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1. Doping of Athletes

Author

Ratnoff Od and Miles Aa

Subjects
Doping in Sports, biology, Computer science, Athletes, Leading Articles, General Engineering, General Medicine, biology.organism_classification, Data science, World Wide Web, General Earth and Planetary Sciences, Humans, General Environmental Science
Published
1964

2. Confirmation of mendelian properties of heterodimeric fibrinogen molecules in a heterozygotic dysfibrinogenemia, "fibrinogen Amarillo," using gprphoresis to differentiate semifibrin molecules from fibrinogen and fibrin.

Author

Shainoff JR, Ratnoff OD, Smejkal GB, DiBello PM, Welches WR, Lill H, Mitkevich OV, and Periman P

Subjects
Dimerization, Electrophoresis, Polyacrylamide Gel, Family Health, Fibrin metabolism, Fibrinogens, Abnormal metabolism, Fibrinopeptide A metabolism, Heterozygote, Humans, Kinetics, Point Mutation, Serine Endopeptidases metabolism, Fibrinogens, Abnormal genetics
Abstract

The fibrinogen molecule consists of two sets of Aalpha, Bbeta, and gamma chains assembled into a bilateral disulfide linked (Aalpha, Bbeta, gamma)2 structure. Cleavage of the two A-fibrinopeptides (FPA, Aalpha1-16) from normal Aalpha chains with arginine at position 16 (RFPA) by thrombin or the venom enzyme atroxin transforms fibrinogen into self-aggregating fibrin monomers (alpha, Bbeta, gamma)(2). Mutant Aalpha16R-->H fibrinopeptide (HFPA) cannot be cleaved from fibrinogen by atroxin. Many studies on heterozygous dysfibrinogenemias with this mutation suggested that incorporation of the mutant chains into the molecules was ordered in a manner yielding only (1) homodimeric normal (RFPARFPA) atroxin-coagulable molecules and (2) homodimeric abnormal (H(FPA)HFPA) atroxin-incoagulable molecules in equal quantities. Although heterodimeric molecules (RFPAHFPA) could not be found in studies on the intact protein, Meh et al. demonstrated their existence by showing that CNBr digests of fibrinogens from atroxin-treated Aalpha16R-->H heterozygotic dysfibrinogenemias consistently yielded N-terminal fragments (NDSKs) with partially resolved electrophoretic bands predominantly in between the NDSKs of fibrinogen and alpha-fibrin. An opportunity to confirm and better quantify the heterodimers arose with the recent development of a method (GPRphoresis) for identifying molecules lacking only one FPA, which is applied here in study of a newly presenting case of an Aalpha16R-->H dysfibrinogenemia, "fibrinogen Amarillo." GPRphoresis uses electrophoretic shifts, staged with GPRP-NH(2) to separate the self-aggregating fibrin monomers lacking both FPAs from weakly aggregating "semifibrin" molecules lacking one FPA An antifibrin alpha17-23 antibody is used to measure and differentiate the semifibrin from fibrinogen with FPA fully intact. Applying GPRphoresis to atroxin digests of fibrinogen Amarillo clearly demonstrated RFPARFPA, RFPAHFPA, and HFPAHFPA molecules in nearly perfect Mendelian 1:2:1 proportions. In turn, the high levels of the semifibrin in the terminal atroxin digests provide genetic phenotypic evidence supporting fidelity of the GPRphoresis method.

Published
2001
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3. Inhibition of expression of monocyte interleukin-1 by inhibitors of Hageman factor (factor XII).

Author

Ratnoff OD, Voytus JA, and Toossi Z

Subjects
Adult, Endotoxins pharmacology, Factor XII physiology, Humans, Trypsin pharmacology, Trypsin Inhibitors, Factor XII antagonists & inhibitors, Interleukin-1 metabolism, Monocytes metabolism, Zea mays chemistry
Abstract

In an earlier study, activated species of Hageman factor (factor XII) induced elaboration of interleukin-1 by human monocytes. These observations did not address whether Hageman factor participated in endotoxin-induced release of interleukin-1. To examine this question, the release of interleukin-1 by endotoxin-stimulated human mononuclear cells was measured in the presence of popcorn inhibitor, a specific inhibitor of Hageman factor. In the experiments herein described, popcorn inhibitor sharply decreased the release of interleukin-1 by human mononuclear cells that were incubated with endotoxin. This observation suggests that Hageman factor may play a role in the elaboration of interleukin-1 by human mononuclear cells. Conforming with this view, the addition of antiserum directed against Hageman factor inhibited the release of interleukin-1 from endotoxin-stimulated mononuclear cells.

Published
1995

4. Inhibitory action of amyloid precursor protein against human Hageman factor (factor XII).

Author

Niwano H, Embury PB, Greenberg BD, and Ratnoff OD

Subjects
Amyloid beta-Protein Precursor genetics, Animals, Baculoviridae genetics, Ellagic Acid pharmacology, Factor Xa Inhibitors, Gallic Acid analogs & derivatives, Gallic Acid pharmacology, Heparin pharmacology, Humans, Insecta, Organometallic Compounds pharmacology, Partial Thromboplastin Time, Prothrombin Time, Recombinant Proteins pharmacology, Thrombin antagonists & inhibitors, Amyloid beta-Protein Precursor pharmacology, Factor XII antagonists & inhibitors
Abstract

Amyloid precursor protein forms that contain Kunitz protease inhibitor domains are released from activated platelets, T-lymphocytes, and leukocytes and inhibit trypsin, plasmin, and activated factor XI. We investigated the effects of amyloid precursor protein isoforms on activated Hageman factor (factor XII), activated factor X (Stuart factor), and thrombin. Recombinant amyloid precursor proteins with or without the Kunitz domain, 770 and 695 amino acids, respectively, were produced in insect cells by Baculovirus expression (BAC770 and BAC695). Neither BAC695 nor BAC770 inhibited human alpha-thrombin or activated factor X. The partial thromboplastin time was prolonged by both amyloid precursor proteins, only one of which, BAC770, contains the Kunitz protease inhibitor domain. Both forms of amyloid precursor proteins inhibited ellagic acid-induced activation of Hageman factor but did not inhibit activated Hageman factor. Bismuth subgallate, which is an insoluble analog of ellagic acid, lost its ability to activate Hageman factor on being exposed to BAC770. Inhibition of ellagic acid-induced activation of Hageman factor by both forms of amyloid precursor protein was enhanced by heparin. These findings suggested that the heparin-binding domain of amyloid precursor proteins is not in the Kunitz domain. This heparin-binding domain may block the activation of Hageman factor by negatively charged agents. Thus, amyloid precursor proteins may be involved in the control of hemostasis, properties not all dependent on the Kunitz domain.

Published
1995

5. Airway obstruction in hemophilia (factor VIII deficiency): a 28-year institutional review.

Author

Bogdan CJ, Strauss M, and Ratnoff OD

Subjects
Adolescent, Adult, Aged, Airway Obstruction diagnosis, Airway Obstruction mortality, Airway Obstruction therapy, Blood Loss, Surgical, Blood Transfusion, Child, Child, Preschool, Combined Modality Therapy, Factor VIII therapeutic use, Female, Humans, Length of Stay, Male, Middle Aged, Recurrence, Retrospective Studies, Tracheotomy, Airway Obstruction etiology, Hemophilia A complications, Hemorrhage complications
Abstract

Life-threatening airway compromise is rarely reported as a major complication of coagulation disorders. However, before adequate factor-replacement therapy became available, this complication was often fatal. A retrospective review of all patients with classic hemophilia admitted to our institution from 1964 through 1992 was performed. The records of 147 patients who had a total of 1804 admissions were examined. Fifteen episodes of airway obstruction occurred. Additionally, 6 cases of potential airway compromise and 5 cases of airway-endangering oropharyngeal bleeding were identified. Tracheotomy was performed in 5 patients; 1 fatality occurred before modern replacement products were available. Patients with this disorder have a 13% chance of some form of airway-endangering event with an 8% chance that it will be immediately life-threatening. Tracheotomy and subsequent decannulation are safe procedures in these patients.

