Hypofibrinogenemia due to Novel 316 Asp → Tyr Substitution in the Fibrinogen Bβ Chain

Stephen O. Brennan; Jane M. Wyatt; Stephen May; Susan De Caigney; Peter M. George

doi:10.1055/s-0037-1615603

Thrombosis and Haemostasis, Table of Contents

Thromb Haemost 2001; 85(03): 450-453
DOI: 10.1055/s-0037-1615603

Review Article

Schattauer GmbH

Hypofibrinogenemia due to Novel 316 Asp → Tyr Substitution in the Fibrinogen Bβ Chain

Stephen O. Brennan

¹Molecular Pathology Laboratory, Christchurch Hospital, Christchurch, New Zealand and Haematology Department Waikato Hospital, Hamilton, New Zealand

,

Jane M. Wyatt

¹Molecular Pathology Laboratory, Christchurch Hospital, Christchurch, New Zealand and Haematology Department Waikato Hospital, Hamilton, New Zealand

,

Stephen May

¹Molecular Pathology Laboratory, Christchurch Hospital, Christchurch, New Zealand and Haematology Department Waikato Hospital, Hamilton, New Zealand

,

Susan De Caigney

¹Molecular Pathology Laboratory, Christchurch Hospital, Christchurch, New Zealand and Haematology Department Waikato Hospital, Hamilton, New Zealand

,

Peter M. George

¹Molecular Pathology Laboratory, Christchurch Hospital, Christchurch, New Zealand and Haematology Department Waikato Hospital, Hamilton, New Zealand

› Author Affiliations

Abstract

Summary

We investigated the molecular basis of hypofibrinogenemia in a woman with a plasma fibrinogen of 1.0 mg/mL. After sequencing the coding region and intronic boundaries of all three fibrinogen genes a single heterozygous GACTAC mutation was identified at codon 316 of the B gene. This AspTyr substitution segregated with the hypofibrinogenemia in the only other affected family member. Examination by SDS-PAGE, isoelectric focussing, reverse phase chromatography and electrospray ionisation (ESI) mass spectrometery, failed to detect expression of the new B chain in purified plasma fibrinogen. The absence of the variant chain was confirmed by ESI tryptic mapping; while the [M + 1 H] and [M + 2 H] ions of the affected peptide (MGPTELLIEMEDWK) were clearly visible at 1,692 and 847 m/z, there were no new signals (1741 or 871 m/z) that would at indicate expression of the variant in plasma. Asp 316 and itschain homologue (Asp 252) are conserved in all known species and this is the first report of a mutation at either of these. The residue appears to be critical in maintaining the structure of the five stranded sheet that forms the dominant structural feature of the D domains.

Keywords

Fibrinogen - hypofibrinogenemia - mutation - mass spectrometery

Full Text

References

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