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HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Laboratoire Sainte Marie, Laboratoire de
Biochimie A, and INSERM E 99-12, Hôtel-Dieu, Paris; Laboratoire
Diféma, Faculté de Médecine et de Pharmacie, Rouen;
INSERM U. 153, Hôpital Saint Louis, Paris; Centre Hospitalier
Régional, Martigues; INSERM U.76, Agence du sang, Paris; Centre
Hopitalier Régional, Alès, France; and TNO-PG, Gaubius
Laboratory, and Pharming, Leiden, The Netherlands.
Congenital homozygous dysfibrinogenemia was diagnosed in a man with
a history of 2 thrombotic strokes before age 30. His hemostatic profile
was characterized by a dramatically prolonged plasma thrombin clotting
time, and no clotting was observed with reptilase. Complete clotting of
the abnormal fibrinogen occurred after a prolonged incubation of plasma
with thrombin. The release of fibrinopeptides A and B by thrombin and
of fibrinopeptide A by reptilase were both normal. Thrombin-induced
fibrin polymerization was impaired, and no polymerization occurred with
reptilase. The polymerization defect was characterized by a defective
site "a," resulting in an absence of interaction between sites A
and a, indicated by the lack of fragment D1 (or fibrinogen)
binding to normal fibrin monomers depleted in fibrinopeptide A only
(Des-AA fm). By SDS-PAGE, the defect was detected on the Fibrinogen is a disulfide-bridged protein of
340 000 d comprised of 2 symmetric half-molecules, each having 3 different polypeptides, designated A During the early stages of the fibrin polymerization process,
protofibrils are stabilized by the factor XIIIa-catalyzed formation of
cross-links between the More than 240 cases of inherited dysfibrinogenemia have been
reported,8 and most were detected because of a prolonged
thrombin clotting time related to a defect in the conversion of
fibrinogen to fibrin. Many of these molecules have abnormalities
located in the carboxyl terminus of the In this study, we report a homozygous case of congenital
dysfibrinogenemia, designated fibrinogen Alès, which is
characterized by amino acid substitution of Asp for Val at position 330 in the Routine hemostasis studies
Whole blood clotting time, recalcification time, 1-stage prothrombin
time, and coagulation factor II, V, and VII + X quantification were
performed by conventional methods reported in Caen et
al.10 Thrombin and reptilase clotting times were
determined using several concentrations of reagents diluted either in
150 mmol/L NaCl or in 25 mmol/L CaCl2. Fibrinogen cofactor
activity in adenosine diphosphate-induced platelet aggregation was
determined using normal washed platelets prepared according to
Patscheke and Worner.11 Plasma fibrinogen concentration
was determined by a functional assay according to
Clauss,12 by an immunologic assay method according to
Mancini et al,13 and by heat precipitation at 56°C as
described previously.14 Fibrinogen-related antigen in
serum was determined by enzyme-linked immunosorbent assay as described by Soria et al.15 Levels of known risk factors recommended
by the International Society of Thrombosis and Haemostasis
(ISTH)16 (protein C, protein S, antithrombin III,
homocysteine, lupus anticoagulant, lipid analysis) were determined in
routine laboratories. Genetic analysis for factor V Leiden was
performed as described by Bertina,17 and prothrombin gene
20210 mutation was conducted as described by Poort et
al.18 Apolipoprotein genotype was performed by gene amplification according to Hixson and Vernier.19
Fibrinogen purification
Analysis of the prolonged thrombin time Fibrin polymerization curves were made according to Bouvier and Gruedlinger.22 Aggregation of fibrin monomer was studied as described by Belitser et al.23 The release of FpA and FpB after thrombin addition to purified fibrinogen (and that of FpA after reptilase addition) was examined by high-performance liquid chromatography (HPLC) as described by Kehl et al.24 Cross-linking of fibrin ( dimerization and  polymerization) was
analyzed by SDS-PAGE according to Weber and Osborn.21
Fibrin stabilized by factor XIIIa was obtained according to Schwartz et