Published
1994
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6. Gene transfer in vivo: sustained expression and regulation of genes introduced into the liver by receptor-targeted uptake.

Author

Perales JC, Ferkol T, Beegen H, Ratnoff OD, and Hanson RW

Subjects
Animals, Asialoglycoprotein Receptor, Base Sequence, DNA administration & dosage, DNA Primers chemistry, Factor IX administration & dosage, Gene Expression Regulation, Liver metabolism, Male, Molecular Sequence Data, Phosphoenolpyruvate Carboxykinase (GTP) genetics, Promoter Regions, Genetic, RNA, Messenger genetics, Rats, Rats, Sprague-Dawley, Receptors, Cell Surface metabolism, Transcription, Genetic, Gene Transfer Techniques
Abstract

Receptor-mediated gene transfer has been used to introduce genes into tissues of animals in vivo. The genes introduced by this approach have been transiently expressed at low levels in animal tissues. High levels of expression, for longer periods, have been attained by the induction of cell division (i.e., partial hepatectomy) or disruption of lysosomal degradation of the DNA. We have studied the correlation of specific structural features on the DNA/ligand complexes with their ability to efficiently introduce DNA into the livers of intact animals. A chimeric gene containing the phosphoenolpyruvate carboxykinase gene promoter (nucleotides -460 to +73) linked to the structural gene for human factor IX (PEPCK-hFIX gene) was condensed with galactosylated poly(L-lysine) by titration with NaCl, resulting in complexes of defined size (10-12 nm in diameter) and shape. The PEPCK-hFIX gene complex was injected into the caudal vena cava of adult rats and the conjugated DNA was specifically targeted to the livers of the animals; no detectable DNA was noted in other tissues. The plasmid containing the PEPCK-hFIX gene was found as an episome in the livers of the rats 32 days after injection of the DNA complex. Human factor IX DNA, mRNA, and functional protein were detected up to 140 days after administration of the DNA complex (the duration of the experiment). Transcription from the PEPCK promoter could be induced over the entire course of the experiment by feeding the rats a high-protein, carbohydrate-free diet. We conclude that the structure of the DNA/ligand complexes is of key importance for the successful introduction of genes into the tissues of animals by receptor-mediated endocytosis.

Published
1994
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7. Familial Sneddon's syndrome: clinical, hematologic, and radiographic findings in two brothers.

Author

Pettee AD, Wasserman BA, Adams NL, McMullen W, Smith HR, Woods SL, and Ratnoff OD

Subjects
Adult, Cerebrovascular Disorders immunology, Cerebrovascular Disorders pathology, Humans, Magnetic Resonance Imaging, Male, Skin Diseases, Vascular immunology, Skin Diseases, Vascular pathology, Syndrome, Antibodies, Antiphospholipid blood, Cerebrovascular Disorders genetics, Skin Diseases, Vascular genetics
Abstract

We present the clinical, hematologic, and radiographic findings in two brothers with Sneddon's syndrome (stroke and livedo reticularis) and antiphospholipid antibodies. Patient 1 had anticardiolipin antibody and patient 2 had lupus anticoagulant, which we detected only upon repeated blood testing. One should test for both anticardiolipin antibody and lupus anticoagulant and repeat the screenings before determining a Sneddon's syndrome patient's antiphospholipid antibody status. Both Sneddon's syndrome and the primary antiphospholipid antibody syndrome are potentially familial causes of stroke. In familial cases, an inherited predisposition to antiphospholipid antibody production may be involved in disease pathogenesis.

Published
1994
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8. The effect of chemical modification of basic amino acid residues on the activation and amidolytic activity of Hageman factor (factor XII).

Author

Ryder J, Everson B, Jentoft J, and Ratnoff OD

Subjects
Amides metabolism, Arginine chemistry, Diethyl Pyrocarbonate pharmacology, Factor XII antagonists & inhibitors, Factor XII metabolism, Factor XIIa metabolism, Histidine chemistry, Humans, Lysine chemistry, Phenylglyoxal pharmacology, Serum Albumin, Bovine pharmacology, Structure-Activity Relationship, Trinitrobenzenesulfonic Acid pharmacology, Amino Acids chemistry, Factor XII chemistry
Abstract

Modification of arginyl residues of Hageman factor by phenylglyoxal hydrate inhibits activation of this clotting factor in a plasma-free system, that is, in the absence of the other constituents of the contact activation system. Activation is also inhibited by alteration of the other two basic amino acid residues present, lysine and histidine. Chemical modification of histidine and arginine residues does not inhibit the amidolytic activity of activated Hageman factor. In contrast, modification of amino group(s) in N-terminal and lysine residues inhibits activated Hageman factor. Thus, basic amino acid residues essential to the activation or activity of Hageman factor appear to be variably accessible to chemical modification.

Published
1993

9. An inhibitor of antihemophilic factor (factor VIII) in an 18-month-old nonhemophilic child.

Author

Stein J and Ratnoff OD

Subjects
Animals, Blood Coagulation Disorders drug therapy, Factor VIII chemistry, Factor VIII therapeutic use, Factor VIIa therapeutic use, Humans, Infant, Male, Recombinant Proteins therapeutic use, Swine, Blood Coagulation Disorders etiology, Factor VIII antagonists & inhibitors
Abstract

Purpose: Inhibitors of factor VIII occur in < or = 20% of severely affected patients with classic hemophilia, but are unusual in nonhemophilic individuals, and have not been reported in very young children. We treated a child with a "high-responding" inhibitor., Patient and Methods: Our patient was an 18-month-old boy who had experienced several episodes of life-threatening hemorrhage. The techniques we used to decrease production of factor VIII in our patient were prolonged small doses of alternate day corticosteroids and continued administration of factor VIII., Results: We controlled the acute bleeding with porcine factor VIII or with recombinant human factor VIIa (rFVIIa). Immune tolerance was successfully achieved using a combination of corticosteroids and daily factor VIII infusions., Conclusions: Multimodal therapy aimed at inducing long-term remission, along with stop-gap measures for hemostasis, may be effective for treating children with this acquired coagulopathy.

Published
1993

10. Regulation of the phosphoenolpyruvate carboxykinase/human factor IX gene introduced into the livers of adult rats by receptor-mediated gene transfer.

Author

Ferkol T, Lindberg GL, Chen J, Perales JC, Crawford DR, Ratnoff OD, and Hanson RW

Subjects
Animals, Asialoglycoprotein Receptor, Base Sequence, Factor IX biosynthesis, Genetic Therapy, Humans, Male, Molecular Sequence Data, Promoter Regions, Genetic, Rats, Rats, Sprague-Dawley, Tumor Cells, Cultured, Factor IX genetics, Liver metabolism, Phosphoenolpyruvate Carboxykinase (GTP) genetics, Receptors, Immunologic physiology, Transfection
Abstract

Gene transfer systems targeting the asialoglycoprotein receptor have been developed to introduce functional genes into cells in culture and livers of intact animals. A synthetic neoglycoprotein carrier was constructed and complexed to a chimeric gene containing the cDNA for human factor IX ligated to the promoter-regulatory region of the gene for phosphoenolpyruvate carboxykinase from the rat. The complex was used to transfect human hepatoma cells that express the asialoglycoprotein receptor. Human factor IX DNA sequences were found in cells 10 days after treatment. A 1.4 kB mRNA transcript was detected by Northern blot hybridization, which was inducible by treatment with dexamethasone or cAMP with theophylline. Western blot hybridization of proteins secreted into the culture medium detected human factor IX. The chimeric gene was also transferred into livers of rats using the neoglycoprotein carrier system after partial hepatectomy. Although the results were variable, the exogenous gene was transcribed in livers of several animals, and maximal levels of expression of the fully processed human factor IX were detected 30 days after introduction. The concentration of factor IX in the blood returned to control levels 60 days after transfection. Factor IX production was induced as late as 96 days after treatment by feeding transfected animals a diet high in protein but devoid of carbohydrates. This DNA carrier system can be used to introduce functional genes into the livers of rats, and may be a useful technique for gene therapy targeting the liver.

