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HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Central Hematology Laboratory, Inselspital,
University Hospital, Bern, Switzerland; and the Department of Pathology
and Laboratory Medicine, University of North Carolina at Chapel Hill.
Fibrinogen Milano XII was detected in an asymptomatic Italian
woman, whose routine coagulation test results revealed a prolonged thrombin time. Fibrinogen levels in functional assays were considerably lower than levels in immunologic assays. Polymerization of purified fibrinogen was strongly impaired in the presence of calcium or ethylenediaminetetraacetic acid (EDTA). Two heterozygous
structural defects were detected by DNA analysis: A Fibrinogen, a soluble plasma glycoprotein of 340 kd, is made up of 2 copies of 3 different polypeptide chains
(A Dysfibrinogenemia is a heritable disorder characterized by structural
mutations in any of the 3 polypeptide chains of fibrinogen. A
repertoire of 191 individual cases in which the structural defects have
been elucidated are listed at
http://www.geht.org/pages/database_ang.html (accessed January
2001). Regarding hemostasis, most of the affected patients are
asymptomatic, but some suffer from bleeding, thrombosis, or
both.3 To date, only one compound heterozygote with
2 mutations in fibrinogen has been described.4 The patient
had hypofibrinogenemia but had no polymerization defect.
We report a dysfunctional fibrinogen variant with 2 single heterozygous
amino acid substitutions, one at position A Routine coagulation tests
Purification of fibrinogen
Coagulation profiles of purified fibrinogen Fibrin polymerization was evaluated turbidimetrically.8 Fibrinogen (540 µL, 0.55 mg/mL) was preincubated with 30 µL 20 mM Ca++ or 20 mM ethylenediaminetetraacetic acid (EDTA) (final concentration 1 mM) in polystyrene cuvettes for 5 minutes at 37°C. After the addition of 30 µL 10 U/mL bovine thrombin (final concentration, 0.5 U/mL; Diagnotec AG, Liestal, Switzerland), the increase in turbidity at 350 nm was measured in a spectrophotometer at 37°C. Each experiment was performed twice.DNA analysis Genomic DNA was isolated as previously described.9 The entire coding region of all 3 fibrinogen genes was amplified by polymerase chain reaction (PCR), and the PCR products were purified using the QIAquick PCR purification kit (Qiagen, Valencia, CA). Coding and complementary strands of the purified products were sequenced (Automated DNA Sequencing Facility, University of North Carolina at Chapel Hill) using the same primers as for PCR.Kinetics of fibrinopeptide release Fibrinogen solutions were diluted with TEA-buffer to a final concentration of 0.2 mg/mL. Human -thrombin (Enzyme Research Laboratory, South Bend, IN) was added to a final concentration of 0.005 U/mL, and the individual reactions were stopped at designated time
points by boiling the incubation mixtures for 15 minutes. To measure
the total amount of fibrinopeptide A and B released at an infinity time
point, the fibrinogen was incubated with 10 U/mL thrombin for 240 minutes. After centrifugation, the supernatants were immediately
analyzed by reverse-phase high-performance liquid chromatography (HPLC)
using the Shimadzu HPLC-System (Shimadzu, Columbia, MD) with a
Discovery C18 250-mm, 5-µm column (Supelco, Bellefonte, PA). The
column was equilibrated with buffer A (25 mM
NaH2PO4/Na2HPO4, pH
6.0), and the autosampler loaded 200 µL each sample on the column.
Peptides were eluted with a linear gradient from 15% to 36% buffer B
(25 mM NaH2PO4/Na2HPO4,
pH 6.0, with 50% acetonitrile) and monitored by absorbance reading at 210 nm. Fibrinopeptide peak areas from 2 experiments were determined by
the accompanying software class 5.0 VP (Shimadzu). Fibrinopeptide release curves were constructed by plotting the percentage release, assuming the total FpA release from normal fibrinogen was
100%.
Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and immunoblot analysis of purified fibrinogen Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) of nonreduced normal and variant fibrinogen was performed on a 3% to 10% gradient slab polyacrylamide gel with a 3% stacking gel.10 Separated proteins were transferred onto nitrocellulose sheets and incubated overnight at room temperature with either a 1/2000 dilution of peroxidase-conjugated rabbit antibody to human fibrinogen (P0445; Dako A/S, Glostrup, Denmark) or a peroxidase-conjugated rabbit antibody to human serum albumin (P0356; Dako A/S). Bound antibodies were visualized by diaminobenzidine in the presence of H2O2.To analyze the fibrinogens under reduced conditions, 10 µL reducing solution (10 mg dithiothreitol in 100 µL 0.05 M Tris pH 8.5, 8 M urea) was added to 50 µL fibrinogen (0.8 mg/mL). The mixture was incubated for 20 minutes at 60°C. SDS-PAGE was performed on an 8% slab gel with a 4.5% stacking gel10 and stained with Coomassie blue. SDS-PAGE and immunoblot analysis of fibrinogen degradation products Purified normal and variant fibrinogen were proteolytically degraded by the addition of plasminogen (purified from human plasma as described by Deutsch and Mertz11) and streptokinase (American Diagnostica, Greenwich, CT). Digestion was performed at 37°C in the presence of Ca++ or EDTA for 4 hours. The reaction was stopped by heating the samples for 5 minutes in the presence of SDS-containing sample buffer at 95°C. SDS-PAGE of fibrinogen degradation products was performed on 8% and 12% polyacrylamide gels10 under nonreducing and reducing conditions, respectively. Gels were loaded with 20 µg initial fibrinogen preparation and stained with Coomassie blue. The experiment was repeated in the presence of the peptide GPRP (0, 2, and 5 mM) with 1 mM EDTA added to all reactions.12 Immunoblot analysis was performed with nonreduced fibrinogen degradation products. Electrophoresed proteins were transferred onto nitrocellulose sheets and incubated at room temperature with the following antibodies: polyclonal rabbit anti-human fibrinogen (A0080; Dako); polyclonal rabbit anti-human fibrinogen -chain prepared by Hazelton Research Products (Denver, PA) using -chain purified from inclusion bodies expressed in Escherichia coli as the antigen13;
monoclonal anti-human serum albumin (clone HAS-11, A6684; Sigma, St
Louis, MO); monoclonal antibody E2F8E5 to fragment E, recognizing the
sequence GHRPLDK ( 15-21) (Immunotech, Marseilles, France);
peroxidase-conjugated anti-mouse or anti-rabbit IgG (Calbiochem, La
Jolla, CA). Bound antibodies were visualized by enhanced
chemiluminescence Western blotting detection reagents (Amersham
Pharmacia Biotech, Piscataway, NJ). Human serum albumin (A9511; Sigma)
was used as a control.
Purification of the fibrinogen degradation fragment D3 The fragment D3 was isolated as described earlier,14 with a slight modification. Briefly, 2 mL normal or variant fibrinogen (3 mg/mL) were proteolytically degraded for 4 hours at 37°C by the addition of 1 U/mL plasminogen (Kabi, Stockholm, Sweden) and 200 U/mL streptokinase (Behring, Marburg, Germany) in the presence 10 mM EDTA. The incubation mixture was dialyzed against the starting buffer (0.01 M TEA, 1 mM CaCl2, pH 7.4) and loaded on a Lysine-Sepharose 4B (Amersham Pharmacia Biotech) column (15 mL) equilibrated with starting buffer. The column was successively rinsed with 20 mL starting buffer, 20 mL elution buffer 1 (0.03 M TEA, 1 mM CaCl2, pH 7.4), and 20 mL elution buffer 2 (0.05 M TEA, 0.1 M NaCl, 1 mM CaCl2, pH 7.4). Fractions of 1 mL were collected and analyzed by SDS-PAGE on 8% polyacrylamide gels. Fragment D3-containing fractions were pooled and dialyzed either against TEA-buffer and frozen or against water and lyophilized.Digestion of purified fragment D3 with chymotrypsin Digestion was performed according to Medved et al.15 Lyophilized fragment D3 (500 µg) was dissolved in 100 µL 0.1 M phosphate buffer pH 7.0.-Chymotrypsin (56 U/mg; type
VII, TLCK-treated, bovine pancreas; Sigma) was added in an
enzyme-substrate ratio of 1:50. The reaction was stopped at 0, 8, and
23 hours by boiling the samples. Fragments were separated by SDS-PAGE
on 10% polyacrylamide gel10 and stained with
Coomassie blue.