al.25
Plasmin digests of fibrinogen Plasmin degradation of fibrinogen was performed in the presence of 5 mmol/L CaCl2 or 10 mmol/L EDTA, according to Haverkate and Timan.26 The samples were loaded onto a 10% or 7.5% SDS-PAGE gel according to Laemmli.27Binding of purified fragment D1 (or of fibrinogen) to immobilized normal fibrin monomers depleted in fibrinopeptide A (Des-AA fm) Purification of fragment D1. Purified normal fibrinogen and fibrinogen Alès were degraded with plasmin (final concentration, 2 U/mL) in the presence of 5 mmol/L CaCl2 for 4 hours at 37°C. The digests were chromatographed on Sepharose-Lysine (Pharmacia, Uppsala, Sweden) to remove plasmin. After an extensive dialysis against 100 mmol/L Tris-HCl, pH 8.6, the fragment D1 was isolated by DEAE cellulose chromatography as described by Nilehn.28 The purity of fragment D1 was tested by SDS-PAGE, and its concentration was calculated from absorbance at 280 nm (A, 1%; 1 cm = 11.20). Preparation of Des-AA fm. Normal human fibrinogen (Kabi AB, Stockholm, Sweden) at 5 mg/mL was clotted with 0.2 U/mL reptilase in the presence of 5 mmol/L EDTA for 30 minutes at 37°C. The fibrin clot was collected, washed extensively with 150 mmol/L NaCl, and dissolved in 4 mol/L urea or in 25 mmol/L acetic acid. The concentration of Des-AA fm was calculated from absorbance at 280 nm (A, 1%; 1 cm = 15.0). Binding of fragment D1 to immobilized Des-AA fm. Des-AA fm (or fibrinogen) solution at 5 µg/mL in urea 4 mol/L was immobilized on glutaraldehyde-treated 96-well microplates, as described by Stanilawski et al.29 To the coated wells, 100 µL of a solution of fragment D1 at concentrations ranging from 1.5 to 25 µg/mL were added. After an incubation period of 2 hours at 37°C, the plates were washed 4 times. Then, in each well, 100 µL of a monoclonal antibody that specifically reacts with an antigenic neo-epitope on fragment D1 (anti-D neo-F2C5), previously described by Mirshahi et al,30 was added. After a 2-hour incubation period, the plates were washed, and bound anti-D neo-F2C5 was detected by adding 100 µL of 0.1% diluted peroxidase-labeled rabbit immunoglobulin anti-mouse to each well (Amersham France SA, Les Ulis, France). All the dilutions were performed in phosphate-buffered saline containing 0.05% Tween 20 and 0.1% serum bovine albumin. After an incubation period of 1 hour at 37°C, the plates were washed, and the amount of bound peroxidase was quantified by adding orthophenylene diamine and perhydrol (Sigma Chemical, St Quentin Fallavier, France) as described by Wolters et al.31 Binding of fibrinogen to immobilized Des-AA fm. Microplates were coated with 100 µL per well of normal Des-AA fm solution at 5 µg/mL in 25 mmol/L acetic acid for 18 hours at 4°C. The plates were washed. Then 100 µL normal fibrinogen or fibrinogen Alès, at concentrations ranging from 0.1 to 10 µg/mL in Tris-buffer saline-Tween (TBST) containing 1 mmol/L CaCl2, were introduced into each well and incubated for 2 hours at room temperature. Identical incubations were performed using 10 µg/mL fibrinogen solution containing Gly-Pro-Arg-Pro peptide at concentrations ranging from 25 nmol/L to 1500 nmol/L. The amount of fibrinogen bound to Des-AA fm was measured using a peroxidase-conjugate monoclonal antibody Y18-peroxidase (Gaubius Laboratory, Leiden, The Netherlands) that reacts with FpA. Immunoconjugate bound to the plates was determined with tetra methyl benzidine and perhydrol as the chromogen (Organon Teknika, Boxtel, The Netherlands). Isolation of genomic DNA, amplification, cloning, and sequencing Genomic DNA was isolated from blood cells according to the manufacturer's instructions using genomic DNA isolation kit (Gentra System, Minneapolis, MN). A 385-bp fragment encoding exon VIII (amino acids 259 to 350) and an 823-bp fragment encoding the exon IX (amino acids 351 to 427) of the-chain were amplified by polymerase chain
reaction (PCR) with the following primer pairs: VIIIR
5'-AACTTGGAATCTAAGAAAGGAAAACTACC-3', VIIIF
5'-GAAGCATCCTACGAAAGAGGG-3' and IXR
5'-AAAAAAGGAATTCTCTTTTGAAACGGTC-3', IXF
5'-GAAGCATCCTACGAAAGAGGG-3'.