Published
1993
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11. Activation of factor XI.

Author

Ratnoff OD

Subjects
Factor XII pharmacology, Humans, Factor XI metabolism, Factor XIa metabolism
Published
1993

13. Some complications of the therapy of hemorrhagic disorders.

Author

Ratnoff OD

Subjects
Acquired Immunodeficiency Syndrome transmission, Blood Transfusion methods, Hepatitis etiology, Humans, Plasma Exchange adverse effects, Platelet Transfusion, Blood Coagulation Disorders therapy, Transfusion Reaction
Abstract

The principal mode for treating disorders of hemostasis is correction of the patient's functional defect by transfusions of appropriate fractions of normal plasma or transfusions of platelets. Two major complications of such therapy are the transmission of infectious diseases, particularly hepatitis and the acquired immune deficiency syndrome (AIDS), and the development of antibodies against clotting factors that are deficient in the patient's plasma. Measures that reduce the occurrence of infection include careful selection of donors, fractionation of plasma with the help of monoclonal antibodies, and treatment of plasma or its fractions with heat or with virus-inactivating organic solvents. No technique of preparing or administering blood or its components can prevent the emergence of antibodies against clotting factors. Desensitization by repeated infusions of antigen, for example, antihemophilic factor, however, appears to result in remission in some patients.

Published
1993
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14. Why does the blood not coagulate?

Author

Ratnoff OD

Subjects
Factor VII antagonists & inhibitors, Factor XII physiology, Humans, Lipoproteins physiology, Protease Inhibitors, Thrombin physiology, Thromboplastin antagonists & inhibitors, Blood Coagulation physiology
Published
1993

15. Inhibition of the activation of hageman factor (factor XII) by eosinophils and eosinophilic constituents.

Author

Ratnoff OD, Gleich GJ, Shurin SB, Kazura J, Everson B, and Embury P

Subjects
Blood Proteins pharmacology, Ellagic Acid antagonists & inhibitors, Ellagic Acid pharmacology, Eosinophil Granule Proteins, Eosinophil Peroxidase, Eosinophil-Derived Neurotoxin, Eosinophils metabolism, Factor XII physiology, Gallic Acid analogs & derivatives, Gallic Acid pharmacology, Humans, Neurotoxins pharmacology, Organometallic Compounds pharmacology, Peroxidases pharmacology, Sulfoglycosphingolipids pharmacology, Eosinophils physiology, Factor XII antagonists & inhibitors, Ribonucleases
Abstract

Several syndromes characterized by striking eosinophilia may be complicated by thrombosis. The experiments described indicate that, paradoxically, eosinophils and certain of their constituents inhibit the activation of Hageman factor (HF, factor XII). In earlier studies, suspensions of mixed types of granulocytes, other nucleated peripheral blood cells, and platelets inhibited activation of Hageman factor by ellagic acid, glass, and sulfatides. After these cells were sedimented by centrifugation, the supernatant fluids were also inhibitory. No attempt had been made earlier to distinguish among different granulocytic species. In the present study, suspensions of eosinophils and the supernatant fluid after eosinophils had been separated by centrifugation inhibited activation of Hageman factor by ellagic acid. The protein concentration of that amount of supernatant fluid that inhibited activation by about half was 16 micrograms/ml, approximately the same as had been described for suspensions of peripheral blood mononuclear cells. Activation of Hageman factor by ellagic acid was also inhibited by certain constituents of eosinophils, including eosinophil peroxidase, eosinophil major basic protein and eosinophil cationic protein. Inhibition was not specific for ellagic acid-induced activation of Hageman factor, as inhibition was also observed with sulfatide-induced activation. Inhibition was presumably related to neutralization of the negative charge of activators of Hageman factor. Thus, bismuth subgallate, a particulate activator of Hageman factor, was no longer effective after it had been exposed to eosinophil cationic protein. The observations reported here raise the question of whether in vivo eosinophils modulate certain of the defense reactions ascribed to Hageman factor.

Published
1993
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16. Induction of expression of monocyte interleukin 1 by Hageman factor (factor XII).

Author

Toossi Z, Sedor JR, Mettler MA, Everson B, Young T, and Ratnoff OD

Subjects
Enzyme Activation, Gene Expression drug effects, Humans, In Vitro Techniques, Interleukin-1 chemistry, Interleukin-1 genetics, Interleukin-6 biosynthesis, RNA, Messenger genetics, Solubility, Factor XII pharmacology, Interleukin-1 metabolism, Monocytes metabolism
Abstract

The results reported here indicate that activated species of Hageman factor (HF, factor XII), a protein that mediates blood clotting, fibrinolysis, and activation of the complement cascade, induce elaboration of interleukin 1 (IL-1) by human monocytes. Augmentation of IL-1 production in mononuclear cell cultures was observed when HF was present along with lipopolysaccharide (LPS) but was not observed with HF alone. Furthermore, antiserum to HF abrogated the enhancement of IL-1 in cultures containing HF and LPS. Total IL-1 activity, which represents secreted and cell-associated IL-1, was enhanced in LPS-stimulated mononuclear cultures by HF. In the absence of LPS, the initial activation product of HF, HFa, which contains the serine protease enzyme activity and the surface-binding domains of the protein, induced IL-1 beta protein and mRNA. In the presence of LPS, the enzymatic moiety (HFf), which is also contained in HF and HFa, amplified IL-1 production. Induction and amplification of monocyte IL-1 by HF provides further evidence for establishing a role for HF in the acute-phase reaction and the cellular immune response.

Published
1992
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17. Inhibition of the activation of Hageman factor (factor XII) by extracts of Schistosoma mansoni.

Author

Foster CB, Flanigan TP, DeStigter KK, Blanton R, Dumenco LL, Gallagher C, and Ratnoff OD

Subjects
Animals, Ellagic Acid pharmacology, Factor XIIa antagonists & inhibitors, Sulfoglycosphingolipids pharmacology, Factor XII antagonists & inhibitors, Schistosoma mansoni metabolism
Abstract

How intravascular helminth parasites evade host hemostatic defense mechanisms and survive within the circulating blood has not been adequately explained. Previous reports have described an inhibitor of the intrinsic clotting pathway in extracts of adult Schistosoma mansoni. Using a purified preparation of Hageman factor, we examined the ability of schistosome extracts and secretory products to inhibit the activation of human Hageman factor (factor XII) in an amidolytic assay. Both schistosome extracts and secretory products inhibited the activation of purified Hageman factor by more than 95%. Schistosome extracts inhibited activation of Hageman factor both by ellagic acid and by bovine sulfatides. In contrast, activated Hageman factor retained full activity in the presence of schistosome extracts as tested both on an amidolytic synthetic substrate and a natural substrate, plasma thromboplastin antecedent (factor XI). Our findings indicate that extracts and secretory products of adult Schistosoma mansoni contain a potent inhibitor of the activation of Hageman factor. Knowledge of a site at which schistosomes inhibit the intrinsic clotting pathway provides added insight into the mechanisms by which the parasites avoid the host hemostatic defense mechanisms.

