Your search keyword '"Afibrinogenemia physiopathology"' showing total 69 results

1. Congenital hypofibrinogenemia associated with a novel heterozygous nonsense mutation in the globular C-terminal domain of the γ-chain (p.Glu275Stop).

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Author

Simurda T, Caccia S, Asselta R, Zolkova J, Stasko J, Skornova I, Snahnicanova Z, Loderer D, Lasabova Z, and Kubisz P

Subjects

Anticoagulants administration & dosage, Codon, Nonsense, Genetic Predisposition to Disease, Genetic Testing methods, Humans, Male, Middle Aged, Recurrence, Warfarin administration & dosage, Afibrinogenemia diagnosis, Afibrinogenemia genetics, Afibrinogenemia physiopathology, Blood Coagulation Tests methods, Fibrinogen genetics, Thrombelastography methods, Venous Thrombosis diagnosis, Venous Thrombosis drug therapy, Venous Thrombosis etiology

Published

2020

2. Genetic Variants in the FGB and FGG Genes Mapping in the Beta and Gamma Nodules of the Fibrinogen Molecule in Congenital Quantitative Fibrinogen Disorders Associated with a Thrombotic Phenotype.

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Author

Simurda T, Brunclikova M, Asselta R, Caccia S, Zolkova J, Kolkova Z, Loderer D, Skornova I, Hudecek J, Lasabova Z, Stasko J, and Kubisz P

Subjects

Afibrinogenemia physiopathology, Blood Coagulation Tests, Factor XIII genetics, Fibrin genetics, Fibrinolysis genetics, Hemorrhage, Hemostasis, Hemostatics, Humans, Phenotype, Thrombosis genetics, Thrombosis physiopathology, Afibrinogenemia genetics, Fibrinogen genetics, Fibrinogen metabolism

Abstract

Fibrinogen is a hexameric plasmatic glycoprotein composed of pairs of three chains (Aα, Bβ, and γ), which play an essential role in hemostasis. Conversion of fibrinogen to insoluble polymer fibrin gives structural stability, strength, and adhesive surfaces for growing blood clots. Equally important, the exposure of its non-substrate thrombin-binding sites after fibrin clot formation promotes antithrombotic properties. Fibrinogen and fibrin have a major role in multiple biological processes in addition to hemostasis and thrombosis, i.e., fibrinolysis (during which the fibrin clot is broken down), matrix physiology (by interacting with factor XIII, plasminogen, vitronectin, and fibronectin), wound healing, inflammation, infection, cell interaction, angiogenesis, tumour growth, and metastasis. Congenital fibrinogen deficiencies are rare bleeding disorders, characterized by extensive genetic heterogeneity in all the three genes: FGA , FGB , and FGG (enconding the Aα, Bβ, and γ chain, respectively). Depending on the type and site of mutations, congenital defects of fibrinogen can result in variable clinical manifestations, which range from asymptomatic conditions to the life-threatening bleeds or even thromboembolic events. In this manuscript, we will briefly review the main pathogenic mechanisms and risk factors leading to thrombosis, and we will specifically focus on molecular mechanisms associated with mutations in the C-terminal end of the beta and gamma chains, which are often responsible for cases of congenital afibrinogenemia and hypofibrinogenemia associated with thrombotic manifestations. more...

Published

2020

3. Fibrinogen Łódź: a new cause of dysfibrinogenemia associated with recurrent thromboembolic arterial events.

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Author

Treliński J, Witkowski M, Chojnowski K, Neerman-Arbez M, Wypasek E, and Undas A

Subjects

Afibrinogenemia diagnosis, Afibrinogenemia physiopathology, Female, Humans, Middle Aged, Poland, Recurrence, Treatment Outcome, Afibrinogenemia drug therapy, Afibrinogenemia etiology, Anticoagulants therapeutic use, Brachial Artery physiopathology, Thromboembolism complications, Thromboembolism drug therapy

Published

2019

4. Thromboelastography and Thromboelastometry in Assessment of Fibrinogen Deficiency and Prediction for Transfusion Requirement: A Descriptive Review.

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Author

Peng HT, Nascimento B, and Beckett A

Subjects

Afibrinogenemia metabolism, Blood Coagulation Tests methods, Blood Transfusion methods, Humans, Thrombelastography methods, Afibrinogenemia physiopathology, Fibrinogen metabolism, Thrombosis physiopathology

Abstract

Fibrinogen is crucial for the formation of blood clot and clinical outcomes in major bleeding. Both Thromboelastography (TEG) and Rotational Thromboelastometry (ROTEM) have been increasingly used to diagnose fibrinogen deficiency and guide fibrinogen transfusion in trauma and surgical bleeding patients. We conducted a comprehensive and comparative review on the technologies and clinical applications of two typical functional fibrinogen assays using TEG (FF TEG) and ROTEM (FIBTEM) for assessment of fibrinogen level and deficiency, and prediction of transfusion requirement. Clot strength and firmness of FF TEG and ROTEM FIBTEM were the most used parameters, and their associations with fibrinogen levels as measured by Clauss method ranged from 0 to 0.9 for FF TEG and 0.27 to 0.94 for FIBTEM. A comparison of the interchangeability and clinical performance of the functional fibrinogen assays using the two systems showed that the results were correlated, but are not interchangeable between the two systems. It appears that ROTEM FIBTEM showed better associations with the Clauss method and more clinical use for monitoring fibrinogen deficiency and predicting transfusion requirements including fibrinogen replacement than FF TEG. TEG and ROTEM functional fibrinogen tests play important roles in the diagnosis of fibrinogen-related coagulopathy and guidance of transfusion requirements. Despite the fact that high-quality evidence is still needed, the two systems are likely to remain popular for the hemostatic management of bleeding patients. more...

Published

2018

5. Identification of Two Novel Fibrinogen Bβ Chain Mutations in Two Slovak Families with Quantitative Fibrinogen Disorders.

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Author

Simurda T, Zolkova J, Snahnicanova Z, Loderer D, Skornova I, Sokol J, Hudecek J, Stasko J, Lasabova Z, and Kubisz P

Subjects

Adult, Afibrinogenemia metabolism, Afibrinogenemia physiopathology, Base Sequence, Blood Coagulation Tests, Family, Fibrinogen chemistry, Fibrinogen metabolism, Fibrinogens, Abnormal genetics, Fibrinogens, Abnormal metabolism, Gene Expression, Hemorrhage metabolism, Hemorrhage physiopathology, Homozygote, Humans, Male, Middle Aged, Models, Molecular, Pedigree, Protein Structure, Secondary, Severity of Illness Index, Venous Thrombosis metabolism, Venous Thrombosis physiopathology, Afibrinogenemia genetics, Fibrinogen genetics, Hemorrhage genetics, Mutation, Venous Thrombosis genetics

Abstract

Congenital fibrinogen disorders are caused by mutations in one of the three fibrinogen genes that affect the synthesis, assembly, intracellular processing, stability or secretion of fibrinogen. Functional studies of mutant Bβ-chains revealed the importance of individual residues as well as three-dimensional structures for fibrinogen assembly and secretion. This study describes two novel homozygous fibrinogen Bβ chain mutations in two Slovak families with afibrinogenemia and hypofibrinogenemia. Peripheral blood samples were collected from all subjects with the aim of identifying the causative mutation. Coagulation-related tests and rotational thromboelastometry were performed. All exons and exon-intron boundaries of the fibrinogen genes ( FGA , FGB and FGG ) were amplified by PCR followed by direct sequencing. Sequence analysis of the three fibrinogen genes allowed us to identify two novel homozygous mutations in the FGB gene. A novel Bβ chain truncation (BβGln180Stop) was detected in a 28-year-old afibrinogenemic man with bleeding episodes including repeated haemorrhaging into muscles, joints, and soft tissues, and mucocutaneous bleeding and a novel Bβ missense mutation (BβTyr368His) was found in a 62-year-old hypofibrinogenemic man with recurrent deep and superficial venous thromboses of the lower extremities. The novel missense mutation was confirmed by molecular modelling. Both studying the molecular anomalies and the modelling of fibrinogenic mutants help us to understand the extremely complex machinery of fibrinogen biosynthesis and finally better assess its correlation with the patient's clinical course., Competing Interests: The authors declare no conflict of interest. more...

