The Impact of Blood Shear Rate On Arterial Thrombus Formation

Sakariassen, Kjell S.; Örning, Lars; Turitto, Vincent T.

doi:10.4155/fso.15.28

Cited by 185 publications

(192 citation statements)

References 53 publications

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“…The T‐TAS is a microchip‐based flow‐chamber system that measures thrombus formation under physiological blood flow conditions , and was used to confirm the effects of the aPCC–SIA and rFVIIa–SIA combinations. Shear rates of 600 s −1 and 240 s −1 on collagen/TF‐coated AR‐chips were used to represent average‐sized arteries and veins, respectively .…”

Section: Resultsmentioning

confidence: 99%

In vitro studies show synergistic effects of a procoagulant bispecific antibody and bypassing agents

Hartmann¹,

Feenstra²,

Valentino

et al. 2018

Journal of Thrombosis and Haemostasis

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Background Investigational non-factor products such as emicizumab offer a treatment option for patients with hemophilia and inhibitors. However, their mechanism of action raises questions regarding safety when they are combined with treatments for breakthrough bleeding. Objectives To evaluate in vitro thrombin generation (TG) and clot formation for combinations of activated prothrombin complex concentrate (aPCC), recombinant activated factor VII (rFVIIa), and a sequence-identical analog of emicizumab (SIA). Methods Therapeutic concentrations of SIA (20-600 nm) alone or with aPCC (0.05-1 U mL ), isolated aPCC components or rFVIIa (0.88-5.25 μg mL ) were tested for TG and compared with reference ranges for healthy donor plasma. Coagulation of FVIII-inhibited blood was determined with a widely established method, i.e. rotational thromboelastometry (ROTEM), and confirmed with the Total Thrombus-formation Analysis System. Results and conclusions SIA (600 nm) or aPCC (0.5 U mL ) alone resulted in peak thrombin levels of 21.4 nm and 38.6 nm, respectively, both of which are lower than normal (83.7 ± 29.8 nm). SIA plus aPCC (0.5 U mL ) increased the peak thrombin level 17-fold over SIA alone, exceeding the reference plasma value by 4.2-fold. This hypercoagulable effect occurred with 600 nmSIA combined with as little as 0.25 U mL aPCC, confirmed by ROTEM. FIX was the main driver for enhanced TG. SIA plus rFVIIa (1.75 μg mL ) induced a 1.8-fold increase in the peak thrombin level in platelet-rich plasma, but it did not reach the normal range. These in vitro experiments demonstrate excessive TG after administration of a combination of aPCC and SIA at clinically relevant doses. Careful judgement may be required when breakthrough bleeding is treated in patients receiving emicizumab.

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Section: Resultsmentioning

confidence: 99%

In vitro studies show synergistic effects of a procoagulant bispecific antibody and bypassing agents

Hartmann¹,

Feenstra²,

Valentino

et al. 2018

Journal of Thrombosis and Haemostasis

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“…The subcommittee recommends using direct thrombin inhibitors such as D‐phenylalanyl‐prolyl‐arginyl chloromethyl ketone (P‐Pack; 50 μM) or hirudin (100 U/mL), which are very potent direct thrombin inhibitors allowing one to work with human blood for up to 3 hours and with mouse blood for up to 2 hours. Other anticoagulants, notably trisodium citrate (0.38%), which is broadly available, can be used; however, citrated blood tends to form larger thrombi than the direct thrombin inhibitors as Ca 2+ chelation results in enhanced TxA2 production Flow device: Whole blood flow perfusion over collagen is a very robust and reproducible assay that works with flow devices including parallel plate flow chambers, microslides, commercial devices, and microfluidic channels.…”

Section: Recommendation For Standardization Of the “In Vitro Thrombosmentioning

confidence: 99%

“…Other anticoagulants, notably trisodium citrate (0.38%), which is broadly available, can be used; however, citrated blood tends to form larger thrombi than the direct thrombin inhibitors as Ca 2+ chelation results in enhanced TxA2 production. 25…”