Published
1992

18. Some clotting factors in plasma during danazol therapy: free and total protein S, but not C4b-binding protein, are elevated by danazol therapy.

Author

Thorisdottir H, Evans JA, Schwartz HJ, Comp P, Haluschak J, and Ratnoff OD

Subjects
Adult, Endometriosis drug therapy, Female, Humans, Male, Protein S, Blood Coagulation Factors metabolism, Carrier Proteins metabolism, Complement C4b metabolism, Complement Inactivator Proteins, Danazol therapeutic use, Endometriosis blood, Glycoproteins metabolism, alpha 1-Antitrypsin Deficiency
Abstract

Anabolic steroids are known to increase the plasma concentrations of certain plasma proteins. In four patients given treatment with danazol, an attenuated androgen, the concentrations of heparin cofactor II, Hageman factor (factor XII), protein C, and both free and total protein S increased significantly when tested 39 to 103 days after the start of therapy. The titers of these proteins in samples obtained 21 days to 5 years after therapy was discontinued were similar to those before treatment, except for total protein S, the titer of which remained elevated. No significant changes in the titers of C4b binding protein or plasma plasmin inhibitory activity were found.

Published
1992

19. Inhibition of the activation of Hageman factor (factor XII) by aprotinin (Trasylol)

Author

Laurel MT, Ratnoff OD, and Everson B

Subjects
Ellagic Acid antagonists & inhibitors, Ellagic Acid pharmacology, Enzyme Activation drug effects, Factor X metabolism, Glass, Humans, In Vitro Techniques, Sulfoglycosphingolipids antagonists & inhibitors, Sulfoglycosphingolipids pharmacology, Aprotinin pharmacology, Blood Coagulation drug effects, Factor XII metabolism
Abstract

Aprotinin (Trasylol; Bayer AG, Leverkusen, Germany), a protease inhibitor resembling or identical with Kunitz' pancreatic trypsin inhibitor, is said to have anticoagulant properties, but these are not clearly defined. The present study provides evidence that one action of aprotinin is inhibition of the activation of Hageman factor (factor XII).

Published
1992

20. Inhibition of the activation of Hageman factor (factor XII) by human vascular endothelial cell culture supernates.

Author

Ratnoff OD, Everson B, Embury P, Ziats NP, Anderson JM, Emanuelson MM, and Malemud CJ

Subjects
Cells, Cultured, Culture Media, Endothelium, Vascular cytology, Enzyme Activation, Factor XII antagonists & inhibitors, Gallic Acid analogs & derivatives, Gallic Acid pharmacology, Humans, Kinetics, Organometallic Compounds pharmacology, Saphenous Vein, Sulfoglycosphingolipids pharmacology, Trypsin metabolism, Trypsin pharmacology, Umbilical Veins, Endothelium, Vascular physiology, Factor XII metabolism
Abstract

The supernatant fluid (conditioned medium) of cultured human vascular endothelial cells inhibits activation of Hageman factor (factor XII), whether by ellagic acid, bovine brain sulfatides, or bismuth subgallate; inhibition appears to be a property of one or more proteins in the culture supernates. This phenomenon may contribute to maintaining the fluidity of circulating blood by inhibiting surface activation of the intrinsic pathway of coagulation.

Published
1991
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21. Inhibition of the activation of Hageman factor (factor XII) by soluble human placental collagens types III, IV, and V.

Author

Koenig JM, Chahine A, and Ratnoff OD

Subjects
Blood Coagulation drug effects, Collagen classification, Collagen metabolism, Dose-Response Relationship, Drug, Ellagic Acid antagonists & inhibitors, Ellagic Acid pharmacology, Glass, Humans, Microbial Collagenase pharmacology, Osmolar Concentration, Solubility, Collagen pharmacology, Factor XII antagonists & inhibitors, Placenta metabolism
Abstract

The initial step in the formation of thrombin via the intrinsic pathway is the activation of Hageman factor (factor XII). Some, but not all, studies have shown that this activation may be brought about by collagen. We examined the effect of three types of soluble human placental collagen on Hageman factor. Collagen types III, IV, and V did not appear to activate Hageman factor under the conditions tested. To the contrary, these collagen species inhibited activation of Hageman factor by glass or ellagic acid. These studies suggest that some types of collagen may play an inhibitory role in blood coagulation.

Published
1991

22. Mitogenic effects of coagulation factor XII and factor XIIa on HepG2 cells.

Author

Schmeidler-Sapiro KT, Ratnoff OD, and Gordon EM

Subjects
Antibodies pharmacology, Antigens immunology, Carcinoma, Hepatocellular metabolism, Cell Division drug effects, DNA biosynthesis, Epidermal Growth Factor immunology, Factor XII immunology, Humans, L Cells cytology, Liver Neoplasms metabolism, Tumor Cells, Cultured, Carcinoma, Hepatocellular pathology, Factor XII pharmacology, Factor XIIa pharmacology, Liver Neoplasms pathology, Mitogens
Abstract

The structure of coagulation factor XII (Hageman factor), inferred from its DNA sequence, includes two epidermal growth factor (EGF)-homologous domains in its amino-terminal region. This suggests that factor XII may exhibit EGF-like activities. Reciprocal antigenic cross-reactivity between factor XII and EGF was shown by exposing purified human factor XII or mouse EGF to anti-mouse EGF or anti-human factor XII. Western blot analysis showed that anti-mouse EGF recognized intact factor XII at 80 kDa. Together, these results suggest that the EGF-homologous domains are accessible for anti-EGF binding in native factor XII. To determine whether factor XII has mitogenic activity, HepG2 or L cells (10(4) cells per well) were grown in serum-free medium in the presence or absence of factor XII or kaolin-activated factor XII (factor XIIa). Both factors XII and XIIa (6.0 micrograms/ml) enhanced cell proliferation by approximately 2-fold (P less than 0.001 and P less than 0.005, respectively). In contrast, L cells, which are not EGF target cells, were not affected by either factor XII or factor XIIa. Various doses of factor XII enhanced cell proliferation, [3H]thymidine incorporation, and [3H]leucine incorporation in HepG2 cells cultured under the same conditions. These data indicate that factor XII, like EGF, is a mitogen for HepG2 cells and suggest a possible autocrine role in the liver.

Published
1991
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23. Inhibition of the activation of Hageman factor (factor XII) and of platelet aggregation by extracts of Brugia malayi microfilariae.

Author

Foster CB, Flanigan TP, Kazura JW, Dumenco LL, and Ratnoff OD

Subjects
Adenosine Diphosphate pharmacology, Adult, Animals, Arachidonic Acid, Arachidonic Acids pharmacology, Blood Coagulation drug effects, Collagen pharmacology, Ellagic Acid pharmacology, Humans, In Vitro Techniques, Male, Partial Thromboplastin Time, Platelet Aggregation Inhibitors pharmacology, Trypsin pharmacology, Brugia pathogenicity, Factor XII antagonists & inhibitors, Platelet Aggregation drug effects
Abstract

In human filariasis, large numbers of blood-borne microfilariae circulate unimpeded through the blood stream. How intravascular filarial parasites avoid precipitating thrombosis has not been studied in detail. We hypothesized that extracts of Brugia malayi microfilariae would contain factors that inhibit activation of hemostatic mechanisms. Initial studies demonstrated an inhibitor specific for the intrinsic coagulation cascade. The addition of microfilarial extracts to human plasma prolonged the activated partial thromboplastin time in a dose-dependent fashion but did not prolong the prothrombin, thrombin, or Russell's viper venom times. Microfilarial extracts (0.1 mg/ml) completely inhibited activation of Hageman factor (factor XII, at 0.05 U/ml) as measured in an amidolytic assay. Hageman factor previously activated by ellagic acid (factor XIIa) retained full enzymatic activity in the presence of microfilarial extract (0.1 mg/ml). The presence of inhibitory activity in the culture medium of live parasites raises the possibility that microfilariae secrete an inhibitory protein into their local environment. Microfilarial extracts at a final concentration of 0.1 mg/ml also inhibited collagen- and adenosine diphosphate-induced platelet aggregation. Arachidonic acid-induced platelet aggregation was inhibited by microfilarial extracts at a final concentration of 0.6 mg/ml. These results suggest that microfilariae of Brugia malayi, a human filarial parasite, may avoid initiating thrombosis through inhibition of the intrinsic coagulation pathway and platelet aggregation.

