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Blood, Vol. 96 No. 1 (July 1), 2000:
pp. 149-152
HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Division of Medical Genetics, University Medical
School and University Hospital, and the Division of Angiology and
Hemostasis, University Hospital, Geneva, Switzerland; the
Center for Molecular and Vascular Biology, Leuven, Belgium; the
Hemophilia Center, Hôpital Purpan, Toulouse, France; the
Department of Pediatrics, Weill Medical College of Cornell Hospital,
New York, New York; the Hemophilia Center and the
Hematology Laboratory, Hôpital Bicêtre, AP-HP
LeKremlin-Bicêtre; the Centre de Transfusion, Annecy; and the
Hematology Laboratory, CHR Amiens, France.
Congenital afibrinogenemia is a rare, autosomal, recessive disorder
characterized by the complete absence of detectable fibrinogen. We
previously identified the first causative mutations in a
nonconsanguineous Swiss family; the 4 affected persons have homozygous
deletions of approximately 11 kb of the fibrinogen alpha (FGA)
gene. Haplotype data implied that these deletions occurred on distinct
ancestral chromosomes, suggesting that this region may be susceptible
to deletion by a common mechanism. We subsequently showed that all the
deletions were identical to the base pair and probably resulted from a
nonhomologous recombination mediated by 7-bp direct repeats. In this
study, we have collected data on 13 additional unrelated patients to
identify the causative mutations and to determine the prevalence of the
11-kb deletion. A common recurrent mutation, at the donor splice site
of FGA intron 4 (IVS4 + 1 G > T), accounted for 14 of the
26 (54%) alleles. One patient was heterozygous for the previously
identified deletion. Three more frameshift mutations, 2 nonsense
mutations, and a second splice site mutation were also identified.
Consequently, 86% of afibrinogenemia alleles analyzed to date have
truncating mutations of FGA, though mutations in all 3 fibrinogen genes, FGG, FGA, and FGB, might be predicted to cause congenital afibrinogenemia.
(Blood. 2000;96:149-152)
Congenital afibrinogenemia (Mendelian Inheritance in
Man #202,400) was originally described in
1920.1 To date some 150 families with this disorder have
been reported,2 with approximately 50% of instances
occurring in consanguineous pedigrees.3 Although functional
assays of clot formation are infinitely prolonged in affected persons,
the coagulation defect is surprisingly no more severe than in severe
hemophilias A and B, varying from severe to moderate.4
Umbilical cord hemorrhage is often the first sign of the disorder; gum
bleeding, epistaxis, menorrhagia, gastrointestinal bleeding, and
hemarthrosis occur with different degrees of intensity, and spontaneous
intracerebral bleeding and splenic rupture can occur throughout life.
Patients generally respond well to fibrinogen replacement therapy. The
genetic defect was assumed to be at the level of fibrinogen synthesis
because the half-life of infused fibrinogen is essentially
normal.2 The fibrinogen locus is comprised of 3 genes
coding for fibrinogen gamma (FGG), fibrinogen alpha
(FGA), and fibrinogen beta (FGB), clustered in a region of approximately 50 kb on chromosome 4q28-q31.5 We
previously studied this region in a Swiss family with 2 pairs of
affected brothers by using microsatellite analysis, polymerase chain
reaction (PCR) amplification, and Southern blotting, identifying the
first causative mutations for the disorder.6 We found that
the genetic defect in this family was an apparently recurrent deletion
of approximately 11 kb of DNA that eliminates most of the FGA
gene, leading to an absence of functional fibrinogen. We subsequently identified the molecular mechanism involved in the generation of the
deletions responsible for congenital afibrinogenemia by cloning and
sequencing the deletion junctions for all mutated chromosomes.
The deletions were all identical to the base pair and probably resulted
from nonhomologous (illegitimate) recombination, mediated by a direct
7-bp repeat, AACTTTT, and perhaps also by indirect repeats in the
breakpoint region.7
In this study, we performed mutation analysis in the FGA gene
in 13 additional unrelated patients with congenital afibrinogenemia from Puerto Rico, France, Pakistan, Belgium, and the United States. One
patient, from the United States, was a heterozygous carrier of the
originally described 11 kb deletion, as revealed by Southern blot
analysis. In addition, we identified the most common mutation, in the
invariant GT dinucleotide of the donor splice site of FGA intron 4 (IVS4 + 1 G > T), which accounted for 14 of the 26 (54%) afibrinogenemia alleles analyzed in this study. Five new mutations leading to premature protein truncation were also identified: 34insC
(exon 1), 3121del AA (exon 4), and 4329del C, G316X, and W334X (all
exon 5). Finally, a potential IVS1 + 3 donor splice site mutation was
identified. All the mutations in patients of Caucasian
origin were identified; in contrast, no mutations were found in FGA
in the 2 non-Caucasian patients studied.