Amplification was performed in a 50-µL reaction volume containing 0.3 µg genomic DNA, 5 U Taq polymerase (Gibco BRL), 0.2 mmol/L
each of dATP, dCTP, dGTP, and dTTP (Pharmacia, Orsay, France), and 0.2 mmol/L each of primer VIII Determination of endogenous thrombin potential Endogenous thrombin potential determination was performed according to Hemker et al33 on the basis of the time course of amidolytic activity using chromothrombin (Stago, Asnières, France) after the triggering of thrombin generation by calcium. Experiments were performed using both native citrated plasma and normal plasma that was depleted in its fibrinogen by removing the clot formed by the addition of reptilase.
Clinical and laboratory data Fibrinogen Alès was discovered in a 25-year-old man admitted to the hospital for multiple traumas. During this period there were no signs of any unusual bleeding or thrombotic tendency. However, at the age of 30, the propositus suffered 2 episodes of thrombotic stroke, as demonstrated by angiography. No history of hemorrhage or thrombotic tendency was observed in the propositus' parents or in his sister (35 years old). The known risk factors for thrombosis, suggested by ISTH,16 were absent in the propositus and his sister. Levels of protein C, protein S, and antithrombin III were within the normal range; levels of triglycerides, total cholesterol, and LDL/ HDL cholesterol were normal; lupus anticoagulant and anticardiolipid findings were negative. The level of homocysteine was also found to be within the normal range. Neither the factor V Leiden nor prothrombin gene 20210 G A polymorphisms were present in the propositus or his
sister. Apo E genotype was found to be epsilon 3/epsilon 4 for the
propositus and his sister.
Results of the coagulation screening tests of the propositus and his
family members are summarized in Table 1.
He and his sister had the same profile. Prothrombin time was markedly
prolonged, whereas the blood factors II, V, and VII + X were within
normal range. Thrombin time was markedly prolonged, resulting in a
small and weak clot. Reptilase time was infinite; no clot was observed with this enzyme. The presence of calcium chloride (from 25 to 100 mmol/L) did not induce any correction of the thrombin time. Polymerization curve, performed with the plasma of the propositus, did
not show any increase of turbidity when thrombin was added to plasma
diluted 1:10. However, using a lower dilution of the plasma (1:3), a
prolonged lag time and a low polymerization rate were demonstrated in
comparison with the polymerization curve of the normal plasma diluted
to 1:10 (Figure 1).
Plasma fibrinogen level determined by the functional assay of Clauss12 was markedly decreased, but when it was determined by heat precipitation and the immunological method, the results were normal. Platelet count and platelet aggregation levels were both normal. The fibrinogen-related antigen, which remained in serum obtained after 18-hour clotting of the plasma with thrombin, was normal. The father and the mother of the propositus, who are cousins, also had abnormal fibrin formation that was less severe than that observed in their children. These data indicate that the patient and his sister are homozygous and that his dysfibrinogenemia is congenital. Coagulation of purified fibrinogen The thrombin clotting time of purified fibrinogen Alès was markedly prolonged compared to normal fibrinogen (165 seconds; control, 15 seconds), and the reptilase time was infinite because fibrinogen Alès remained unclottable even when a high concentration of reptilase was used.The HPLC profiles of FpA and FpB, released by thrombin from fibrinogen Alès, were normal with respect to both the initial rate and the total amount released. Furthermore, the rate of FpA released after the addition of reptilase to fibrinogen Alès was normal (data not shown). Fibrin monomer aggregation of Des-AABB-fm (fibrin monomers depleted in
fibrinopeptides A and B), derived from the abnormal fibrinogen, did not
show any increase of the turbidity (Figure 2). The analysis of the cross-linking
profiles of fibrin mediated by factor XIIIa showed that
Analysis of fibrinogen molecule SDS-PAGE of purified fibrinogen Alès was carried out under reducing conditions according to the method of Laemmli.27 A-chain with higher mobility than that of the normal -chain was observed (Figure 3A), and there was no
-chain with a normal mobility. In contrast, SDS-PAGE, performed
according to the method of Weber and Osborn,21
showed no difference in electrophoretic migration between -chains of
normal fibrinogen and those of fibrinogen Alès (Figure
3B).
Plasmin digestion of purified fibrinogen When plasmin digestion was performed in the presence of calcium and the profile of the plasmin digest of fibrinogen Alès was analyzed by SDS-PAGE under reducing conditions, only the-chain and the  -chain remnants of fragment D1 remained, and the
Alès -chain remnant of fragment D1
(Alès/D1) had a higher mobility than that of
normal fragment D1 (/D1) (Figure
4, lanes 2, 4).