Published
1991

25. The changing prognosis of classic hemophilia (factor VIII "deficiency").

Author

Jones PK and Ratnoff OD

Subjects
Acquired Immunodeficiency Syndrome complications, Acquired Immunodeficiency Syndrome mortality, Adolescent, Adult, Aged, Aged, 80 and over, Child, Child, Preschool, Hemophilia A complications, Hemophilia A history, History, 20th Century, Humans, Infant, Life Tables, Male, Middle Aged, Prognosis, Retrospective Studies, Risk, Severity of Illness Index, Survival Analysis, United States epidemiology, Hemophilia A mortality, Longevity
Abstract

Objective: To estimate relative risk of mortality and median life expectancy for patients with classic hemophilia by a life-table analysis, taking into account deaths that may have occurred in infancy or childhood before the onset of symptoms., Design: Retrospective chart review of clinical series., Setting: Referral-based university medical center., Patients: Seven hundred one patients with classic hemophilia (hemophilia A; factor VIII "deficiency") were studied for the years from 1900 to 1990; patients were identified in 289 families., Measurements and Main Results: Relative risk for mortality and median life expectancy among hemophiliacs were compared with those among normal U.S. males. Overall, mortality (relative to that of contemporaneous U.S. males) was increased about sixfold among severely affected patients, more than twofold among moderately affected patients, and was equivalent to that of U.S. males among mildly affected patients. Median life expectancy at 1 year of age had reached almost 68 years in the decade 1971 to 1980, but declined to only 49 years in the decade 1981 to 1990., Conclusions: After improvement in survival from 1971-1980 (corresponding to widespread treatment with lyophilized concentrates of antihemophilic factor [factor VIII]), relative mortality is now increasing, especially among severely affected patients, in large measure because of the acquired immunodeficiency syndrome (AIDS).

Published
1991
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26. Fibrinolysis, thrombocytopenia, and coagulation abnormalities complicating high-dose interleukin-2 immunotherapy.

Author

Fleischmann JD, Shingleton WB, Gallagher C, Ratnoff OD, and Chahine A

Subjects
Adult, Aged, Humans, Middle Aged, Platelet Count drug effects, Blood Coagulation Disorders chemically induced, Fibrinolysis drug effects, Immunotherapy adverse effects, Interleukin-2 adverse effects, Thrombocytopenia chemically induced
Abstract

High-dose interleukin-2 (IL-2) immunotherapy can cause hypotension, respiratory distress, interstitial edema, and thrombocytopenia, similar to endotoxic shock. We have observed that IL-2 has no direct effect on coagulation factors in vitro, but it has been observed to alter the coagulant properties of vascular endothelium. Accordingly, we investigated the possibility that IL-2 infusions initiate plasma fibrinolysis and disseminated intravascular coagulation (DIC). We studied the clinical course, platelet count, and coagulation profile in response to IL-2 infusion in seven patients, two with metastatic melanoma and five with metastatic renal cell carcinoma. Every patient experienced hemodynamic instability and thrombocytopenia, and one patient suffered an unusual complication, mesenteric thrombosis. No patient had appreciable changes in the prothrombin time or the partial thromboplastin time, nor did factors V or VIII decline in the two patients observed. In four patients examined, we found decreased titers of Hageman factor (factor XII), high molecular weight kininogen, prekallikrein, and plasma thromboplastin antecedent, as if these had been consumed by reactions of the intrinsic pathway of thrombin formation. Circulating D-dimer fragments were found in the plasma of every patient at some point during each infusion cycle, and we observed decreased titers of plasminogen in the four patients just mentioned, suggesting that IL-2 infusions initiated fibrinolysis. Taken together, the clotting factor derangements and related toxicity phenomena cannot be ascribed firmly to DIC. Activation of the intrinsic (contact) system of coagulation, however, may provide one link between the vascular endothelial surface alterations caused by IL-2 infusions and the development of the systemic toxicity that resembles septic shock.

Published
1991

27. Adsorption of Hageman factor (factor XII) and other human plasma proteins to biomedical polymers.

Author

Ziats NP, Pankowsky DA, Tierney BP, Ratnoff OD, and Anderson JM

Subjects
Adsorption, Dimethylpolysiloxanes, Fibrinogen chemistry, Fibronectins chemistry, Hemoglobins chemistry, Humans, Immunoglobulin G chemistry, Immunohistochemistry, Kinetics, Microscopy, Electron, Scanning, Polyethylene Terephthalates, Polyethylenes, Polytetrafluoroethylene, Radioimmunoassay, Serum Albumin chemistry, Silicone Elastomers, Silicones, Biocompatible Materials, Blood Proteins chemistry, Factor XII chemistry, Polymers
Abstract

Protein adsorption to surfaces occurs whenever blood comes into contact with biomaterials, prosthetic devices, and artificial organs. The plasma protein Hageman factor (factor XII) present at the interface between blood and foreign surfaces can be qualitatively and quantitatively detected after in vitro perfusion of anticoagulated human blood through important biomedical polymers. We have determined protein adsorption by a modified radioimmunoassay and by scanning electron microscopy using immunogold labeling techniques. The materials used included vascular graft materials (Dacron and expanded polytetrafluoroethylene) and the National Heart, Lung, and Blood Institute-Devices and Technology Branch reference materials polydimethylsiloxane, polyethylene, and silicone rubber. Factor VIII-von Willebrand factor, another trace plasma protein, and other plasma proteins such as fibrinogen, immunoglobulin G, albumin, fibronectin, and hemoglobin were also detected at the blood-contacting surface. At physiologic flow rates, the adsorption of these proteins from the circulating blood to the surface of these materials appears to be a function of time, with certain materials, as well as of the physical and chemical characteristics of the material surface. Hageman factor adsorption to surfaces, quantified under static conditions, occurs at nanogram concentrations. These data suggest that trace proteins, such as those important in the activation of the coagulation cascade, can significantly affect the blood compatibility or thrombogenicity of an implanted device.

Published
1990

28. Notes on clotting in a Burmese python (Python molurus bivittatus).

Author

Ratnoff OD, Rosenberg MJ, Everson B, Emanuelson M, and Tulodziecki N

Subjects
Animals, Blood Coagulation Factors analysis, Hemostatics analysis, Humans, Indicators and Reagents, Prothrombin Time, Species Specificity, Blood Coagulation, Snakes physiology
Abstract

Studies of the clotting mechanisms in the plasma of a Burmese python (Python molurus bivittatus) confirm earlier information that both extrinsic and intrinsic pathways of thrombin formation participate in reptilian hemostasis. Plasma fibrinogen was present at a concentration comparable to that in human plasma. Other assays were hampered by the need to use nonreptilian reagents. The activated partial thromboplastin time was shorter than was that of human plasma, thus implying the presence of prothrombin in python plasma; however, this protein could be demonstrated only in trace amounts. Similarly, only small amounts of Hageman factor (factor XII) and antihemophilic factor (factor VIII) were detected, and none of plasma prekallikrein, high-molecular-weight kininogen, and Christmas factor (factor IX). The prothrombin time was slower than that of human plasma. Factor VII was not detected, but both proaccelerin (factor V) and Stuart factor (factor X) were present. Python plasma inhibited bovine thrombin and human plasmin, but it was deficient in fibrinolytic capacity.