Patients
Mutation screening
Southern blotting
Haplotype analysis
Screening of normal alleles Ninety-five DNA samples from anonymous European control subjects were screened for the IVS1 + 3 A > G mutation by PCR amplification of FGA exon 1 followed by nonradioactive, single-stranded conformation analysis using GeneGel Excel gels (Pharmacia Biotech, St Albans, UK) as previously described.12
Data from 13 unrelated patients with afibrinogenemia were collected for this study. For all these patients, plasma fibrinogen was undetectable by functional and immunologic assays, and the prothrombin, activated partial thromboplastin, and thrombin time tests were unclottable in all patients. Factor V, factor VII, and factor X were measured in all patients and were within normal ranges. In the 7 patients tested, factors VIII, IX, and XI were within normal ranges. Furthermore, for some patients, inhibitors (antithrombin, protein C, and protein S), factor V Leiden, and prothrombin G20210A mutations were assayed, and all results were normal.
Deletion of 11 kb
Splice site mutations
Deletions and insertions One patient (A8) was found to be a compound heterozygote for 2 frameshift mutations in FGA. The first mutation, 34insC (numbered according to Genbank M64982), was a 1-bp insertion in the second codon of exon 1 that led to an in-frame TAG stop codon in exon 2. The second mutation, 3121delAA, was a 2-bp deletion in exon 4 that led to an in-frame TAG stop codon 15 codons downstream, in the same exon. Another patient (A12) was also a compound heterozygote for 3121delAA. A third frameshift mutation in exon 5, 4329delC, was identified in patient B3. This deletion generated an in-frame TAA stop codon 69 codons downstream.Nonsense mutations Two nonsense mutations were identified in exon 5, both in compound heterozygosity: G316X (patient A7, GGA > TGA) and W334X (patient A12, TGG > TGA).
In this study, we analyzed the FGA gene in 13 unrelated patients with congenital afibrinogenemia from Puerto Rico, France, Pakistan, Belgium, and the United States to identify the causative mutations in affected persons and to determine the prevalence of the 11-kb FGA deletion. Including the 3 alleles in the 4 affected family members described in our original report,6 we have now studied a total of 29 alleles in 17 patients and have identified 8 different FGA mutations that account for 86% (25 of 29) of the afibrinogenemia alleles.
We thank all the families for their cooperation and for donating blood samples. We thank Hewlett-Packard (Switzerland) for their kind support through their donation of computer equipment.
Submitted January 13, 2000; accepted February 21, 2000.
Supported by a Marie Heim-Voegtlin grant (M.N.-A.), Swiss National Science Foundation grant 31-55848.98, and the Roche Research Foundation.
Reprints: Marguerite Neerman-Arbez, Centre Médical Universitaire, 1 rue Michel Servet, CH-1211 Geneva, Switzerland; e-mail: marguerite.arbez{at}medecine.unige.ch.
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.