Published

2017

6. Mild factor XIII deficiency and concurrent hypofibrinogenemia: effect of pregnancy.

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Author

Kaveney AD and Philipp CS

Subjects

Abortion, Spontaneous blood, Abortion, Spontaneous physiopathology, Adult, Afibrinogenemia blood, Afibrinogenemia complications, Afibrinogenemia physiopathology, Factor XIII metabolism, Factor XIII Deficiency blood, Factor XIII Deficiency complications, Factor XIII Deficiency physiopathology, Female, Fibrinogen genetics, Fibrinogen metabolism, Gene Expression, Heterozygote, Humans, Menorrhagia blood, Menorrhagia complications, Menorrhagia physiopathology, Mutation, Postpartum Hemorrhage blood, Postpartum Hemorrhage physiopathology, Pregnancy, Abortion, Spontaneous genetics, Afibrinogenemia genetics, Factor XIII genetics, Factor XIII Deficiency genetics, Menorrhagia genetics, Postpartum Hemorrhage genetics

Abstract

Factor XIII (FXIII) deficiency is a rare bleeding disorder. Patients with mild congenital FXIII deficiency tend to be asymptomatic, but may demonstrate significant bleeding symptoms with surgery, trauma, and pregnancy. Postpartum hemorrhage has been described in mild FXIII deficiency. We present a case of mild FXIII deficiency and concurrent hypofibrinogenemia manifested by recurrent postpartum hemorrhage, menorrhagia, and miscarriage. Mutational analysis identified a previously unreported heterozygous mutation of the FXIIIA subunit (p.Trp315Arg). No mutation was noted in the fibrinogen gene. FXIII levels decreased approximately 50% from nonpregnant levels to their nadir during labor, whereas fibrinogen levels rose approximately 1.5-fold from decreased nonpregnant levels to their peak at the time of labor. This case illustrates the course of mild FXIII and fibrinogen deficiencies during pregnancy, labor, and postpartum, and raises possible management options for prevention of antepartum and postpartum hemorrhage in women with these deficiencies. more...

Published

2016

7. Coexisting congenital dysfibrinogenemia with a novel mutation in fibrinogen γ chain (γ322 Phe→Ile, Fibrinogen Beijing) and haemophilia B in a family.

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Author

Hua B, Li K, Lee A, Poon MC, and Zhao Y

Subjects

Adolescent, Afibrinogenemia physiopathology, Blood Coagulation Tests, DNA Mutational Analysis, Female, Fibrinogen chemistry, Fibrinogen metabolism, Fibrinolysis, Humans, Male, Peptide Fragments chemistry, Peptide Fragments metabolism, Protein Multimerization, Protein Structure, Quaternary, Afibrinogenemia complications, Afibrinogenemia genetics, Fibrinogen genetics, Hemophilia B complications, Mutation, Pedigree, Peptide Fragments genetics

Abstract

Introduction: Both congenital dysfibrinogenemia and haemophilia B (HB) are rare coagulopathies caused by mutations within the fibrinogen and F9 genes respectively., Aim: To investigate the pathogenesis of combined dysfibrinogenemia with HB in a family., Methods: Coagulation assays, factor IX (FIX) activity (one-stage method), fibrinogen activity (Clauss method), antigen (immunoturbidimetry), fibrinogen polymerization and fibrinolysis velocity were measured. The sequences of fibrinogen genes and F9 were amplified by PCR and analysed by sequencing., Results: The proband, a 16-year-old boy with HB (FIX 2 IU dL(-1) ), also had persistently low Clauss fibrinogen level (0.64-0.65 g L(-1) ) with normal antigen level (2.23 g L(-1) ). The mother had a FIX 45 IU dL(-1) and similarly discrepant low Clauss fibrinogen (0.79 g L(-1) ) to antigen levels (2.23 g L(-1) ). Thrombin time for both were either slightly prolonged or at boundary value. Genetic analysis of the proband and the mother identified similar mutations in the FGG gene (heterozygous c.1042T>A resulting in p.Phe348Ile or γPhe322Ile in the mature protein) and in the F9 gene (c.1243del p.His415Metfs*11 and c.1245T>A p.His415Gln). The father had no fibrinogen or F9 gene mutations. Plasma fibrinogen polymerization was delayed, but fibrinolysis velocity was normal in the proband and his mother., Conclusion: To our knowledge, this is the first report of a family with combined novel dysfibrinogen (Fibrinogen Beijing) and HB with bleeding manifestations., (© 2015 John Wiley & Sons Ltd.) more...

Published

2015

8. Paradoxical bleeding and thrombosis in a patient with afibrinogenemia and fibrinogen Mumbai mutation.

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Author

Mukaddam A, Patil R, Jadli A, Chandrakala S, Ghosh K, and Shetty S

Subjects

Adult, Afibrinogenemia complications, Afibrinogenemia physiopathology, Diagnosis, Differential, Exons genetics, Female, Fibrinogen genetics, Hemorrhage etiology, Homozygote, Humans, Mutation, Missense, Sequence Analysis, DNA, Thrombosis physiopathology, Afibrinogenemia genetics, Fibrinogens, Abnormal genetics, Hepatic Veins physiopathology, Portal Vein physiopathology, Splenic Vein physiopathology, Thrombosis etiology

Abstract

Objectives: Thrombosis is rarely reported in cases of afibrinogenemia and is generally associated with thrombophilia or replacement therapy. Often, it is difficult to predict whether the patients will bleed or whether they are exposed to the risk of thrombosis., Methods: We report a patient with afibrinogenemia who presented with complete thrombosis of right hepatic, portal, and splenic veins and who described a lifelong history of bleeding. Direct sequencing of the three fibrinogen genes was performed to identify the mutation., Results: DNA sequencing showed the presence of a homozygous for G8017A substitution in exon 8 of the fibrinogen β-chain gene, resulting in a G434D missense mutation (Fibrinogen Mumbai)., Conclusions: Presence of both bleeding and thrombotic manifestations in a patient with afibrinogenemia in the presence of other associated risk factors warrants a very careful individualized approach in the management of patients with afibrinogenemia., (Copyright© by the American Society for Clinical Pathology.) more...

Published

2015

9. Loss of fibrinogen in zebrafish results in symptoms consistent with human hypofibrinogenemia.

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Author

Vo AH, Swaroop A, Liu Y, Norris ZG, and Shavit JA

Subjects

Animals, Blood Coagulation physiology, DNA Primers, Fibrinogen genetics, Gene Knockdown Techniques, Hemorrhage pathology, Humans, In Situ Hybridization, Morpholinos metabolism, Afibrinogenemia physiopathology, Blood Coagulation genetics, Disease Models, Animal, Fibrinogen metabolism, Phenotype, Zebrafish

Abstract

Cessation of bleeding after trauma is a necessary evolutionary vertebrate adaption for survival. One of the major pathways regulating response to hemorrhage is the coagulation cascade, which ends with the cleavage of fibrinogen to form a stable clot. Patients with low or absent fibrinogen are at risk for bleeding. While much detailed information is known about fibrinogen regulation and function through studies of humans and mammalian models, bleeding risk in patients cannot always be accurately predicted purely based on fibrinogen levels, suggesting an influence of modifying factors and a need for additional genetic models. The zebrafish has orthologs to the three components of fibrinogen (fga, fgb, and fgg), but it hasn't yet been shown that zebrafish fibrinogen functions to prevent bleeding in vivo. Here we show that zebrafish fibrinogen is incorporated into an induced thrombus, and deficiency results in hemorrhage. An Fgb-eGFP fusion protein is incorporated into a developing thrombus induced by laser injury, but causes bleeding in adult transgenic fish. Antisense morpholino knockdown results in intracranial and intramuscular hemorrhage at 3 days post fertilization. The observed phenotypes are consistent with symptoms exhibited by patients with hypo- and afibrinogenemia. These data demonstrate that zebrafish possess highly conserved orthologs of the fibrinogen chains, which function similarly to mammals through the formation of a fibrin clot. more...

Published

2013

10. Role of fibrinogen in acute ischemic kidney injury.

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Author

Sörensen-Zender I, Rong S, Susnik N, Lange J, Gueler F, Degen JL, Melk A, Haller H, and Schmitt R

Subjects

Afibrinogenemia physiopathology, Animals, Epithelial Cells metabolism, Fibrinogen biosynthesis, Fibrinogen genetics, Interleukin-6 pharmacology, Kidney Transplantation, Male, Mice, Mice, Inbred C57BL, Oncostatin M pharmacology, Acute Kidney Injury physiopathology, Fibrinogen physiology, Reperfusion Injury physiopathology

Abstract

Renal ischemia-reperfusion (I/R) is associated with activation of the coagulation system and accumulation of blood clotting factors in the kidney. The aim of the present study was to examine the functional impact of fibrinogen on renal inflammation, damage, and repair in the context of I/R injury. In this study, we found that I/R was associated with a significant increase in the renal deposition of circulating fibrinogen. In parallel, I/R stress induced the de novo expression of fibrinogen in tubular epithelial cells, as reflected by RT-PCR, immunofluorescence, and in situ hybridization. In vitro, fibrinogen expression was induced by oncostatin M and hyper-IL-6 in primary tubular epithelial cells, and fibrinogen-containing medium had an inhibitory effect on tubular epithelial cell adhesion and migration. Fibrinogen(+/-) mice showed similar survival as wild-type mice but better preservation in early postischemic renal function. In fibrinogen(-/-) mice, renal function and survival were significantly worse than in fibrinogen(+/-) mice. Renal transplant experiments revealed reduced expression of tubular damage markers and attenuated proinflammatory cytokine expression but increased inflammatory cell infiltrates and transforming growth factor-β expression in fibrinogen(-/-) isografts. These data point to heterogeneous effects of fibrinogen in renal I/R injury. While a complete lack of fibrinogen may be detrimental, partial reduction of fibrinogen in heterozygous mice can improve renal function and overall outcome. more...