Published
1990

29. Morphologic characteristics of adsorbed human plasma proteins on vascular grafts and biomaterials.

Author

Pankowsky DA, Ziats NP, Topham NS, Ratnoff OD, and Anderson JM

Subjects
Adsorption, Blood Proteins ultrastructure, Dimethylpolysiloxanes, Factor VIII analysis, Factor XII analysis, Fibrinogen analysis, Humans, Immunoglobulin G analysis, Materials Testing, Polyethylenes, Polytetrafluoroethylene, Serum Albumin analysis, Silicones, von Willebrand Factor analysis, Biocompatible Materials, Blood Proteins analysis, Blood Vessel Prosthesis
Abstract

Protein adsorption on the surfaces of clinically significant prosthetic vascular graft materials from human whole blood was independent of plasma concentration as determined morphologically by use of immunogold labels. Some proteins, such as fibrinogen, adsorbed in a multilayer pattern on expanded polytetrafluoroethylene and had a preference for particular surface features of the polymer. Other proteins, such as Hageman factor (factor XII), showed diffuse adsorption patterns. Physiologically significant proteins that have not been well studied, such as immunoglobulin G and factor VIII, adsorbed readily to the surface of expanded polytetrafluoroethylene. This finding may be significant since adsorbed proteins may activate coagulation mechanisms and immunologic responses, including platelet and monocyte adhesion and activation. Any human blood protein for which an antibody has been developed can be studied by use of this technique.

Published
1990

30. Interactions of C1(-)-inhibitors from normal persons and patients with type II hereditary angioneurotic edema with purified activated Hageman factor (factor XIIa).

Author

Donaldson VH, Mitchell BH, Everson B, and Ratnoff OD

Subjects
Angioedema congenital, Electrophoresis, Polyacrylamide Gel, Factor XII isolation & purification, Humans, Angioedema blood, Complement C1 Inactivator Proteins metabolism, Factor XII metabolism
Abstract

Activated high molecular weight Hageman factor (75 Kd) and Hageman factor carboxy-terminal fragments both formed complexes with purified C1(-)-inhibitor, but the Hageman factor fragments appeared to have a higher affinity for the C1(-)-inhibitor than activated Hageman factor. Therefore, the clot-promoting activity of activated Hageman factor might be relatively unimpaired if Hageman factor fragments are also present. Normal C1(-)-inhibitor was cleaved by Hageman factor fragments. Clot-promoting activity was not generated in Hageman factor by exposure to Hageman factor fragments, nor was Hageman factor cleaved by Hageman factor fragments. When Hageman factor was cleaved by streptokinase-activated plasminogen, a 40 Kd fragment was released. In contrast to their interactions with other proteinases, which are blocked by normal C1(-)-inhibitor, Type II C1(-)-inhibitors from plasmas of affected members of eight different kindred with this form of hereditary angioneurotic edema all inhibited the specific coagulant activity of activated Hageman factor to some degree. They did not all form complexes with activated Hageman factor that were stable during sodium dodecyl sulfate-polyacrylamide gel electrophoresis.

Published
1990

31. Cabbage seed protease inhibitor: a slow, tight-binding inhibitor of trypsin with activity toward thrombin, activated Stuart factor (factor Xa), activated Hageman factor (factor XIIa), and plasmin.

Author

Carter TH, Everson BA, and Ratnoff OD

Subjects
Protease Inhibitors isolation & purification, Protein Binding, Seeds enzymology, Trypsin Inhibitors isolation & purification, Trypsin Inhibitors pharmacology, Brassica enzymology, Factor XIIa antagonists & inhibitors, Factor Xa Inhibitors, Fibrinolysin antagonists & inhibitors, Protease Inhibitors metabolism, Thrombin antagonists & inhibitors, Trypsin metabolism
Abstract

An inhibitor of procoagulant and fibrinolytic enzymes was derived from cabbage seeds by a procedure using acetone precipitation, ion-exchange chromatography, and gel filtration. The cabbage seed inhibitor was a 10-Kd monomeric protein with intrachain disulfide bonds. This preparation prevented clot formation in whole blood and blocked the ability of thrombin to induce clot formation in plasma and to induce platelet aggregation. A number of proteases were inhibited, as demonstrated by using purified enzymes in amidolytic assays. Tight-binding inhibition was observed for activated Stuart factor (factor Xa) and plasmin. Inhibition of thrombin and activated Hageman factor (factor XIIa) was observed with a molar excess of inhibitor. No inhibition was detected for activated plasma thromboplastin antecedent (factor XIa), plasma kallikrein, or C1 esterase. Reaction progress curves for trypsin indicated slow, tight-binding inhibition, with an apparent inhibition constant in the nanomolar range or less. The electrophoretic mobility of trypsin was altered by the inhibitor in nondenaturing polyacrylamide gel electrophoresis (PAGE) but not in sodium dodecyl sulfate (SDS)-PAGE, indicating noncovalent bonding. Only partial reversal of trypsin inhibition could be demonstrated by washing the inhibitor from enzyme immobilized on solid beads. A dot-blot technique with cabbage seed inhibitor was capable of detecting 10 ng nitrocellulose-bound trypsin. The dot-blot technique also appeared capable of detecting plasmin. These findings demonstrated the potential utility of this inhibitor as a probe for detection of tightly bound proteases. In summary, cabbage seed extracts contain an inhibitor with activity toward a broad range of proteases important to hemostasis. To our knowledge, this agent represents the first inhibitor isolated from a plant source that inhibits thrombin.

Published
1990

32. The Arthus reaction in cats deficient in Hageman factor (factor XII).

Author

Kier AB, McDonnell JJ, Stern A, and Ratnoff OD

Subjects
Animals, Arthus Reaction pathology, Biopsy, Cats, Chickens blood, Erythrocyte Transfusion, Female, Hemagglutination, Male, Skin pathology, Skin Tests, Arthus Reaction etiology, Factor XII Deficiency complications
Abstract

A study was made of the Arthus reaction in an animal model of Hageman-factor deficiency, namely Hageman trait cats, and in control cats with normal Hageman-factor activity. At three time points, there was a significant decrease (P less than 0.01) in the size of the cutaneous Arthus reaction to chicken red blood cells in biopsies from Hageman trait cats compared with the reaction in biopsies from control animals. Injection of a positive control, histamine, and a negative control, phosphate-buffered saline, produced no significant differences between the two groups. Hageman trait cats had a significant decrease (P less than 0.001) in the number of neutrophils in the skin lesions compared with controls. When Hageman trait cats were injected intravenously with purified cat Hageman factor, Arthus reactions were similar to those observed in control cats.

Published
1990
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33. Studies on some coagulation factors (Hageman factor, plasma prekallikrein, and high molecular weight kininogen) in the normal newborn.

