Venous Thrombosis and Thrombocyte Activity in Zebrafish Models of Quantitative and Qualitative Fibrinogen Disorders

Venous Thrombosis and Thrombocyte Activity in Zebrafish Models of Quantitative and Qualitative Fibrinogen Disorders

Venous thrombosis occurs in patients with quantitative and qualitative fibrinogen disorders. Injury-induced thrombosis in zebrafish larvae has been used to model human coagulopathies. We aimed to determine whether zebrafish models of afibrinogenemia and dysfibrinogenemia have different thrombotic ph...

Full description

Bibliographic Details
Main Authors: Richard J. Fish, Cristina Freire, Corinne Di Sanza, Marguerite Neerman-Arbez
Format: Article
Language:English
Published: MDPI AG 2021-01-01
Series:International Journal of Molecular Sciences
Subjects:
fibrinogen
fibrin
thrombocytes
thrombosis
zebrafish
Online Access:https://www.mdpi.com/1422-0067/22/2/655
Description
Summary:Venous thrombosis occurs in patients with quantitative and qualitative fibrinogen disorders. Injury-induced thrombosis in zebrafish larvae has been used to model human coagulopathies. We aimed to determine whether zebrafish models of afibrinogenemia and dysfibrinogenemia have different thrombotic phenotypes. Laser injuries were used to induce venous thrombosis and the time-to-occlusion (TTO) and the binding and aggregation of fluorescent <i>Tg(itga2b:EGFP)</i> thrombocytes measured. The <i>fga<sup>−/−</sup></i> larvae failed to support occlusive venous thrombosis and showed reduced thrombocyte binding and aggregation at injury sites. The <i>fga<sup>+/−</sup></i> larvae were largely unaffected. When genome editing zebrafish to produce fibrinogen Aα R28C, equivalent to the human Aα R35C dysfibrinogenemia mutation, we detected in-frame skipping of exon 2 in the fga mRNA, thereby encoding Aα<sup>Δ<i>19–56</i></sup>. This mutation is similar to Fibrinogen Montpellier II which causes hypodysfibrinogenemia. Aα<sup><i>+/</i>Δ<i>19–56</i></sup> fish had prolonged TTO and reduced thrombocyte activity, a dominant effect of the mutation. Finally, we used transgenic expression of fga R28C cDNA in fga knock-down or <i>fga<sup>−/−</sup></i> mutants to model thrombosis in dysfibrinogenemia. Aα R28C expression had similar effects on TTO and thrombocyte activity as Aα<sup><i>+/</i>Δ<i>19–56</i></sup>. We conclude that thrombosis assays in larval zebrafish can distinguish between quantitative and qualitative fibrinogen disorder models and may assist in anticipating a thrombotic phenotype of novel fibrinogen mutations.
ISSN:1661-6596
1422-0067

Similar Items