Published

2013

11. Surgical wound healing in bleeding disorders.

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Author

Rodriguez-Merchan EC

Subjects

Afibrinogenemia physiopathology, Animals, Factor XIII Deficiency physiopathology, Hemophilia B physiopathology, Hemorrhage prevention & control, Hemostasis physiology, Humans, Models, Animal, Risk Factors, Surgical Procedures, Operative, Blood Coagulation Disorders physiopathology, Wound Healing physiology

Abstract

Animal experiments have shown that a number of bleeding disorders may affect wound healing (WH), including haemophilia B, deficiency of factor XIII and abnormalities of fibrinogen. Therefore, normal healing requires adequate haemostatic function for the appropriate time frame (up to 4 weeks in the clean and uncontaminated wound). Many factors may affect WH, including impaired haemostasis, diabetes, poor nutrition, insufficient oxygenation, infection, smoking, alcoholism, old age, stress and obesity. The gold standard for the correct care of surgical wounds in patients with bleeding disorders includes wound dressing and comprehensive standard care (haemostasis, nutritional support, treatment of co-morbidities, offloading, reperfusion therapy and compression). Although complications of surgical wounds healing in patients with bleeding disorders are uncommon, a low level of the deficient factor for an insufficient period of time could cause WH complications such as haematomas, infection, and skin necrosis and dehiscence. Clinical experience and animal experiments appear to indicate that, to get a satisfactory healing of surgical wounds and avoid potential complications of WH, a good level of haemostasis is necessary for 2-3 weeks after surgery. However, many treaters would regard this recommendation at odds with (i.e. more aggressive than) current standards. Unfortunately no additional clinical evidence for this recommendation can be provided., (© 2012 Blackwell Publishing Ltd.) more...

Published

2012

12. Rare deletion from the fibrinogen Bβ gene in a patient with a provoked venous thrombotic event.

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Author

Shen YM, Sarode R, Bhogaraju A, and Brennan S

Subjects

Adult, Afibrinogenemia complications, Afibrinogenemia diagnosis, Afibrinogenemia physiopathology, Chromatography, Reverse-Phase, DNA Mutational Analysis, Genotype, Humans, Male, Phenotype, Venous Thrombosis complications, Venous Thrombosis diagnosis, Venous Thrombosis physiopathology, White People, Afibrinogenemia genetics, Fibrinogen genetics, Hemorrhage genetics, Sequence Deletion, Venous Thrombosis genetics

Abstract

Hypodysfibrinogenemia is characterized by both a qualitative and quantitative deficiency of fibrinogen. Here we report a patient with remote history of bleeding and presents with provoked deep venous thrombosis associated with hypodysfibrinogenemia. Molecular studies identified the presence of fibrinogen Epsom, which was previously reported in a family with pregnancy associated bleeding. This case illustrates the difficulty in linking the genotype and phenotype in patients with defective fibrinogen. more...

Published

2011

13. A novel frameshift mutation in FGA (c.1846 del A) leading to congenital afibrinogenemia in a consanguineous Syrian family.

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Author

Levrat E, Aboukhamis I, de Moerloose P, Farho J, Chamaa S, Reber G, Fort A, and Neerman-Arbez M

Subjects

Adult, Afibrinogenemia congenital, Afibrinogenemia genetics, Afibrinogenemia physiopathology, Consanguinity, Disease Susceptibility, Exons, Female, Fibrinogen metabolism, Genetic Association Studies, Genetic Testing, Genotype, Hemorrhage, Heterozygote, Homozygote, Humans, Male, Pedigree, Phenotype, Syria, Fibrinogen genetics, Frameshift Mutation

Abstract

Congenital afibrinogenemia is a rare autosomal recessive coagulation disorder characterized essentially by bleeding symptoms, but miscarriages and, paradoxically, thromboembolic events can also occur. Most reported mutations leading to congenital afibrinogenemia are located in FGA encoding the fibrinogen A α-chain. In this study, we analysed 12 individuals from a consanguineous Syrian family with reduced or absent fibrinogen levels: those with fibrinogen levels around 1 g/l (n = 7) were found to be heterozygous for a novel frameshift mutation in FGA exon 5 (c.1846 del A) and those with undetectable fibrinogen levels (n = 5) were homozygous for the same mutation. This novel frameshift mutation is the most C-terminal causative FGA mutation identified to date in afibrinogenemic patients. The resulting aberrant Aα-chain (p.Thr616HisfsX32) is most likely synthesized, but is less efficiently assembled and/or secreted into the circulation given the phenotype of asymptomatic hypofibrinogenemia in heterozygous individuals and bleeding diathesis in homozygous individuals. more...

Published

2011

14. Cryoprecipitate: no longer the best therapeutic choice in congenital fibrinogen disorders?

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Author

Bevan DH

Subjects

Afibrinogenemia congenital, Afibrinogenemia physiopathology, Fibrinogens, Abnormal genetics, Fibrinogens, Abnormal metabolism, Humans, Plasma, Afibrinogenemia therapy, Fibrinogen therapeutic use

Abstract

Congenital abnormalities of fibrinogen are rare disorders classified as quantitative (afibrinogenemia and hypofibrinogenemia) or qualitative types (dysfibrinogenemia and hypodysfibrinogenemia). Fibrinogen is essential to haemostasis as the substrate for fibrin clot formation and also acts in primary haemostasis as a key ligand in platelet aggregation. Quantitative deficiency of fibrinogen can result in severe bleeding, or arterial and venous thromboembolism, and poor wound healing. Dysfibrinogenemia is characterized by functional abnormalities of fibrinogen, which may be asymptomatic (in 50% of cases), or cause bleeding (25%) or thrombosis (25%). Replacement of the deficient or abnormal fibrinogen with frozen plasma, cryoprecipitate, or fibrinogen concentrate has been found to be effective in practice in treating haemostatic complications of these disorders. Although cryoprecipitate is the most commonly used replacement material, pathogen-reduced fibrinogen concentrates have several advantages, most importantly a lower potential risk of viral transmission and standardized fibrinogen content allowing accurate dosing. They also avoid transfusing unwanted clotting factors, platelet microparticles and immunoglobulins, and can be administered rapidly without thawing. The use of fibrinogen concentrate to treat congenital fibrinogen disorders is strongly supported in principle and increasingly by practical experience and evidence. more...

Published

2009

15. Severe spontaneous arterial thrombotic manifestations in patients with inherited hypo- and afibrinogenemia.

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Author

Castaman G, Lunardi M, Rigo L, Mastroeni V, Bonoldi E, and Rodeghiero F

Subjects

Adult, Afibrinogenemia complications, Amputation, Surgical statistics & numerical data, Angiography, Female, Foot surgery, Humans, Middle Aged, Renal Artery drug effects, Thrombosis etiology, Tibial Arteries drug effects, Treatment Outcome, Afibrinogenemia physiopathology, Fibrinogen metabolism, Foot physiopathology, Renal Artery physiology, Thrombosis physiopathology, Tibial Arteries physiology

Abstract

We report two novel cases of severe arterial thrombotic episodes occurring in two women with severe hypofibrinogenemia, not linked to the administration of replacement therapy. The first patient had sudden acute occlusion of the anterior branch of left renal artery with infarction of the antero-lateral region of the upper part of the left kidney during treatment with combined oestrogen-progestogen started 16 years before for recurrent haemoperitoneum caused by bleeding at ovulation. The second patient showed recurrent arterial thrombosis of lower limbs over 2 years, which eventually led to amputation of affected limbs. Thrombotic events in patients with inherited severe hypofibrinogenemia are rather frequent, may be severe and not associated with the use of replacement therapy. more...

Published

2009

16. Neither fibrin nor plasminogen activator inhibitor-1 deficiency protects lung function in a mouse model of acute lung injury.