When plasmin digestion was performed in the presence of EDTA, the
profile of fibrinogen digest from Alès revealed Binding of fibrinogen and its derived fragment D1 to Des-AA fm In contrast to normal fragment D1, the fragment D1 isolated from fibrinogen Alès did not bind to immobilized normal Des-AA fm (Figure 5). In the same way, fibrinogen Alès did not bind to Des-AA fm (Figure 6). As a control, it was shown that 750 nmol/L of the peptide Gly-Pro-Arg-Pro, (corresponding to the site A), inhibited the binding of normal fibrinogen to Des-AA fm by more than 80%.
Determination of the -chain as shown by
SDS-PAGE and the localization of the abnormality to the carboxyl terminus part of the -chain by plasmic digest, 2 DNA fragments comprising exons VIII and IX encoding for amino acids 259 through 350 and 351 through 427 of the -chain were amplified by PCR. The DNA
sequence of the amplified exon IX from our patient was indistinguishable from the DNA normal sequence. DNA sequence analysis of exon VIII from Alès demonstrated a single base substitution in
the codon for Asp330 (GAT), changing this for the codon for
Val (GTT) (Figure 7). Sequence analysis
of 10 clones derived from DNA of the patient showed only the abnormal
sequence, indicating that this patient is homozygous.
Analysis of endogenous thrombin potential Endogenous thrombin potential (ETP), the area under the thrombin generation curve, was higher in normal fibrinogen-depleted plasma than in the corresponding untreated plasma. Thrombin measured at the peak from 5 normal healthy volunteers was 50% to 63% of that measured using the corresponding reptilase-treated plasmas, indicating that 50% to 37% of thrombin was bound to the clot.In contrast, ETP in Alès plasma (experiment performed in
triplicate) was found to be much higher than that observed using the
pool of 5 normal untreated plasmas. Both plasmas, however, have the
same immunologic level of fibrinogen. Furthermore, ETP was found to be
similar in Alès samples, regardless of whether they were treated
by reptilase (Figure 8). The coefficient
of variation in thrombin evaluation measured at the peak was 8% in Alès plasma, 13% to 15% in untreated normal plasma, and 10% in reptilase-treated plasma (due to experimental error in sampling time).
Homozygous dysfibrinogenemia was described in 2 members of the same family (the propositus and his sister), denoted as fibrinogen Alès. Each of the parents, who are cousins, had a heterozygous form of the anomaly. The abnormal fibrinogen of the propositus was unclottable by reptilase, and the thrombin-clotting time was dramatically delayed. Fibrinogen concentration was decreased when measured by functional assay, but it was normal when determined by heat precipitation or immunologic assay. Prolongation of the thrombin clotting time was not related to the defective release of FpA or FpB. In the same way, the absence of clotting by reptilase did not result from an abnormal release of FpA. Fibrin polymerization performed by adding thrombin to plasma was markedly impaired, and the aggregation of fm derived from thrombin-treated fibrinogen Alès did not show any increase in turbidity. In addition, with plasma diluted 1:10, there was no polymerization. SDS-PAGE of purified fibrinogen Alès indicated that the
structural defect was located in the The A-a interaction occurring between the reptilase-activated E domain of one molecule of fibrin monomer and the D domain of another plays an essential role in fibrin formation because the cleavage of FpA alone is sufficient to induce the fibrin assembly process.36 In fibrinogen Alès, this type of interaction does not occur because fragment D1 from Alès, which contains the site a, does not bind to immobilized normal Des-AA fm, which has the site A available. Under the same conditions, normal fragment D1 binds to Des-AA fm. Similarly, intact fibrinogen Alès does not bind to normal Des-AA fm, whereas normal fibrinogen does. As a control, it was shown that this binding process was inhibited by the addition of GPRP peptide (corresponding to the site A), which is known to compete for binding of normal fibrinogen or normal fragment D1 to Des-AA fm. Therefore, these results demonstrate that the mutation of the
residue Another mutation at the same position, Furthermore, in determining by crystallography the structure of the