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  R. Park, H.-J. Doh, S.-S. A. An, J.-R. Choi, K.-H. Chung, and K.-S. Song A novel fibrinogen variant (fibrinogen Seoul II; A{alpha}Gln328Pro) characterized by impaired fibrin {alpha}-chain cross-linking Blood, September 15, 2006; 108(6): 1919 - 1924. [Abstract] [Full Text] [PDF]
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 D. Vu, C. Di Sanza, D. Caille, P. de Moerloose, H. Scheib, P. Meda, and M. Neerman-Arbez Quality control of fibrinogen secretion in the molecular pathogenesis of congenital afibrinogenemia Hum. Mol. Genet., November 1, 2005; 14(21): 3271 - 3280. [Abstract] [Full Text] [PDF]
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 D Vu, P de Moerloose, A Batorova, J Lazur, L Palumbo, and M Neerman-Arbez Hypofibrinogenaemia caused by a novel FGG missense mutation (W253C) in the {gamma} chain globular domain impairing fibrinogen secretion J. Med. Genet., September 1, 2005; 42(9): e57 - e57. [Abstract] [Full Text] [PDF]
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M. Neerman-Arbez, M. Germanos-Haddad, K. Tzanidakis, D. Vu, S. Deutsch, A. David, M. A. Morris, and P. de Moerloose Expression and analysis of a split premature termination codon in FGG responsible for congenital afibrinogenemia: escape from RNA surveillance mechanisms in transfected cells Blood, December 1, 2004; 104(12): 3618 - 3623. [Abstract] [Full Text] [PDF]
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P. Lefebvre, P. T. Velasco, A. Dear, K. C. Lounes, S. T. Lord, S. O. Brennan, D. Green, and L. Lorand Severe hypodysfibrinogenemia in compound heterozygotes of the fibrinogen A{alpha}IVS4 + 1G>T mutation and an A{alpha}Gln328 truncation (fibrinogen Keokuk) Blood, April 1, 2004; 103(7): 2571 - 2576. [Abstract] [Full Text] [PDF]
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D. Vu, P. H. B. Bolton-Maggs, J. R. Parr, M. A. Morris, P. de Moerloose, and M. Neerman-Arbez Congenital afibrinogenemia: identification and expression of a missense mutation in FGB impairing fibrinogen secretion Blood, December 15, 2003; 102(13): 4413 - 4415. [Abstract] [Full Text] [PDF]
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M. Neerman-Arbez, D. Vu, B. Abu-Libdeh, I. Bouchardy, and M. A. Morris Prenatal diagnosis for congenital afibrinogenemia caused by a novel nonsense mutation in the FGB gene in a Palestinian family Blood, May 1, 2003; 101(9): 3492 - 3494. [Abstract] [Full Text] [PDF]
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C. Attanasio, A. David, and M. Neerman-Arbez Outcome of donor splice site mutations accounting for congenital afibrinogenemia reflects order of intron removal in the fibrinogen alpha gene (FGA) Blood, March 1, 2003; 101(5): 1851 - 1856. [Abstract] [Full Text] [PDF]
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S. Spena, S. Duga, R. Asselta, M. Malcovati, F. Peyvandi, and M. L. Tenchini Congenital afibrinogenemia: first identification of splicing mutations in the fibrinogen Bbeta -chain gene causing activation of cryptic splice sites Blood, December 15, 2002; 100(13): 4478 - 4484. [Abstract] [Full Text] [PDF]
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N. Okumura, F. Terasawa, H. Tanaka, M. Hirota, H. Ota, K. Kitano, K. Kiyosawa, and S. T. Lord Analysis of fibrinogen gamma -chain truncations shows the C-terminus, particularly gamma Ile387, is essential for assembly and secretion of this multichain protein Blood, May 15, 2002; 99(10): 3654 - 3660. [Abstract] [Full Text] [PDF]
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R. Asselta, S. Duga, S. Spena, E. Santagostino, F. Peyvandi, G. Piseddu, R. Targhetta, M. Malcovati, P. M. Mannucci, and M. L. Tenchini Congenital afibrinogenemia: mutations leading to premature termination codons in fibrinogen Aalpha -chain gene are not associated with the decay of the mutant mRNAs Blood, December 15, 2001; 98(13): 3685 - 3692. [Abstract] [Full Text] [PDF]
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C. Attanasio, P. de Moerloose, S. E. Antonarakis, M. A. Morris, and M. Neerman-Arbez Activation of multiple cryptic donor splice sites by the common congenital afibrinogenemia mutation, FGA IVS4 + 1 G{right-arrow}T Blood, March 15, 2001; 97(6): 1879 - 1881. [Abstract] [Full Text] [PDF]
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R. Asselta, S. Duga, T. Simonic, M. Malcovati, E. Santagostino, P. L. F. Giangrande, P. M. Mannucci, and M. L. Tenchini Afibrinogenemia: first identification of a splicing mutation in the fibrinogen gamma chain gene leading to a major gamma chain truncation Blood, October 1, 2000; 96(7): 2496 - 2500. [Abstract] [Full Text] [PDF]
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| Copyright © 2000 by American Society of Hematology Online ISSN: 1528-0020 | |||||||||
gene account for the majority of
cases of congenital afibrinogenemia
Top
Abstract
Introduction
isoform were amplified from genomic DNA by PCR, under standard conditions. The
alternatively spliced exon 6 was excluded from this study because it
persists only in the mRNA encoding the longer 
G splice-donor-site mutation at position +3 of the collagenlike-tail subunit gene (COLQ): how does G at position +3 result in aberrant splicing?
Am J Hum Genet.
1999;65:635-644
fibrinogen gene cause congenital afibrinogenemia by impairing fibrinogen secretion.
Blood.
2000;95:1336-1341