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Author

Allen GB, Cloutier ME, Larrabee YC, Tetenev K, Smiley ST, and Bates JH

Subjects

Acute Lung Injury etiology, Acute Lung Injury genetics, Acute Lung Injury physiopathology, Afibrinogenemia genetics, Afibrinogenemia physiopathology, Animals, Bronchoalveolar Lavage Fluid chemistry, Disease Models, Animal, Female, Fibrin physiology, Fibrinogen genetics, Fibrinogen physiology, Inflammation Mediators physiology, Lung pathology, Lung physiopathology, Mice, Mice, Inbred C57BL, Mice, Knockout, Respiratory Mechanics genetics, Respiratory Mechanics physiology, Serpin E2, Serpins genetics, Serpins physiology, Acute Lung Injury prevention & control, Fibrin deficiency, Serpins deficiency

Abstract

Fibrin impairs surfactant function in vitro, and inhibition of fibrinolysis by plasminogen activator inhibitor (PAI-1) is thought to promote fibrin accumulation in acute lung injury (ALI). This has led to speculation that impaired PAI-1 and fibrin accumulation should protect lung function in ALI. We tested this hypothesis by investigating ALI severity in fibrinogen-deficient (Fgn-/-) and PAI-1-deficient (PAI-1-/-) mice. PAI-1-/-, C57BL/6, Fgn-/-, and Fgn+/- females were anesthetized and allowed to aspirate 4 microl/g of hydrochloric acid (pH 1.0) and then reanesthetized and connected to a ventilator 48 h later. Naive C57BL/6 and Fgn+/- females served as controls. Following deep inflation (DI), forced oscillations were delivered periodically over 8 min to measure changes in elastance (H) as a surrogate of lung derecruitment, at positive end-expiratory pressures (PEEP) of 6, 3, and 1 cmH(2)O. Increases in H following DI in acid-injured mice were greater than naive strain-matched controls. Increases in H were no different between injured PAI-1-/- and C57BL/6, or between injured Fgn-/- and +/- mice, at any PEEP. Pressure-volume curves were no different between injured groups. Total lung fibrin was lower in injured PAI-1-/- and Fgn-/- mice relative to injured C57BL/6 and Fgn+/- mice, respectively, but indices of permeability were no different between strains. Unexpectedly, neither fibrin nor PAI-1 deficiency protects lung mechanical function in mice with acid-induced ALI. We speculate that in vivo lung function may be more closely tied to permeability and alveolar protein in general, rather than being linked specifically to fibrin. more...

Published

2009

17. Efficacy and tolerability of human fibrinogen concentrate administration to patients with acquired fibrinogen deficiency and active or in high-risk severe bleeding.

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Author

Danés AF, Cuenca LG, Bueno SR, Mendarte Barrenechea L, and Ronsano JBM

Subjects

Adolescent, Adult, Afibrinogenemia blood, Afibrinogenemia complications, Afibrinogenemia physiopathology, Aged, Aged, 80 and over, Child, Child, Preschool, Drug Tolerance, Female, Fibrinogen adverse effects, Fibrinogen isolation & purification, Hemorrhage blood, Hemorrhage etiology, Hemorrhage physiopathology, Humans, Infant, Male, Middle Aged, Retrospective Studies, Risk Factors, Safety, Afibrinogenemia drug therapy, Fibrinogen administration & dosage, Hemorrhage drug therapy

Abstract

Background and Objectives: Fibrinogen deficiency is a cause for massive haemorrhage whose management in emergency situations is the subject of debate. Plasma-derived fibrinogen concentrates are indicated for reversing the haemorrhagic diathesis found in congenital and acquired deficiencies., Materials and Methods: We report on the results of an observational study that evaluated the effects of fibrinogen concentrates in patients suffering from various forms of acquired severe hypofibrinogenaemia with life-threatening consumptive thrombo-haemorrhagic disorders (surgery, trauma and digestive haemorrhage), or underlying disease states that limit fibrinogen synthesis (hepatic dysfunction, haematological malignancies)., Results: Sixty-nine patients were identified and included, in whom most of the processes (62%) corresponded to consumptive hypofibrinogenaemia. After a median dose of 4 g, a mean absolute increase of 1.09 g/l in plasma fibrinogen was measured and coagulation parameters were significantly improved (P < 0.001). Mortality rates of 32.3% and 44.2% were reported after 24 h and 72 h, respectively., Conclusion: We conclude that the administration of fibrinogen concentrates in unresponsive, life-threatening haemorrhage with acquired hypofibrinogenaemia improves laboratory measures of coagulation, and may also be life saving. Although observational in nature, our data indicate a direct relationship between plasma fibrinogen levels and survival in acquired fibrinogen deficiency. Further studies are warranted to ascertain a clear relationship between fibrinogen levels and survival. more...

Published

2008

18. Afibrinogenemia resulting from homozygous nonsense mutation in A alpha chain gene associated with multiple thrombotic episodes.

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Author

Simsek I, de Mazancourt P, Horellou MH, Erdem H, Pay S, Dinc A, and Samama MM

Subjects

Adult, Afibrinogenemia physiopathology, Codon, Nonsense, Consanguinity, Homozygote, Humans, Male, Pedigree, Afibrinogenemia complications, Afibrinogenemia genetics, Fibrinogen genetics, Polymorphism, Single Nucleotide genetics, Thrombosis etiology

Abstract

Congenital afibrinogenemia is a rare disorder characterized by the absence in circulating fibrinogen, a hexamer composed of two sets of three polypeptides (Aalpha, Bbeta and gamma). Although predisposition to thrombosis is a well known feature of dysfibrinogenemia, the relatively frequent thrombotic manifestations seen in congenital afibrinogenemia are puzzling. We herein report a mutational analysis of a young afibrinogenemic man from Turkey with multiple thrombo-embolic events involving both arteries and veins. Purified DNAs of the propositus was used for amplification by polymerase chain reaction of all the exons of the A subunit gene with primers allowing the analysis of the intron-exon boundaries. Analysis of the genes coding for the three fibrinogen chains of the propositus found a homozygous G to A transition in the exon 5 of the A alpha chain gene (g.g4277a; access number gi458553). The TGG to TGA codon change predicts a homozygous W315X in the A alpha chain (p.W334X when referring to the translation initiation codon). Both parents and his brother were found to carry this heterozygous mutation. This is the first report of a patient homozygous for this rare mutation associated with afibrinogenemia. Our patient was free of known risk factors as well as diseases associated with thrombosis including atherosclerosis, vasculitis, Buerger's disease, and it seems therefore probable that afibrinogenemia itself might have contributed to both arterial and venous thrombosis. more...

Published

2008

19. Budd-Chiari syndrome in an afibrinogenemic patient: a paradoxical complication.

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Author

Oruc N, Tokat Y, Killi R, Tombuloglu M, and Ilter T

Subjects

Adolescent, Afibrinogenemia physiopathology, Budd-Chiari Syndrome diagnosis, Female, Humans, Afibrinogenemia complications, Budd-Chiari Syndrome etiology

Published

2006

20. [Congenital afibrinogenemia: focusing on molecular mechanisms controlling fibrinogen secretion].

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Author

Vu D and Neerman-Arbez M

Subjects

Animals, COS Cells metabolism, Cell Compartmentation, Chickens, Chlorocebus aethiops, Fibrinogen chemistry, Fibrinogen genetics, Fibrinogen physiology, Humans, Models, Biological, Models, Molecular, Mutation, Protein Conformation, Protein Structure, Tertiary, Recombinant Fusion Proteins metabolism, Structure-Activity Relationship, Transfection, Afibrinogenemia physiopathology, Fibrinogen metabolism

Published

2006

21. Maternal fibrinogen is necessary for embryonic development.

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Author

Iwaki T and Castellino FJ

Subjects

Adult, Afibrinogenemia drug therapy, Animals, Blood Coagulation Disorders physiopathology, Female, Humans, Mice, Pregnancy, Pregnancy Complications, Hematologic drug therapy, Pregnancy Complications, Hematologic physiopathology, Thrombosis physiopathology, Afibrinogenemia physiopathology, Embryonic Development physiology, Fibrinogen physiology

Abstract

Fibrinogen (Fg) is a precursor of fibrin, which is one of the main components of blood clots generated during the hemostatic response. Beyond its important role in hemostasis, Fg is involving in several physiologic and pathophysiologic states, such as infection, wound healing, the progression of certain types of tumors, and the severity of atherosclerosis. In addition, Fg has a critical role in maintaining pregnancy. Ovulation, fertilization, and implantation of the fertilized egg to the uterine wall can occur in afibrinogenemic women. However, all pregnancies in these patients resulted in spontaneous miscarriage. Fg supplemental therapy allows the patients to sustain the pregnancy. Mice with a total fibrinogen deficiency (FG-/-) reproduce the human experience. Despite of successes with fibrinogen supplementation, "paradoxical thrombosis" sometimes occurs, wherein supplemental therapies cause catastrophic thrombosis, such as pulmonary and mesenteric venous thrombosis. In these therapies, syncytial knots, hyaline membrane, and multiple recent infarctions with abruptio placenta were also observed. These findings indicate that the dosage regimen of Fg in afibrinogenemia-related pregnancies needs to be optimized according to other coagulation markers, such as thrombin-antithrombin complex (TAT) concentration, which represents the extent of thrombin formation. In addition, baseline thrombin assays would be helpful to predict the potential for paradoxical thrombosis during the supplemental therapy offered during pregnancy. more...