Circular dichroism analysis of purified fragment D3 Purified fragment D3 was dialyzed against 10 mM phosphate buffer pH 7.4. The concentration of the dialyzed samples was determined at 280 nm in the presence of 1 M urea (E
Case report and routine coagulation tests The propositus of dysfibrinogen Milano XII was born in 1929 in Italy and had no reported history of bleeding or thrombosis. Unfortunately, no other family members were available for testing. Routine coagulation tests with plasma samples from the propositus revealed a significantly prolonged thrombin time; furthermore, her plasma was not clottable with reptilase (Table 1). Immunologically determined fibrinogen levels (Laurell) were within normal range, but fibrinogen concentrations measured by a functional method (Clauss) were dramatically lower.
Coagulation profiles of purified fibrinogen Turbidity curves (Figure 1) represent the kinetics of fibrin formation after the addition of thrombin to purified normal or variant fibrinogen in the presence of 1 mM calcium ions or 1 mM EDTA. In the presence of calcium, the variant showed a prolonged lag time and strongly reduced final turbidity compared to normal fibrinogen. In the presence of EDTA, only a minute turbidity increase occurred over the recording period.
DNA analysis Sequence analysis of the entire coding region of the 3 fibrinogen genes revealed 2 point mutations (data not shown). The first mutation was found in exon 6 of the-chain, a substitution of base 4682 guanine to adenine, changing the amino acid glycine to arginine at
position 165 of the -chain. The second mutation was detected in exon
2 of the A-chain. A single base change at position 1202 from
cytosine to thymine led to the replacement A R16C.
Kinetics of fibrinopeptide release We examined the rate of thrombin-catalyzed fibrinopeptide release by measuring the peak areas of FpA and FpB as detected by reverse-phase HPLC. After a 240-minute incubation, only approximately 50% of the FpA was released from fibrinogen Milano XII (Figure 2). Increasing the amount of thrombin, the time of incubation, or both did not change this percentage. The release of FpB from fibrinogen Milano XII was delayed but approached 100% with a higher thrombin concentration (data not shown).
SDS-PAGE and immunoblot analysis of fibrinogen Nonreduced normal and variant fibrinogens were subjected to SDS-PAGE and immunoblot analysis. HMW fibrinogen (Mr 340 000), LMW fibrinogen (Mr 305 000), and LMW' fibrinogen (Mr 270 000) were observed in both fibrinogens (Figure 3A). With the variant fibrinogen, these 3 bands were much broader and consistently migrated more slowly than the comparable bands of normal fibrinogen. Two additional bands with higher molecular weights were detected in the variant sample. Because these 2 bands reacted with an antibody against human albumin, they likely represent HMW and LMW fibrinogen complexed with albumin (Figure 3B), similar to earlier reports for the fibrinogen variants IJmuiden (B R14C) and Nijmegen (B R44C).20
SDS-PAGE of reduced samples revealed that the A-, B-, and
-chains from normal and variant fibrinogen were identical and
stained with the same intensity. No abnormally migrating chains were
visible (data not shown).
SDS-PAGE and immunoblot analysis of fibrinogen degradation products It is known that the extent of plasmin degradation of fibrinogen is sensitive to calcium bound to the high-affinity site and to the peptide GPRP bound to the a polymerization site. Both sites are located in the D domain, and normal binding of Ca++ or the peptide GPRP protects the fibrinogenolysis fragment D1 against further degradation to D2 and D3. Plasmin digests of normal and Milano XII fibrinogens produced fragment D1 in the presence of calcium and fragment D3 in the presence of EDTA (Figure 4A), indicating complete protection of the substrates by bound calcium. Under both conditions, the digests of fibrinogen Milano XII showed an additional band of apparently higher molecular weight, denoted D1* and D3* in Figure 4A. We compared the plasmin digestion of fibrinogen Milano XII to the digestion of fibrinogen St Gallen I ( G292V),21 a variant that is
abnormally digested to give the fragments D2 and D3 because of only
partial protection of D1 by Ca++. As shown in Figure 4A,
fragment D3* was not the same as fragment D2 and thus did not arise
from the incomplete conversion of D1 in D3. When the plasmin digests
were examined under reducing conditions, normal and variant chain
remnants were indistinguishable (Figure 4B). This indicates that the
unusual D1* and D3* fragments arose from disulfide-linked molecules. We
also digested the normal and variant fibrinogens in the presence of 2 mM and 5 mM GPRP and saw complete protection in both samples (data not
shown). These degradation patterns indicate that both the high-affinity
calcium-binding site and the a polymerization site are normal in
fibrinogen Milano XII.
