Cugno M, Beretta A, Zingale LC, Colombo M, and Agostoni A

Subjects

Abdomen, Acute etiology, Angioedema diagnosis, Angioedema genetics, Angioedema immunology, Autoantibodies immunology, Autoantigens immunology, Autoimmune Diseases immunology, Complement Activation, Complement C1 Inactivator Proteins genetics, Complement C1 Inactivator Proteins immunology, Complement System Proteins analysis, Diagnosis, Differential, Factor XIIa analysis, Humans, Laryngeal Edema etiology, Paraproteinemias complications, Paraproteinemias immunology, Peritonitis diagnosis, Angioedema etiology, Complement C1 Inactivator Proteins deficiency

Abstract

People deficient in C1-INH present recurrent angioedema localized to subcutaneous or mucous tissues. The defect can be caused by impaired synthesis, due to a genetic defect (hereditary angioedema), or by increased catabolism (acquired angioedema). In our experience the majority of patients with acquired angioedema (16 of 18) have autoantibodies to C1-INH in their serum. These autoantibodies bind to C1-INH with different and generally low affinity. The vasopermeability mediator responsible for attacks is still undefined: bradykinin (derived from cleavage of high molecular weight kininogen) and a kinin-like peptide (derived from the second component of complement) still remain the two primary candidates. We examined the systems controlled by C1-INH (complement, contact system, fibrinolysis and coagulation) and found that all of them are activated during angioedema attacks. Activation of the coagulation leads to generation of thrombin whose vasoactive effect can thus influence edema formation. Treatment of severe angioedema attacks is satisfactorily performed with C1-INH plasma concentrate although patients with an acquired defect frequently need very high doses. Attenuated androgens effectively prevent attacks in hereditary angioedema, but their safety, on the very long-term, needs to be further assessed. Acquired angioedema generally fail to respond to these drugs, but can be treated prophylactically with antifibrinolytic agents.

Published

1998

47. Availability in pooled normal blood plasma of activated Hageman factor and kallikrein for contact induced coagulation.

Author

Real KJ and Masterson BF

Subjects

Blood Coagulation, Factor XIIa analysis, Humans, Kallikreins analysis, Kinetics, Reference Values, Trypsin Inhibitors pharmacology, Factor XII Deficiency blood, Factor XIIa metabolism, Kallikreins metabolism

Published

1998

48. The association of factor VIIa, factor XIIa and beta2-glycoprotein-1 with triglyceride-rich lipoproteins in normolipidaemic subjects.

Author

Cardigan RA, Donohoe S, Purdy G, Mackie IJ, and Machin SJ

Subjects

Chylomicrons blood, Chylomicrons drug effects, Chylomicrons isolation & purification, Factor VIIa drug effects, Factor XIIa drug effects, Fasting blood, Glycoproteins drug effects, Humans, Lipase pharmacology, Lipoproteins chemistry, Lipoproteins drug effects, Membrane Glycoproteins blood, Membrane Glycoproteins drug effects, Polyethylene Glycols pharmacology, Postprandial Period physiology, Reference Values, beta 2-Glycoprotein I, Factor VIIa analysis, Factor XIIa analysis, Glycoproteins blood, Lipoproteins blood, Triglycerides blood

Abstract

The activation of factors XII (FXII) and VII (FVII) has been shown to occur on the surface of lipoproteins in the presence of lipoprotein lipase and may be modulated by beta2glycoprotein-1 (beta2GP1). In the postprandial state FVII is activated without apparent activation of FXII in plasma. We investigated whether beta2GP1, FXIIa and FVIIa are associated with triglyceride-rich lipoproteins in the fasting and postprandial state. Six normal subjects were studied while fasting and 1, 2 and 4 h after ingestion of 100 g fat. We confirmed that plasma FVIIa activity, but not FXIIa antigen, was increased in the postprandial period. FXIIa, FVIIa and beta2GP1 were associated with chylomicra-rich lipoproteins, and lipase or Triton X-100 treatment caused an increase in FXIIa in plasma and chylomicra without an increase in FVIIa. This suggests that FXIIa may be formed in the postprandial period, but its antigenic determinants are masked by the association with lipoprotein particles, although it could still express proteolytic activity. Alternatively a FXII-independent mechanism or surface other than triglyceride-rich lipoproteins may be responsible for FVII activation in the postprandial state.

Published

1998

49. Complement and contact activation in term neonates after fetal acidosis.

Author

Sonntag J, Wagner MH, Strauss E, and Obladen M

Subjects

Acidosis etiology, Acidosis immunology, Brain Ischemia etiology, Complement C1 Inactivator Proteins analysis, Complement C1q analysis, Complement C3a analysis, Complement C5a analysis, Complement Factor B analysis, Factor XIIa analysis, Female, Fetal Hypoxia complications, Humans, Infant, Newborn, Pregnancy, Brain Ischemia immunology, Complement Activation, Fetal Hypoxia immunology

Abstract

Aims: To evaluate complement and contact activation after fetal acidosis., Methods: Fifteen term neonates with hypoxic-ischaemic encephalopathy after umbilical arterial pH < 7.10 were compared with 15 healthy neonates with umbilical arterial pH > 7.20. Determinations of the complement function and C1-inhibitor activity were performed as kinetic tests 22-28 hours after birth. C1q, C1-inhibitor, and factor B concentrations were determined by radial immunodiffusion and those of C3a, C5a, and factor XIIa by enzyme immunoabsorbent assay., Results: Median complement function (46 vs 73%), C1q (4.3 vs 9.1 mg/dl), and factor B (5.2 vs 7.7 mg/dl) decreased after fetal acidosis. The activated split products C3a (260 vs 185 micrograms/l), C5a (5.0 vs 0.6 micrograms/l), and factor XIIa (3.2 vs 1.3 micrograms/l) increased in the neonates after fetal acidosis. No differences were found in the concentration and activity of C1-inhibitor., Conclusions: Complement and contact activation occurred in the newborns with hypoxic-ischaemic encephalopathy. Activation of these systems generates mediators which can trigger inflammation and tissue injury.

Published

1998

50. Complement and contact activation during cardiovascular operations in infants.

Author

Sonntag J, Dähnert I, Stiller B, Hetzer R, and Lange PE

Subjects

Cardiopulmonary Bypass adverse effects, Complement Factor B analysis, Complement System Proteins analysis, Factor XIIa analysis, Female, Heart Defects, Congenital surgery, Humans, Infant, Infant, Newborn, Male, Prekallikrein metabolism, Prospective Studies, Systemic Inflammatory Response Syndrome etiology, Systemic Inflammatory Response Syndrome metabolism, Cardiac Surgical Procedures, Complement Activation

Abstract

Background: By comparing the results of cardiac operations with or without cardiopulmonary bypass (CPB) in infants in a prospective study, we sought to determine which part of the postoperative systemic inflammatory response was caused by CPB., Methods: Thirty-five patients were divided into two groups: 11 infants operated on without CPB and 24 infants operated on with CPB. Blood samples were drawn before, during, and after the operation. We assessed complement function and the concentrations or activities of C1q, C3, C4, C1 inhibitor, factor B, the activated split product C3a, and prekallikrein and factor XIIa of the contact system., Results: All of the patients exhibited a decrease of complement proteins. This was greater in infants who underwent CPB. A increase in C3a and factor XIIa and changes in prekallikrein activity occurred only in infants during CPB., Conclusions: Complement activation occurs in all infants, but is significantly higher in the group with CPB. Contact activation only occurs in patients who undergo CPB. Thus, the inflammatory response is caused by the use of a CPB circuit and to a lesser degree by surgical procedures and anesthesia.

Published

1998