A quantitative and humane tail bleeding assay for efficacy evaluation of antihaemophilic factors in haemophilia A mice

Molina, Enedelia; Fujita, André; Sogayar, Mari Cleide; Demasi, Marcos Angelo Almeida

doi:10.1111/hae.12484

Cited by 9 publications

(4 citation statements)

References 31 publications

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“…Bleeding time was determined using a stop clock. Measurement of rebleeding events was performed using a method adapted from Molina et al (36); the mice were returned to individual cages 5 min after cessation of bleeding, and a filter paper was applied to the end of the mouse tail every 15 min over a 1-h period. Appearance of fresh blood on the filter paper was counted as a rebleeding event.…”

Section: Discussionmentioning

confidence: 99%

Elimination of fibrin γ-chain cross-linking by FXIIIa increases pulmonary embolism arising from murine inferior vena cava thrombi

Duval

Baranauskas

Feller

et al. 2021

Proc. Natl. Acad. Sci. U.S.A.

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The onset of venous thromboembolism, including pulmonary embolism, represents a significant health burden affecting more than 1 million people annually worldwide. Current treatment options are based on anticoagulation, which is suboptimal for preventing further embolic events. In order to develop better treatments for thromboembolism, we sought to understand the structural and mechanical properties of blood clots and how this influences embolism in vivo. We developed a murine model in which fibrin γ-chain cross-linking by activated Factor XIII is eliminated (FGG3X) and applied methods to study thromboembolism at whole-body and organ levels. We show that FGG3X mice have a normal phenotype, with overall coagulation parameters and platelet aggregation and function largely unaffected, except for total inhibition of fibrin γ-chain cross-linking. Elimination of fibrin γ-chain cross-linking resulted in thrombi with reduced strength that were prone to fragmentation. Analysis of embolism in vivo using Xtreme optical imaging and light sheet microscopy demonstrated that the elimination of fibrin γ-chain cross-linking resulted in increased embolization without affecting clot size or lysis. Our findings point to a central previously unrecognized role for fibrin γ-chain cross-linking in clot stability. They also indirectly indicate mechanistic targets for the prevention of thrombosis through selective modulation of fibrin α-chain but not γ-chain cross-linking by activated Factor XIII to reduce thrombus size and burden, while maintaining clot stability and preventing embolism.

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Section: Discussionmentioning

confidence: 99%

Elimination of fibrin γ-chain cross-linking by FXIIIa increases pulmonary embolism arising from murine inferior vena cava thrombi

Duval

Baranauskas

Feller

et al. 2021

Proc. Natl. Acad. Sci. U.S.A.

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“…To evaluate hemorrhage responses in F8KO mice, before and after AAV injection, a filter paper-based tail vein bleeding time assay was performed as described previously 29 , with modifications. As shown in Suppl.…”

Section: Methodsmentioning

confidence: 99%

Hemophilia A ameliorated in mice by CRISPR-based in vivo genome editing of human Factor VIII

Chen

Shi

Gilam

et al. 2019

Sci Rep

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Hemophilia A is a monogenic disease with a blood clotting factor VIII (FVIII) deficiency caused by mutation in the factor VIII (F8) gene. Current and emerging treatments such as FVIII protein injection and gene therapies via AAV-delivered F8 transgene in an episome are costly and nonpermanent. Here, we describe a CRISPR/Cas9-based in vivo genome editing method, combined with non-homologous end joining, enabling permanent chromosomal integration of a modified human B domain deleted-F8 (BDD-F8) at the albumin (Alb) locus in liver cells. To test the approach in mice, C57BL/6 mice received tail vein injections of two vectors, AAV8-SaCas9-gRNA, targeting Alb intron 13, and AAV8-BDD-F8. This resulted in BDD-F8 insertion at the Alb locus and FVIII protein expression in the liver of vector-, but not vehicle-, treated mice. Using this approach in hemophilic mice, BDD-F8 was expressed in liver cells as functional human FVIII, leading to increased plasma levels of FVIII and restoration of blood clotting properties in a dose-dependent manor for at least 7 months, with no detectable liver toxicity or meaningful off-target effects. Based on these findings, our BDD-F8 genome editing approach may offer an efficacious, long-term and safe treatment for patients with hemophilia A.

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“…The supernatant was discarded to get platelet-rich plasma (PRP). Then the pellet was centrifuged at 3000 rpm for 5 min and the supernatant is the poor platelet plasma (PPP) [ 31 ]. PT, APTT, and TT were determined according to the kit instructions.…”

Section: Methodsmentioning

confidence: 99%

Anticoagulant Activities of Indobufen, an Antiplatelet Drug

Liu¹,

Xia

et al. 2018

Molecules

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Indobufen is a new generation of anti-platelet aggregation drug, but studies were not sufficient on its anticoagulant effects. In the present study, the anticoagulant activity of indobufen was determined by monitoring the activated partial thromboplastin time (APTT), prothrombin time (PT), and thrombin time (TT) in rabbit plasma. We evaluated the anticoagulant mechanisms on the content of the platelet factor 3,4 (PF3,4), and the coagulation factor 1, 2, 5, 8, 10 (FI, II, V, VIII, X) in rabbits, as well as the in vivo bleeding time and clotting time in mice. The pharmacodynamic differences between indobufen and warfarin sodium, rivaroxaban, and dabigatran were further studied on thrombus formation and the content of FII and FX in rats. Animal experiments showed that intragastric-administrated indobufen can significantly reduce the APTT, PT, TT, PF3, FI, II, V, VIII, and X plasma contents. Its inhibitory effect on plasma FII was better than thrombin inhibitor dabigatran with effect on FX better than FXa inhibitor rivaroxaban. These results suggest that indobufen has some anticoagulant effects as strong as some conventional anticoagulants. The mechanism may be related to both exogenous and endogenous coagulation system.

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A quantitative and humane tail bleeding assay for efficacy evaluation of antihaemophilic factors in haemophilia A mice

Cited by 9 publications

References 31 publications

Elimination of fibrin γ-chain cross-linking by FXIIIa increases pulmonary embolism arising from murine inferior vena cava thrombi

Elimination of fibrin γ-chain cross-linking by FXIIIa increases pulmonary embolism arising from murine inferior vena cava thrombi

Hemophilia A ameliorated in mice by CRISPR-based in vivo genome editing of human Factor VIII

Anticoagulant Activities of Indobufen, an Antiplatelet Drug

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