Published

2005

22. The past decade: fibrinogen.

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Author

Pulanić D and Rudan I

Subjects

Afibrinogenemia physiopathology, Cardiovascular Diseases physiopathology, Fibrinogen chemistry, Fibrinogen genetics, Hemostasis, Humans, Fibrinogen physiology, Platelet Aggregation, Wound Healing

Abstract

This paper reviews the advances in understanding of fibrinogen structure and function, its genetic and environmental determinants, role in the process of hemostasis, platelet aggregation, plasma viscosity and erythrocyte aggregation, cellular and matrix interactions, inflammation, wound healing, tumor development, atherogenesis and involvement in pathogenesis of diseases, that have been made over the past decade. Future studies will seek to define precise mechanisms of complex gene-environment interactions that influence fibrinogen levels and its complex role in the pathogenesis of fibrinogen-associated diseases. more...

Published

2005

23. Congenital hypofibrinogenemia in pregnancy: report of two cases and review of the literature.

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Author

Frenkel E, Duksin C, Herman A, and Sherman DJ

Subjects

Adult, Afibrinogenemia physiopathology, Afibrinogenemia therapy, Animals, Female, Fibrinogen therapeutic use, Humans, Mice, Pregnancy, Pregnancy Outcome, Prenatal Care, Afibrinogenemia congenital, Pregnancy Complications, Hematologic

Abstract

Fibrinogen abnormalities have been implicated in many adverse pregnancy outcomes, mainly spontaneous abortion, placental abruption, and postpartum hemorrhage. Two new cases of congenital hypofibrinogenemia in pregnancy are reported detailing their obstetric course and management. The relevant obstetric and hematologic literature is reviewed, including previous case reports and studies concerning the mechanisms of pregnancy complications. Suggestions for treatment guidelines and management strategies are detailed. more...

Published

2004

24. Dysfibrinogenemia and thrombosis.

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Author

Hayes T

Subjects

Afibrinogenemia complications, Afibrinogenemia physiopathology, Blood Coagulation Tests, Evidence-Based Medicine, Fibrinogens, Abnormal metabolism, Humans, Practice Guidelines as Topic, Risk Assessment, Risk Factors, Thrombophilia complications, Thrombophilia diagnosis, Thrombophilia physiopathology, Thrombosis etiology, Thrombosis physiopathology, Afibrinogenemia diagnosis, Thrombosis diagnosis

Abstract

Objectives: To review the state of the art relating to congenital dysfibrinogenemia as a potential risk factor for thrombosis, as reflected by the medical literature and the consensus opinion of recognized experts in the field, and to make recommendations for the use of laboratory assays for assessing this thrombotic risk in individual patients., Data Sources: Review of the medical literature, primarily from the last 10 years., Data Extraction and Synthesis: After an initial assessment of the literature, key points were identified. Experts were assigned to do an in-depth review of the literature and to prepare a summary of their findings and recommendations. A draft manuscript was prepared and circulated to every participant in the College of American Pathologists Conference on Diagnostic Issues in Thrombophilia. Each of the key points and associated recommendations were then presented for discussion at the conference. Recommendations were accepted if a consensus of experts attending the conference was reached. The results of the discussion were used to revise the manuscript into its final form., Conclusions: Consensus was reached on 5 conclusions and 2 recommendations concerning the use of testing for dysfibrinogens in the assessment of thrombotic risk in individual patients. Detailed discussion of the rationale for each of these recommendations is found in the text of this article. Compared with the other, more common hereditary thrombophilias, dysfibrinogenemia encompasses a diverse group of defects with varied clinical expressions. Congenital dysfibrinogenemia is a relatively rare cause of thrombophilia. Therefore, routine testing for this disorder is not recommended as part of the laboratory evaluation of a thrombophilic patient. This is an evolving area of research, and further clinical studies may change these recommendations in the future. more...

Published

2002

25. Elevated fibrinogen in an acute phase reaction prolongs the reptilase time but typically not the thrombin time.

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Author

Van Cott EM, Smith EY, and Galanakis DK

Subjects

Adult, Afibrinogenemia blood, Afibrinogenemia physiopathology, Age Factors, Humans, Middle Aged, Time Factors, Acute-Phase Reaction metabolism, Fibrinogen metabolism, Thrombin Time

Abstract

The effects of elevated fibrinogen on thrombin and reptilase times have not been well documented. High fibrinogen levels are common (38% of specimens submitted to our coagulation laboratory). Among 102 patients in the present study, an endogenously elevated fibrinogen level was significantly associated, as follows, with prolonged reptilase times: 1 (4%) of 28 with normal fibrinogen levels, 6 (20%) of 30 with levels in the 400 to 700 mg/dL (4.0-7.0 g/L) range, 10 (34%) of 29 with levels in the 700 to 1,000 mg/dL (7.0-10.0 g/L) range, and 7 (47%) of 15 with fibrinogen levels greater than 1,000 mg/dL (10.0 g/L). This association was independent of patient age and fibrin degradation product titer. In contrast, thrombin time was not altered notably by elevated fibrinogen levels. In 4 patients studied further, the prolonged clotting times could be corrected or nearly corrected by adding calcium chloride or albumin, whereas no such corrections were demonstrable in samples from several hereditary dysfibrinogenemia control subjects. An elevated fibrinogen level is common and is associated with reptilase time prolongations. For patients with prolonged reptilase times, a fibrinogen assay is suggested before establishing a diagnosis of dysfibrinogenemia. more...

Published

2002

26. Genetic interactions between the coagulation and fibrinolytic systems.

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Author

Degen JL

Subjects

Afibrinogenemia genetics, Afibrinogenemia physiopathology, Animals, Coagulation Protein Disorders genetics, Coagulation Protein Disorders physiopathology, Fibrinolysis physiology, Mice, Phenotype, Plasminogen deficiency, Plasminogen genetics, Plasminogen physiology, Blood Coagulation genetics, Fibrinolysis genetics

Abstract

Nearly all of the genes encoding the established coagulation and fibrinolytic factors have been successfully altered or disrupted in transgenic mice. Although comprehensive studies of each of these gene-targeted mouse lines are still ongoing, the initial findings have significantly refined our understanding of the roles of selected hemostatic factors in vivo, and occasionally altered long-standing concepts. This review summarizes some of the progress that has been made in the generation and phenotypic characterization of mice lacking key hemostatic factors, including coagulation, fibrinolytic, platelet and endothelial cell-associated factors. New insights regarding the role(s) and interplay of hemostatic factors that have emerged from detailed studies of mice carrying multiple deficits in coagulation and fibrinolytic system components are highlighted. more...

Published

2001

27. Healing of corneal epithelial defects in plasminogen- and fibrinogen-deficient mice.

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Author

Kao WW, Kao CW, Kaufman AH, Kombrinck KW, Converse RL, Good WV, Bugge TH, and Degen JL

Subjects

Afibrinogenemia genetics, Afibrinogenemia metabolism, Animals, Epithelium, Corneal cytology, Epithelium, Corneal injuries, Extracellular Matrix Proteins metabolism, Eye Injuries metabolism, Eye Injuries pathology, Immunoenzyme Techniques, Mice, Plasminogen deficiency, Plasminogen genetics, Afibrinogenemia physiopathology, Epithelium, Corneal physiology, Eye Injuries physiopathology, Plasminogen physiology, Wound Healing physiology

Abstract

Purpose: The local deposition of fibrinogen and other plasma products from tears within corneal wounds and the expression of plasminogen activator by corneal epithelial cells suggest that the coagulation and fibrinolytic systems play an important role in corneal wound healing. The authors used mouse lines deficient in plasminogen (Plg), fibrinogen (Fib), or both to elucidate the roles of these key fibrinolytic and coagulation factors in the healing of corneal epithelial defects., Methods: Mice were anesthetized, and corneal epithelial defects (3 mm) were created with a blade. The authors conducted histologic examination and immunohistochemical analysis on the healing of injured corneas., Results: The corneal epithelial defects of wild-type mice with transparent corneas healed quickly in 7 days, whereas the healing of plasminogen-deficient mice was impaired and complicated by severe and persistent inflammatory responses, the formation of retrocorneal fibrin deposits, corneal cloudiness caused by scar-tissue formation, and often stromal neovascularization. To determine whether these defects in corneal wound repair were specifically related to an impediment in fibrinolysis, corneal wound healing was compared in mice with a combined deficiency in plasminogen and fibrinogen. The loss of fibrinogen in mice lacking plasminogen resulted in the restoration of normal healing with transparent corneas in 7 days, similar to that of wild-type mice., Conclusions: These results provide direct evidence that hemostatic factors play a crucial role in corneal wound repair despite the lack of local hemorrhage. Furthermore, they demonstrate that the essential role of plasmin in corneal would healing is fibrinolysis. It prevents the adverse inflammatory responses caused by prolonged fibrin and fibrinogen deposition in injured corneas. more...