complex GPRP-fragment D41 or that of the complex GPRP- rFbgC30 (recombinant 30-kd protein, corresponding to the carboxyl terminus region of the The absence of interaction between the polymerization sites A and a explains the unclottability of fibrinogen Alès by reptilase. More interesting, the observation that thrombin induces clotting of fibrinogen Alès suggests that polymerization can occur only through B-b interaction because the polymerization site B is unmasked in Des-AABB fm and masked in Des-AA fm. This should be compared to the Metz fibrinogen data, reported by Soria et al,43 a homozygous abnormal fibrinogen characterized by a whole blood clot formation occurring only through B-b interaction, because the addition of thrombin to fibrinogen Metz induces only the release of FpB. Therefore, because FpA is not released, this leads to an unavailability of site A. This situation represents "the other side of the coin" to fibrinogen Alès. Given that no hemorrhagic disease was observed in the propositus or in his sister, it is assumed that the clot resulting from the interaction B-b is sufficient to stop bleeding. With respect to the 2 episodes of arterial thrombosis it seems likely that, because clotting by thrombin is dramatically delayed in the patient, thrombin generated in the Alès sample is not trapped in fibrin, allowing platelet aggregation to occur. This hypothesis is consistent with endogenous thrombin potential, which has been proposed as a parameter for plasma-based hypercoagulability, being much higher in Alès plasma than in control. This difference was attributed to the fact that 37% to 50% of thrombin formed after calcium addition was trapped into the normal forming clot. The percentage of thrombin bound to the clot was deduced from the difference between thrombin activity in recalcified defibrinated plasma and that in recalcified plasma. Because clotting was dramatically delayed in Alès plasma, the thrombin generated remained in solution and its activity was similar to that found with fibrinogen-depleted normal plasma. Because reptilase added to plasma from Alès did not induce any clotting, it was shown, as a control, that endogenous thrombin potential was identical in Alès native and reptilase-treated plasmas. In all samples, a decay of thrombin activity that resulted from the neutralization of thrombin by antithrombin III was observed after 120 seconds, as already reported.44 However, it is important to know whether thrombin bound to Alès fibrin monomers is still accessible for platelet aggregation. In fact, it is well established that fibrin contains independent sites having affinity for thrombin. One of these sites, located in the E domain of the fibrin monomer, interacts with the anion binding site of thrombin. This binding exosite of thrombin is implicated in both fibrin and platelet binding. It has been shown that an equilibrium exists between thrombin bound to fibrin monomers and thrombin bound to platelets.45,46 Therefore thrombin bound to fibrin monomers is still active for platelet aggregation, but its activity is reduced in comparison to free thrombin. Thus, thrombin bound to fibrin monomers remains partly available for platelet aggregation. Furthermore, it has been reported that clot-associated thrombin induces platelet aggregation.47,48 In 2 other patients with congenital dysfibrinogenemia, an arterial
thrombotic risk is reported that can be related to a defective thrombin
binding to the clot, responsible for platelet
aggregation.49,50 However, the sister of the propositus,
though also homozygous for dysfibrinogenemia, is asymptomatic. We tried
to determine whether the thrombotic risk could be linked to other risk
factors associated with dysfibrinogenemia. The known risk factors for thrombosis, recommended by ISTH, were absent in the propositus and in
his sister. The propositus is a smoker, but his sister is not. Both the
patient and his sister also have apoE The parents of this propositus and the affected members of the family Milano I are asymptomatic, but they are heterozygous for the mutation with a circulating mixture of normal and abnormal fibrinogens. Therefore, as already reported for other dysfibrinogenemias, the potential risk factor would explain the variability observed in the clinical symptoms associated with this homozygous dysfibrinogenemia because the mutation is associated with severe thrombophilia in the patient and appears to be silent in his sister. In summary, a structural defect in a variant of fibrinogen, called
fibrinogen Alès, was identified. Our results demonstrate that the
substitution of the aspartic acid in position
The authors thank Dr J. C. Gris, Centre Hospitalier Universitaire de Nimes, for performing the risk factors recommended by ISTH, and Mr Richard Medeiras for his advice in editing the manuscript.
Submitted October 4, 1999; accepted July 24, 2000.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Jeannette Soria, Laboratoire de Biochimie A, Hotel-Dieu de Paris, 1 Place du Parvis de Notre Dame, 75181 Paris cedex 04, France.
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© 2000 by The American Society of Hematology.
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-Asp330 
Val) characterized by a defective fibrin
polymerization site "a"
Top
Abstract
Introduction
80°C.
), plasma from
the propositus diluted to 1:10 (
), and plasma from the propositus
diluted to 1:3 (
).
), Alès plasma (
3/