Author

Gordon EM, Ratnoff OD, Saito H, Gross S, and Jones PK

Subjects
Antigens analysis, Blood Coagulation drug effects, Factor XII analysis, Humans, Kininogens blood, Molecular Weight, Partial Thromboplastin Time, Prekallikrein analysis, Blood Coagulation Factors analysis, Infant, Newborn
Abstract

Normal newborn infants have a prolonged partial thromboplastin time compared to that of older infants or adults. This finding has been related to combined deficiencies of multiple clotting factors, with the exception of proaccelerin (factor V) and antihemophilic factor (factor VIII). The present study confirms the presence of decreased titers of Hageman factor (HF, factor XII), plasma prekallikrein, and high molecular weight kininogen during the neonatal period, as demonstrated in clotting assays; the degree of these relative deficiencies is usually such that only the low titer of HF appears to contribute significantly to the abnormally long PTT. Additionally, procoagulant titers of HF and plasma prekallikrein were relatively lower than the concentration of these factors determined immunologically. The mechanisms underlying this phenomenon are not known.

Published
1980

34. Activation of Hageman factor (factor XII) by sulfatides and other agents in the absence of plasma proteases.

Author

España F and Ratnoff OD

Subjects
Aniline Compounds pharmacology, Animals, Blood Coagulation drug effects, Cattle, Ellagic Acid pharmacology, Glass, Humans, Immunoglobulin G pharmacology, Kaolin pharmacology, Partial Thromboplastin Time, Stimulation, Chemical, Factor XII physiology, Peptide Hydrolases deficiency, Sulfoglycosphingolipids pharmacology
Abstract

Incubation of purified human HF (factor XII) with sulfatides, EA, kaolin, or glass resulted in the generation of amidolytic activity in the apparent absence of other enzymes. Sulfatides or EA rapidly and efficiently initiated intrinsic coagulation in normal plasma but, under the conditions tested, only trivially corrected the prolonged partial thromboplastin clotting times of plasma deficient in prekallikrein or HMWK. Preliminary incubation of HF with crude IgG directed against plasma kallikrein or SBTI did not influence the results. The presence of albumin greatly enhanced activation of the amidolytic properties of purified HF by EA, even when albumin had been lipid-extracted or treated with DFP or SBTI; albumin also increased activation of HF by sulfatides. Internal cleavage and minimal scission of the HF molecule accompanied the generation of amidolytic properties in mixtures of HF and sulfatides; cleavage was not blocked by SBTI. These experiments demonstrate that negatively charged substances can activate HF in absence of other enzymes and that this activation is accompanied by formation of a two-chain species of HF.

Published
1983

35. Heparin cofactor II activity in plasma during pregnancy and oral contraceptive use.

Author

Massouh M, Jatoi A, Gordon EM, and Ratnoff OD

Subjects
Adult, Contraceptives, Oral administration & dosage, Female, Humans, Contraceptives, Oral metabolism, Heparin Cofactor II analysis, Pregnancy blood
Abstract

Inhibition of thrombin by heparin is mediated by at least two plasma proteins, antithrombin III, and heparin cofactor II. The plasma titer of heparin cofactor II was significantly elevated in both pregnant women and users of oral contraceptives.

Published
1989

36. Impaired cell-mediated immunity in patients with classic hemophilia.

Author

Lederman MM, Ratnoff OD, Scillian JJ, Jones PK, and Schacter B

Subjects
Adult, Factor VIII adverse effects, Factor VIII therapeutic use, Fibrinogen adverse effects, Fibrinogen therapeutic use, Freeze Drying, Hemophilia A blood, Hemophilia A complications, Hemophilia A therapy, Humans, Immunity, Cellular, Killer Cells, Natural immunology, Leukocyte Count, Lymphocyte Activation, Male, Rosette Formation, T-Lymphocytes immunology, T-Lymphocytes, Helper-Inducer immunology, T-Lymphocytes, Regulatory immunology, Hemophilia A immunology, Immunologic Deficiency Syndromes etiology
Published
1983
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38. Sources of variability in antihemophilic factor (factor VIII) procoagulant titers and precipitating antigen levels among obligate carriers of classic hemophilia.

Author

Jones PK and Ratnoff OD

Subjects
Adolescent, Adult, Aging, Chemical Precipitation, Female, Hemophilia A genetics, Hemophilia A immunology, Humans, Male, Mathematics, Middle Aged, Antigens, Blood Coagulation, Factor VIII immunology, Genetic Carrier Screening
Abstract

Chediak et al. have reported that the titer of procoagulant antihemophilic factor (AHF:C; factor VIII:C) was significantly lower in obligate carriers of classic hemophilia who were daughters of affected men (paternal carriers) than in those whose fathers were normal by history (maternal carriers). In contrast, among 113 obligate carriers of hemophilia, no significant difference in procoagulant AHF titers was observed between paternal and maternal carriers. The concentration of AHF-like precipitating antigens, however, was significantly higher in maternal than in paternal carriers. This difference may have reflected in part the greater severity of disease in affected males in the families of maternal carriers.

Published
1981

40. Tendency to serious sequelae of infection with the human immunodeficiency virus in sibships with hemophilia.

Author

Meropol NJ, Krause PR, Ratnoff OD, Eyster ME, Levine PH, White GC, Debanne S, Rowland D, and Lederman MM

Subjects
Acquired Immunodeficiency Syndrome transmission, Hematologic Diseases genetics, Hemophilia A genetics, Humans, Male, Risk Factors, Acquired Immunodeficiency Syndrome complications, Hematologic Diseases etiology, Hemophilia A therapy
Abstract

Cofactors for the clinical expression of infection due to the human immunodeficiency virus (HIV) are not well understood. We asked if there was a familial tendency to the development of complications of HIV infection. We examined 35 hemophilic sibships in which at least two brothers with classic hemophilia (factor VIII deficiency) were infected with HIV. Twenty-four (34%) of the 70 patients had serious sequelae of infection, and 46 (66%) were asymptomatic or had only lymph node enlargement. Using Fisher's exact test, we found the concordance among siblings for serious sequelae of HIV infection was greater than would be expected by chance. When analysis was restricted to include only siblings known to be infected for more than two years, this concordance was still present. In the study population, birth order and mean yearly usage of factor VIII concentrate were unrelated to the outcome of HIV infection. The data indicate a familial tendency to serious complications of HIV infection. The factor(s) responsible for this familial tendency are currently under investigation.

Published
1989

41. Surface-mediated defenses against injury.

Author

Ratnoff OD

Subjects
Angioedema blood, Animals, Ellagic Acid pharmacology, Factor XI physiology, Fibrinolysin physiology, Humans, Kallikreins blood, Kallikreins physiology, Kinins physiology, Thrombosis blood, Blood Coagulation, Factor XII physiology
Published
1983

42. Elevated antihemophilic factor (AHF, factor VIII) procoagulant activity and AHF-like antigen in alcoholic cirrhosis of the liver.

Author

Green AJ and Ratnoff OD

Subjects
Adult, Aged, Animals, Blood Coagulation Tests, Humans, Immune Sera, Immunodiffusion, Immunoelectrophoresis, Immunologic Techniques, Liver Cirrhosis etiology, Liver Cirrhosis immunology, Male, Middle Aged, Rabbits immunology, Alcoholism complications, Antigens analysis, Factor VIII analysis, Liver Cirrhosis blood
Published
1974

43. The secondary structure of human Hageman factor (factor XII) and its alteration by activating agents.

Author

McMillin CR, Saito H, Ratnoff OD, and Walton AG

Subjects
Adsorption, Amino Acids analysis, Chemical Phenomena, Chemistry, Circular Dichroism, Electrophoresis, Disc, Electrophoresis, Polyacrylamide Gel, Humans, Hydrochloric Acid, Hydrogen-Ion Concentration, Molecular Conformation, Peptides, Sodium Hydroxide, Temperature, Benzopyrans, Factor XII analysis, Quartz, Silicon Dioxide, Trypsin
Abstract