Published

1998

28. Loss of fibrinogen rescues mice from the pleiotropic effects of plasminogen deficiency.

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Author

Bugge TH, Kombrinck KW, Flick MJ, Daugherty CC, Danton MJ, and Degen JL

Subjects

Afibrinogenemia genetics, Age Factors, Animals, Blood Coagulation Disorders etiology, Blood Coagulation Disorders genetics, Blood Coagulation Disorders mortality, Cell Movement, Digestive System pathology, Enzyme Activation, Fibrinogen genetics, Fibrinolysis, Keratinocytes physiology, Liver pathology, Mice, Mice, Mutant Strains, Plasminogen genetics, Skin cytology, Skin Physiological Phenomena, Wasting Syndrome mortality, Wound Healing genetics, Afibrinogenemia physiopathology, Blood Coagulation Disorders physiopathology, Plasminogen deficiency, Wasting Syndrome etiology

Abstract

Plasmin(ogen) is an extracellular serine protease implicated in the activation of latent growth factors and procollagenase, degradation of extracellular matrix components, and fibrin clearance. Plasminogen (Plg) deficiency in mice results in high mortality, wasting, spontaneous gastrointestinal ulceration, rectal prolapse, and severe thrombosis. Furthermore, Plg-deficient mice display delayed wound healing following skin injury, a defect partly related to impaired keratinocyte migration. We generated mice deficient in Plg and fibrinogen (Fib) and show that removal of fibrin(ogen) from the extracellular environment alleviates the diverse spontaneous pathologies previously associated with Plg deficiency and corrects healing times. Mice deficient in Plg and Fib are phenotypically indistinguishable from Fib-deficient mice. These data suggest that the fundamental and possibly only essential physiological role of Plg is fibrinolysis. more...

Published

1996

29. Plasminogen and wound healing.

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Author

Rømer J, Bugge TH, Pyke C, Lund LR, Flick MJ, Degen JL, and Danø K

Subjects

Afibrinogenemia physiopathology, Animals, Mice, Mice, Knockout, Neovascularization, Physiologic, Plasminogen deficiency, Plasminogen genetics, Receptors, Peptide biosynthesis, Receptors, Peptide physiology, Plasminogen physiology, Wound Healing physiology

Published

1996

30. Resolution of spontaneous bleeding events but failure of pregnancy in fibrinogen-deficient mice.

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Author

Suh TT, Holmbäck K, Jensen NJ, Daugherty CC, Small K, Simon DI, Potter S, and Degen JL

Subjects

Afibrinogenemia blood, Afibrinogenemia physiopathology, Aging blood, Alleles, Animals, Animals, Newborn, Base Sequence, Blood Cell Count, DNA Primers, Exons, Female, Fibrinogen biosynthesis, Hematocrit, Hemorrhage blood, Hemorrhage genetics, Male, Mice, Mice, Transgenic, Molecular Sequence Data, Ovarian Follicle pathology, Platelet Aggregation, Polymerase Chain Reaction, Pregnancy, Pregnancy Complications, Hematologic pathology, Restriction Mapping, Afibrinogenemia genetics, Fibrinogen genetics, Hemorrhage physiopathology, Mutation, Pregnancy Complications, Hematologic blood

Abstract

To explore the role of the key coagulation factor, fibrinogen, in development, hemostasis, wound repair, and disease pathogenesis, we disrupted the fibrinogen A alpha chain gene in mice. Homozygous, A alpha chain-deficient (A alpha-/-) mice are born normal in appearance, and there is no evidence of fetal loss of these animals based on the Mendelian pattern of transmission of the mutant A alpha chain allele. All of the component chains of fibrinogen (A alpha, B beta, and gamma) are immunologically undetectable in the circulation of both neonatal and adult A alpha-/- mice, and blood samples fail to either clot or support platelet aggregation in vitro. Overt bleeding events develop shortly after birth in approximately 30% of A alpha-/- mice, most frequently in the peritoneal cavity, skin, and soft tissues around joints. Remarkably, most newborns displaying signs of bleeding ultimately control the loss of blood, clear the affected tissues, and survive the neonatal period. Juveniles and young adult A alpha-/- mice are predisposed to spontaneous fatal abdominal hemorrhage, but long-term survival is variable and highly dependent on genetic background. The periodic rupture of ovarian follicles in breeding-age A alpha-/- females does not appear to significantly diminish life expectancy relative to males; however, pregnancy uniformly results in fatal uterine bleeding around the tenth day of gestation. Microscopic analysis of spontaneous lesions found in A alpha-/- mice suggests that fibrin(ogen) plays a fundamental role in the organization of cells at sites of injury. more...

Published

1995

31. Congenital afibrinogenemia.

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Author

al-Mondhiry H and Ehmann WC

Subjects

Afibrinogenemia physiopathology, Diagnosis, Differential, Fibrinogen adverse effects, Fibrinogen therapeutic use, Humans, Incidence, Afibrinogenemia congenital, Afibrinogenemia therapy

Abstract

Congenital afibrinogenemia is a rare disorder with unusual clinical manifestations. The disease is inherited as an autosomal recessive trait and consanguinity is common among affected families. Clinical manifestations range from minimal bleeding to catastrophic hemorrhage. Congenitally afibrinogenemic patients seem to be peculiarly susceptible to spontaneous rupture of the spleen. Coagulation tests which depend on clot formation as an end point may be infinitely prolonged and abnormalities of platelet function are usually present. The diagnosis is established by demonstrating trace or no immunoreactive fibrinogen. The disease is caused by markedly reduced or absent synthesis of fibrinogen by liver cells, but the genetic defect remains unknown. Bleeding episodes can be effectively treated with cryoprecipitate. Purified virally inactivated fibrinogen concentrates have been used in Europe and may soon be widely available. more...

Published

1994

32. The effect of hypofibrinogenemia and fibrinolysis on skeletal muscle function after ischemia and reperfusion.

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Author

Colburn MD, Gelabert HA, Nowara H, Hajjar GE, Moore WS, and Quiñones-Baldrich WJ

Subjects

Ancrod pharmacology, Animals, Isometric Contraction, Male, Muscles drug effects, Plasminogen pharmacology, Rabbits, Time Factors, Urokinase-Type Plasminogen Activator pharmacology, Afibrinogenemia physiopathology, Fibrinogen metabolism, Fibrinolysis, Ischemia physiopathology, Muscles blood supply, Muscles physiopathology, Reperfusion

Abstract

Isometric contraction to direct supramaximal tetanic stimulation of the anterior tibialis (AT) muscle was measured in 50 New Zealand White rabbits after ischemia and reperfusion. Ischemia was produced unilaterally by collateral ligation and temporary inflow control until AT muscle function decreased to < 5% of contralateral (control) AT muscle and the ischemic interval was recorded. Reperfusion was carried out in one of the following ways: group I (n = 20), release of vascular clamps (blood reperfusion [BR]); group II (n = 10), release of vascular clamps and simultaneous intraarterial administration of 50,000 units of urokinase (urokinase reperfusion [UR]); group III (n = 10), release of vascular clamps and simultaneous administration of 50,000 units of urokinase and 28 mg (5 units) of purified rabbit plasminogen (urokinase plasminogen reperfusion [UPR]); and group IV (n = 10), animals defibrinated to < 50 mg/dl with ancrod prior to ischemia and received BR (ancrod blood reperfusion [ABR]). During reperfusion, function was recorded every 60 min for 2 hr. Recovery of experimental muscle function is expressed as the percentage of contralateral control limb function. The mean ischemic interval (mean +/- SEM), to achieve < 5% of contralateral control limb function, was 206.7 +/- 9.9, 209.5 +/- 16.6, 221.7 +/- 12.5, and 272.0 +/- 14.2 min for animals in groups I-IV, respectively. The mean experimental muscle function (mean +/- SEM) following the ischemic interval was 3.2 +/- 0.8, 4.5 +/- 1.4, 4.4 +/- 1.2, and 3.3 +/- 1.0 for groups I-IV, respectively.(ABSTRACT TRUNCATED AT 250 WORDS) more...