To identify the fragment of fibrinogen Milano XII that bound albumin,
we performed immunoblot analysis of nonreduced plasmin digests
comparing the patterns obtained with 4 antibodies: polyclonal antibodies against fibrinogen and
Purification of the fibrinogen degradation fragment D3 Using a Lysine Sepharose 4B column and a strategy of different buffers with increasing salt concentration, fragment D3 was eluted in an early peak and was separated from fragment E and plasmin. The D3 and D3* fraction from fibrinogen Milano XII eluted concomitantly and could not be separated from each other (data not shown).Digestion of purified fragment D3 with chymotrypsin Fragment D3 (Mr 82 kd) can be further digested by chymotrypsin to a fragment called TSD (thermodynamic stable domain).22 In bovine fibrinogen, a chymotrypsin cleavage site had been identified between 151 and 152 leading to a
digestion fragment of 63 kd. Because of the similarity of bovine and
human fibrinogen,23 it is likely that the cleavage site
for chymotrypsin in human fibrinogen may be situated close to that
found in bovine fibrinogen. Incubation of normal and variant fragment
D3 with chymotrypsin led to a 63-kd fragment, and the double band
associated with fibrinogen Milano XII disappeared (data not shown).
Therefore, removal of the mutation site at position 165 led to a
chymotryptic fragment of the same size as the fragment derived from
normal fibrinogen.
Far UV-CD analysis of purified fragment D3 Figure 6 shows far UV-CD spectra of purified fragments D3 of normal and variant fibrinogen. A slight reduction of the mean residual ellipticity was calculated with fragment D3 derived from fibrinogen Milano XII. The curve representing the normal fragment D3 showed a minimum at 210 nm reflecting the-helical structure in the protein.24,25 This feature
was less prominent in the CD-spectra of variant fragment D3. The
-helical content in the variant fragment D3 (28.2% ± 0.9%) was
significantly different from normal D3 (31.8% ± 0.7%;
P = .005).
We describe a dysfunctional fibrinogen variant with 2 mutations,
one in the A The mutation in the The amino acid substitution A Fibrinogen Milano XII is the first dysfunctional fibrinogen variant
with 2 amino acid substitutions associated with a strong polymerization
defect. Brennan et al4 reported earlier a fibrinogen variant with 2 mutations in the coding region of fibrinogen. Both structural defects were detectable in the circulating fibrinogen but
did not affect fibrin polymerization. Neither the substitution
We thank Drs F. Baudo and R. Redaelli (Ospedale Niguarda, Milan, Italy) for providing the patient's plasma; Dr A. Tripathy (University of North Carolina, Chapel Hill) for help with CD analysis; and Dr Kelly A. Hogan for critical review of the manuscript.
Submitted November 14, 2000; accepted March 19, 2001.
Supported by grants from the Swiss National Science Foundation (32-47033.96) and the National Institutes of Health (R01 HL 31048).
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: Bettina Bolliger-Stucki, Department of Pathology and Laboratory Medicine, University of North Carolina at Chapel Hill, CB #7525, 605 Brinkhous-Bullitt Bldg, Chapel Hill, NC 27599-7525; e-mail: bettina_bolliger{at}med.unc.edu.
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© 2001 by The American Society of Hematology.
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R16C and 
G165R
Top
Abstract
Introduction
, 
, normal fibrinogen; 
, 
, fibrinogen Milano XII; 
G and B