Hageman factor (factor XII) is activated by exposure to surfaces such as glass or by solutions of certain compounds, notably ellagic acid. Changes in the structure of Hageman factor accompanying activation have been examined in this study by circular dichroism spectroscopy. The spectrum of unactivated Hageman factor in aqueous solutions suggests that its conformation is mainly aperiodic. Various perturbants altered the conformation of Hageman factor in differing ways, demonstrating the sensitivity of Hageman factor to its environment. After activation of Hageman factor with solutions of ellagic acid, a negative trough appeared in the region of the circular dichroism spectrum commonly assigned to tyrosine residues, along with other minor changes in the peptide spectral region. Some of these changes are similar to changes that occurred upon partial neutralization of the basic residues at alkali pH. Activation of Hageman factor by adsorption to quartz surfaces (in an aqueous environment) also produced changes similar to those in the ellagic acid-activated Hageman factor, including the negative ellipticity in the tyrosine region. These observations suggest that the activation process may be related to a change in status of some of the basic amino acid residues, coupled with a specific change in the environment of some tyrosine residues. The importance of these changes during the activation process remains to be determined. The sensitivity of Hageman factor to its environment is consistent with the view that the initiation of clotting by exposure of plasma to appropriate agents is brought about by alterations in the conformation of Hageman factor that occur in the apparent absence of Fletcher factor or other recognized clotting factors.

Published
1974
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44. Defective activation of clotting, fibrinolytic, and permeability-enhancing systems in human Fletcher trait plasma.

Author

Saito H, Ratnoff OD, and Donaldson VH

Subjects
Biological Assay, Blood Coagulation drug effects, Blood Coagulation Tests, Buffers, Capillary Permeability, Citrates, Esterases blood, Factor IX analysis, Factor VIII analysis, Factor XI analysis, Factor XII analysis, Factor XII isolation & purification, Fibrinolysis, Humans, In Vitro Techniques, Kaolin pharmacology, Kinins biosynthesis, Thromboplastin analysis, Blood Coagulation Disorders blood
Published
1974
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45. The role of prekallikrein and high-molecular-weight kininogen in the contact activation of Hageman factor (factor XII) by sulfatides and other agents.

Author

España F and Ratnoff OD

Subjects
Ellagic Acid pharmacology, Enzyme Activation, Factor XIIa, Humans, Hydrolysis, Kaolin pharmacology, Male, Molecular Weight, Factor XII biosynthesis, Kallikreins physiology, Kininogens physiology, Peptide Fragments biosynthesis, Prekallikrein physiology, Sulfoglycosphingolipids pharmacology
Abstract

Hageman factor (HF, factor XII), adsorbed to negatively charged agents, is transformed to an activated state in which it initiates reactions of the intrinsic pathway of thrombin formation by activating plasma thromboplastin antecedent (PTA, factor XI). High-molecular-weight kininogen (HMWK, Fitzgerald factor) and plasma prekallikrein accelerate these early steps in the clotting process. Questions have been raised about the role of HMWK in the activation of Hageman factor by surfaces. In the present studies, we report that the activation of purified human HF by sulfatides, ellagic acid, kaolin, or glass occurred in the absence of HMWK. Indeed, small amounts of HMWK inhibited activation of HF by ellagic acid. Physiological concentration of HMWK had little or no influence on the activation of HF by sulfatides, kaolin, or glass, but higher concentrations (3 to 6 times more) showed the same inhibitory effect as after activation by ellagic acid. This inhibitory property of HMWK may be attributed to competitive binding of HF and HMWK on the surface of the activating agents. In fact, when HF was added to kaolin or glass that had been incubated with HMWK and then washed, the inhibitory effect persisted, indicating HMWK that was bound to the surface blocked activation of HF. Studies with 125I-HF and 125I-HMWK supported this interpretation. Plasma prekallikrein accelerated activation of the amidolytic properties of HF by sulfatides, kaolin, or glass but did not influence activation of HF by ellagic acid. In the presence of plasma kallikrein, HMWK at moderate concentrations slightly accelerated the rate of activation of HF by activating agents other than ellagic acid. Higher concentrations of HMWK counteracted both the accelerating effect of prekallikrein and the inhibitory effect observed when HF was incubated with an excess of kaolin. These experiments, then, support the view that the procoagulant function of HMWK is localized to a point subsequent to the activation of HF.

Published
1983

47. Psychogenic purpura (autoerythrocyte sensitization): an unsolved dilemma.

Author

Ratnoff OD

Subjects
Adult, Autoimmune Diseases immunology, Autoimmune Diseases psychology, Female, Humans, Psychophysiologic Disorders immunology, Psychophysiologic Disorders psychology, Purpura immunology, Purpura psychology, Autoimmune Diseases complications, Erythrocytes immunology, Psychophysiologic Disorders complications, Purpura complications
Abstract

Experience at University Hospitals of Cleveland with 71 cases of Gardner and Diamond's syndrome of autoerythrocyte sensitization is reviewed. Gardner and Diamond attributed the pathogenesis of the inflammatory bruises typical of this syndrome to sensitization to the stroma of the patients' own erythrocytes, as demonstrated by reproduction of the lesion on intracutaneous injection of erythrocytic stroma. Nearly all the cases my colleagues and I have seen were in adult women, in whom the onset of inflammatory bruising could often be precisely dated, frequently some weeks after an injury or surgical procedure or, more often, severe emotional stress. Bouts of bruising were often preceded by sensations localized to the affected site. Cutaneous responses to the injection of erythrocytes were erratic. The patients described a wide range of both hemorrhagic and nonhemorrhagic complaints, including, among others, severe headaches, paresthesias, repeated syncope, diplopia (sometimes monocular), and "nervousness." Psychiatric studies indicated that patients had overt depression, sexual problems, feelings of hostility, and obsessive-compulsive behavior. The patients had traits that can be described as typical of a hysterical character disorder. Therapy of autoerythrocyte sensitization--that is, psychogenic purpura--has been difficult; in younger individuals, psychiatric therapy has appeared to be beneficial.

Published
1989

48. A quarter century with Mr. Hageman.

Author

Ratnoff OD

Subjects
Animals, Blood Pressure, Factor XI metabolism, Fibrinolysis, Humans, Kallikreins metabolism, Kininogens physiology, Prekallikrein metabolism, Factor XII metabolism
Published
1980

49. Classic gout in Hageman factor (Factor XII) deficiency.

Author

Green D, Arsever CL, Grumet KA, and Ratnoff OD

Subjects
Extremities, Factor XII, Gout metabolism, Humans, Kinins analysis, Male, Middle Aged, Synovial Fluid analysis, Factor XII Deficiency, Gout complications
Abstract

A 62-year-old man with a typical history of gout was admitted to the hospital with left-sided hemiplegia. His serum uric acid level was 10.3 mg/dL, his partial thromboplastin time was 198 s, and his Hageman factor (factor XII) coagulant activity and antigen were less than 1% of normal. Aspiration of synovial fluid from his inflamed knee disclosed urate crystals and abundant leukocytes but an absence of Hageman factor antigen. The presence of acute gouty arthritis in a patient with Hageman trait challenges the role of Hageman factor in the pathogenesis of gouty arthropathy.

Published
1982

50. Defective esterase and kinin-forming activity in human Fletcher trait plasma. A fraction rich in kallikreinlike activity.

Author

Donaldson VH, Saito H, and Ratnoff OD

Subjects
Aprotinin blood, Arginine, Blood Coagulation drug effects, Blood Coagulation Tests, Bradykinin blood, Citrates, Factor XI analysis, Factor XII analysis, Humans, In Vitro Techniques, Kaolin pharmacology, Kininogens blood, Kinins biosynthesis, Kinins blood, Trypsin pharmacology, Blood Coagulation Disorders enzymology, Esterases blood, Kallikreins blood
Published
1974
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