Published

1994

33. The role of von Willebrand factor and fibrinogen in platelet aggregation under varying shear stress.

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Author

Ikeda Y, Handa M, Kawano K, Kamata T, Murata M, Araki Y, Anbo H, Kawai Y, Watanabe K, and Itagaki I

Subjects

Afibrinogenemia physiopathology, Bernard-Soulier Syndrome physiopathology, Humans, In Vitro Techniques, Protein Binding, Stress, Mechanical, Thrombasthenia physiopathology, Time Factors, von Willebrand Diseases physiopathology, Fibrinogen metabolism, Platelet Aggregation, Platelet Membrane Glycoproteins metabolism, von Willebrand Factor metabolism

Abstract

Exposure of platelets to shear stress leads to aggregation in the absence of exogenous agonists. We have now found that different adhesive proteins and platelet membrane glycoproteins are involved in aggregation depending on the shear stress conditions and the concentration of divalent cations in the medium. When blood is collected with trisodium citrate as anticoagulant, which causes a decrease in the levels of external ionized calcium ([Ca2+]o), platelet aggregation can be induced under low shear force (12 dyn/cm2) and is mediated by fibrinogen binding to the glycoprotein IIb-IIIa complex. Aggregates formed under these conditions are not stable, and when shear force is increased to 68 dyn/cm2, disaggregation results. By contrast, platelets from blood collected with hirudin as anticoagulant, wherein [Ca2+]o is within normal plasma levels, do not undergo low shear-induced aggregation; however, after exposure to a shear force above 80 dyn/cm2, aggregation is observed but only when von Willebrand factor is present and can interact with both its platelet binding sites, glycoprotein Ib-IX and glycoprotein IIb-IIIa. Fibrinogen is not involved in high shear-induced aggregation which, in fact, occurs normally in patients with severe afibrinogenemia. Thus, von Willebrand factor in the absence of exogenous agonists can mediate platelet aggregation in experimental conditions that may mimic the hemorheological situation of partially occluded arteries. This pathway of platelet aggregation involving only one adhesive ligand and two membrane adhesion receptors may play a relevant role in thrombogenesis. more...

Published

1991

34. Fibrinogen and fibrin formation and its role in fibrinolysis.

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Author

Blombäck B

Subjects

Afibrinogenemia genetics, Afibrinogenemia physiopathology, Amino Acid Sequence, Animals, Blood Proteins metabolism, Calcium physiology, Epitopes immunology, Fibrinolysin metabolism, Gels, Glycosylation, Hemostasis, Humans, Models, Molecular, Molecular Sequence Data, Molecular Structure, Phylogeny, Polymers, Thrombin metabolism, Thrombosis genetics, Thrombosis physiopathology, Fibrin biosynthesis, Fibrinogen chemistry, Fibrinogen genetics, Fibrinogen immunology, Fibrinogen physiology, Fibrinolysis

Published

1991

35. The effect of defibrinogenation on pulmonary embolism in dogs.

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Author

Meissner AG, O'Sullivan G, and Macbeth RA

Subjects

Afibrinogenemia physiopathology, Animals, Dogs, Hemodynamics, Pulmonary Embolism complications, Respiration Disorders complications, Rheology, Fibrinogen physiology, Pulmonary Embolism physiopathology

Published

1976

36. Phagocytic and catabolic function of the reticuloendothelial system in dogs subjected to defibrinogenation.

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Author

Ahlgren T, Berghem L, Lagergren H, Lahnborg G, and Schildt B

Subjects

Afibrinogenemia metabolism, Animals, Dogs, Mononuclear Phagocyte System metabolism, Serum Albumin, Radio-Iodinated metabolism, Time Factors, Afibrinogenemia physiopathology, Mononuclear Phagocyte System physiopathology, Phagocytosis

Published

1976

37. [Fibrinogen anomalies and extracorporeal circulation: apropos of 2 cases].

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Author

Pelissier E, Le Pennec PY, Terrier E, and Jaulmes B

Subjects

Afibrinogenemia surgery, Child, Fibrinogen therapeutic use, Heparin therapeutic use, Humans, Male, Risk, Afibrinogenemia physiopathology, Cardiovascular Surgical Procedures, Extracorporeal Circulation, Postoperative Complications prevention & control

Published

1980

38. [Management of congenital afibrinogenemia in an oral surgery patient (author's transl)].

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Subjects

Afibrinogenemia physiopathology, Afibrinogenemia therapy, Blood Coagulation, Hemorrhage prevention & control, Humans, Afibrinogenemia congenital, Surgery, Oral

Published

1981

39. [Case of familial hypofibrinogenemia and hereditary afibrinogenemia].

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Author

Karavanov AG and Kutsenko TA

Subjects

ABO Blood-Group System, Adult, Afibrinogenemia physiopathology, Child, Female, Hemorrhagic Disorders genetics, Hemorrhagic Disorders physiopathology, Humans, Male, Rh-Hr Blood-Group System, Afibrinogenemia genetics

Published

1980

40. Fibrinogen-bound sialic acid levels in the dysfibrinogenaemia of liver disease.

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Author

Francis JL and Armstrong DJ

Subjects

Afibrinogenemia blood, Afibrinogenemia physiopathology, Fibrin Fibrinogen Degradation Products analysis, Fibrinogen metabolism, Humans, Liver Cirrhosis complications, Liver Cirrhosis physiopathology, Liver Diseases physiopathology, Platelet Membrane Glycoproteins, Thrombin Time, Afibrinogenemia complications, Liver Diseases complications, Receptors, Cell Surface, Sialic Acids blood

Abstract

Fibrinogen-bound sialic acid levels were determined in 75 normal controls and 80 patients with liver disease. Patients with abnormal fibrin monomer polymerisation (FMP) had sialic acid levels significantly higher than controls or patients with normal FMP. Enzymatic removal of sialic acid from the abnormal fibrinogens corrected the abnormal FMP and thrombin-clotting times to the range of desialated controls. The accelerating effects of calcium ions, protamine sulphate and Polybrene were largely abolished by desialation, suggesting that these cations accelerate FMP by neutralising the negativity charged sialic acid residues. more...

Published

1982

41. Use of a monoclonal antibody to measure the surface expression of thrombospondin following platelet activation.

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Author

Legrand C, Dubernard V, Kieffer N, and Nurden AT

Subjects

Afibrinogenemia physiopathology, Antibodies, Monoclonal, Antibody Specificity, Blood Coagulation Disorders physiopathology, Edetic Acid pharmacology, Humans, Thrombospondins, Blood Platelets physiology, Fibrinogen physiology, Glycoproteins metabolism

Abstract

The radiolabelled monoclonal antibody, 5G11, directed against native thrombospondin, has been used to assess the surface expression of secreted thrombospondin on human blood platelets. Emphasis has been placed on studying the role of fibrinogen in this process. Unstimulated platelets bound low amounts of 5G11 (about 2000 molecules/platelet). Binding increased 2-fold and 5-7-fold after stimulation of platelets with ADP or thrombin (or ionophore A23187) respectively. Unstimulated platelets from patients deficient in alpha-granule proteins (gray platelet syndrome) bound baseline levels of 5G11. However, binding was not increased after activation. Thrombospondin expression on thrombin-stimulated normal platelets was for a large part divalent-cation-dependent and was not affected by AP-2, a monoclonal antibody to GPIIb-IIIa complexes. However, binding of 5G11 was some 50% lower when platelets were stimulated in the presence of Fab fragments of a polyclonal rabbit antibody to fibrinogen. This suggested either a direct binding of thrombospondin to surface-bound fibrinogen or a steric inhibition due to a close proximity of the two proteins. The fact that binding of 5G11 was at the lower limit of the normal range to the stimulated platelets of an afibrinogenaemic patient specifically lacking detectable fibrinogen favoured the latter explanation. Thus, a major fibrinogen-independent pathway for thrombospondin expression must exist. more...

Published

1988

42. von Willebrand factor interaction with the glycoprotein IIb/IIa complex. Its role in platelet function as demonstrated in patients with congenital afibrinogenemia.

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Author

De Marco L, Girolami A, Zimmerman TS, and Ruggeri ZM

Subjects

Adenosine Diphosphate pharmacology, Bleeding Time, Collagen pharmacology, Deamino Arginine Vasopressin therapeutic use, Fibrinogen analysis, Humans, Immunoglobulin Fab Fragments, Platelet Aggregation drug effects, Platelet Membrane Glycoproteins, Afibrinogenemia physiopathology, Blood Platelets physiology, Receptors, Cell Surface metabolism, von Willebrand Factor metabolism

Abstract

We have studied three afibrinogenemic patients, who had only trace amounts of plasma and platelet fibrinogen as measured by radioimmunoassay, and demonstrate here that the residual aggregation observed in their platelet-rich plasma is dependent upon von Willebrand factor (vWF) binding to the platelet membrane glycoprotein (GP)IIb/IIIa complex. The abnormality of aggregation was more pronounced when ADP, rather than thrombin, collagen, or the combination of ADP plus adrenaline was used to stimulate platelets. With all stimuli, nevertheless, the platelet response was completely inhibited by a monoclonal antibody (LJP5) that is known to block vWF, but not fibrinogen binding to GPIIb/IIIa. Addition of purified vWF to the afibrinogenemic plasma resulted in marked increase in the rate and extent of aggregation, particularly when platelets were stimulated with ADP. This response was also completely blocked by LJP5. Addition of fibrinogen, however, restored normal aggregation even in the presence of LJP5, a finding consistent with the knowledge that antibody LJP5 has no effect on platelet aggregation mediated by fibrinogen binding to GPIIb/IIIa. Two patients gave their informed consent to receiving infusion of 1-desamino-8-D-arginine vasopressin (DDAVP), a vasopressin analogue known to raise the vWF levels in plasma by two- to fourfold. The bleeding time, measured before and 45 min after infusion, shortened from greater than 24 min to 12 min and 50 s in one patient and from 16 min to 9 min and 30 s in the other. Concurrently, the rate and extent of ADP-induced platelet aggregation improved after DDAVP infusion. The pattern, however, reversed to baseline levels within 4 h. The concentration of plasma vWF increased after DDAVP infusion, but that of fibrinogen remained at trace levels. We conclude that vWF interaction with GPIIb/IIIa mediates platelet-platelet interaction and may play a role in primary hemostasis. more...

Published

1986

43. Dental treatment of a patient with congenital afibrinogenemia--complications of supportive care.

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Author

Helpin ML and Morrison FS

Subjects

Afibrinogenemia complications, Afibrinogenemia physiopathology, Child, Female, Hemorrhage etiology, Humans, Afibrinogenemia congenital, Dental Care for Persons with Disabilities

Published

1981

44. [Effect of antithrombin III on anticoagulating system function in animals intravenously injected with tissue thromboplastin].

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Author

Pastorova VE and Kovalev SV

Subjects

Afibrinogenemia physiopathology, Animals, Antithrombins isolation & purification, Blood Coagulation drug effects, Blood Coagulation Tests, Cattle, Female, Fibrinogen analysis, Injections, Intravenous, Male, Rats, Time Factors, Antithrombins pharmacology, Fibrinolysis drug effects, Thromboplastin administration & dosage

Abstract

In experiments with rats, antithrombin III (a natural inhibitor of fibrinolysis) was shown to decrease the activation of the anticoagulation system either in prophylactic administration or during the development of thrombogenesis, caused by intravenous administration of tissue thromboplastin. The phenomenon led to the maintaining of the more high content of fibrinogen in blood of experimental animals, to the shortening of the thrombin time and to the increase in content of alpha2-macroglobulin and alpha1-antitrypsin (in-hibitors of fibrinolysis) as compard with control animals, administered with the only thrombolastin. Effect of antithrombin III depended on periods of administration of the prearation and on injection of tissue thromboplastin. more...

Published

1976

45. Dysfibrinogenemia. A current perspective.

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Author

Galanakis DK

Subjects

Afibrinogenemia congenital, Amino Acid Sequence, Blood Coagulation, Fetus, Fibrin biosynthesis, Fibrin physiology, Fibrinogen genetics, Fibrinogen physiology, Genetic Variation, Humans, Time Factors, Afibrinogenemia physiopathology

Abstract

At least 24 single amino acid substitution dysfibrinogens are currently known. Emerging evidence supports conclusions reached from studies on normal fibrinogen, which relate to the importance of release of A peptides to formation of a physiologically adequate fibrin clot; the existence of "D-D" or (b-b) polymerization sites; and the importance of the gamma chain carboxy terminal segment in fibrin assembly. more...

Published

1984

46. [How does defibrinogenization influence wound healing?].

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Author

Köhnlein HE, Blümel J, Seitz HD, and Krieg G

Subjects

Animals, Batroxobin administration & dosage, Male, Rats, Afibrinogenemia physiopathology, Wound Healing

Published

1976

47. [Hypodysfibrinogenemia: fibrinogen giessen II (author's transl)].

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Author

Krause WH, Huth K, Heene DL, and Lasch HG

Subjects

Adult, Afibrinogenemia complications, Afibrinogenemia physiopathology, Batroxobin, Female, Fibrin metabolism, Fibrinogen metabolism, Fibrinolysis, Hemorrhagic Disorders physiopathology, Humans, Streptokinase pharmacology, Thrombin biosynthesis, Thromboplastin biosynthesis, Afibrinogenemia congenital, Fibrinogen analysis, Hemorrhagic Disorders etiology

Abstract

A new case of facultative hemorrhagic diathesis is described in a 19 year old female and the coagulatory anomaly examined. The experiments show that the coagulatory disturbance should be ascribed to a defective aggregation of fibrin monomers associated with hypofibrinogenemia. Some of its characteristics are the markedly prolonged thrombin-, reptilase-time as well prolonged prothrombin and partial thromboplastin time. The plasma fibrinogen concentration measured by the immunologic method is reduced. The streptokinase induced digestion of fibrinogen Giessen II plasma occurred at a slower rate than normal plasma with persistence of the large fibrinogen degradation products. Fibrinogen Giessen II appears to be a congenital hypodysfibrinogenemia with abnormality of fibrinogen resulting in delayed coagulation and a retarded fibrinogenolysis rate. more...

Published

1975

48. The fibrinogenopathies.

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Author

Morse EE

Subjects

Adolescent, Adult, Afibrinogenemia genetics, Amino Acid Sequence, Blood Coagulation, Child, Child, Preschool, Female, Fibrinogen metabolism, Fibrinopeptide A metabolism, Fibrinopeptide B metabolism, Humans, Infant, Male, Middle Aged, Pedigree, Structure-Activity Relationship, Afibrinogenemia physiopathology

Abstract

This paper reviews the reported clinical, functional and biochemical abnormalities associated with abnormal fibrinogens. It appears from studies on fibrinogen Detroit that a single amino acid substitution in a critical part of the molecule can lead to major functional abnormalities and clinical consequences of either bleeding or thrombosis. Functional defects observed include: abnormal release of fibrinopeptide A or B or both after incubation with thrombin, abnormal polymerization and abnormal clot stabilization. more...

Published

1978

49. Proceedings: Approaches to the structure of fibrinogen.

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Author

Finlayson JS

Subjects

Afibrinogenemia physiopathology, Chemical Phenomena, Chemistry, Humans, Models, Chemical, Structure-Activity Relationship, Fibrinogen analysis

Published

1975

50. Fibrinogen-independent aggregation and deaggregation of human platelets: studies in two afibrinogenemic patients.

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Author

Cattaneo M, Kinlough-Rathbone RL, Lecchi A, Bevilacqua C, Packham MA, and Mustard JF

Subjects

Adenosine Diphosphate pharmacology, Adolescent, Adult, Afibrinogenemia physiopathology, Antibodies administration & dosage, Antibodies immunology, Chymotrypsin pharmacology, Edetic Acid pharmacology, Female, Fibrinogen analysis, Hirudins pharmacology, Humans, Immunoglobulin Fab Fragments immunology, Platelet Membrane Glycoproteins immunology, Platelet Membrane Glycoproteins physiology, Thrombin pharmacology, Afibrinogenemia blood, Fibrinogen physiology, Platelet Aggregation drug effects

Abstract

Platelets from two afibrinogenemic patients were used to determine whether fibrinogen is essential for platelet aggregation and to examine whether released fibrinogen contributes to the stabilization of platelet aggregates when platelets have been induced to aggregate and release their granule contents by stimulation with thrombin. The addition of adenosine diphosphate (ADP) to platelet-rich plasma (PRP) or to suspensions of washed platelets from the afibrinogenemic patients caused the formation of small aggregates, which was either not inhibited or only slightly inhibited by the F(ab')2 fragments of an antibody to fibrinogen but was inhibited by an antibody (10E5) to glycoprotein IIb/IIIa. Thus there is a component of ADP-induced platelet aggregation that is not dependent on fibrinogen or other plasma proteins but is dependent on glycoprotein IIb/IIIa. There was little difference in the extent of aggregation and the release of granule contents of normal and afibrinogenemic platelets in response to the release-inducing agents collagen, platelet-activating factor (PAF), sodium arachidonate, or thrombin. With normal or afibrinogenemic platelets, aggregation by thrombin (0.2 U/mL or higher) was not inhibited by the F(ab')2 fragments of an antibody to human fibrinogen. Deaggregation by combinations of inhibitors of platelets aggregated by 1 U/mL thrombin showed no difference between platelets from afibrinogenemic and control subjects, indicating that released fibrinogen does not make a major contribution to the stabilization of platelet aggregates formed by thrombin stimulation. more...

Published

1987