Section: Flow-ba S Ed a Ssays To D Iss Ec T The Vari Ous Pl Atele Tmentioning

confidence: 99%

In vitro flow based systems to study platelet function and thrombus formation: Recommendations for standardization: Communication from the SSC on Biorheology of the ISTH

Mangin

Gardiner

Nesbitt

et al. 2020

Journal of Thrombosis and Haemostasis

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Experimental videomicroscopic in vitro assays of thrombus formation based on blood perfusion are instrumental in a wide range of basic studies in thrombosis, screening for hereditary or acquired plateletrelated pathologies, and assessing the effectiveness of novel anti‐platelet therapies. Here, we discuss application of the broadly used “in vitro thrombosis model”: a frequently used assay to study the formation of 3D aggregates under flow, which involves perfusing anticoagulated whole blood over fibrillar collagen in a flow geometry of rectangular cross‐section, such as glass microcapillaries or parallel‐plate flow chambers. Major advantaged of this assay are simplicity and ability to reproduce the four main stages of platelet thrombus formation, i.e. platelet tethering, adhesion, activation and aggregation under a wide range of hemodynamic conditions. On the other hand, these devices represent, at best, simple reductive models of thrombosis. We also describe how blood flow assays can be used to study various aspects of platelet function on adhesive proteins and discuss the relevance of such flow models. Finally, we propose recommendations for standardization related to the use of this assay that cover collagen source, coating methods, micropatterning, sample composition, anticoagulation, choice of flow device, hemodynamic conditions, quantification challenges, variability, pre‐analytical conditions and other issues.

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“…Human platelets normally circulate in a resting state and are exposed to shear rates within a physiologic range (~20‐2000 s −1 ) . Platelets may encounter shear rates well beyond 10 000 s −1 under pathologic conditions, for example, in a stenosed atherosclerotic artery or within mechanocirculatory support devices such as left ventricular assist devices (LVADs) or extra‐corporeal membrane oxygenation (ECMO) devices, and become activated and begin to aggregate.…”

Section: Triggers Of Platelet Receptor Sheddingmentioning

confidence: 99%

“…Platelets may encounter shear rates well beyond 10 000 s −1 under pathologic conditions, for example, in a stenosed atherosclerotic artery or within mechanocirculatory support devices such as left ventricular assist devices (LVADs) or extra‐corporeal membrane oxygenation (ECMO) devices, and become activated and begin to aggregate. Shear‐dependent platelet activation is initiated by binding of plasma VWF to platelets primarily through GPIbα, leading to platelet activation, secretion of ADP, and other agonists, and αIIbβ3‐dependent aggregation . Additionally, when exposed to elevated fluid shear stress, metalloproteolytic shedding of GPVI is triggered .…”

Section: Triggers Of Platelet Receptor Sheddingmentioning

confidence: 99%

Proteolytic processing of platelet receptors

Gardiner

2018

Research and Practice in Thrombosis and Haemostasis

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Essentials Metalloproteinases regulate release/shedding of bioactive membrane proteins.Shedding is critically important for normal cell function in the vasculature.Levels of platelet receptors GPIb‐IX‐V and GPVI are regulated by metalloproteolytic shedding.The premier platelet sheddases belong to the A Disintegrins And Metalloproteinase (ADAMs) family.Modulating ADAM activity may alter platelet adheso‐signalling receptor density and function. Platelets have a major role in hemostasis and an emerging role in biological processes including inflammation and immunity. Many of these processes require platelet adhesion and localization at sites of tissue damage or infection and regulated platelet activation, mediated by platelet adheso‐signalling receptors, glycoprotein (GP) Ib‐IX‐V and GPVI. Work from a number of laboratories has demonstrated that levels of these receptors are closely regulated by metalloproteinases of the A Disintegrin And Metalloproteinase (ADAM) family, primarily ADAM17 and ADAM10. It is becoming increasingly evident that platelets have important roles in innate immunity, inflammation, and in combating infection that extends beyond processes of hemostasis. This overview will examine the molecular events that regulate levels of platelet receptors and then assess ramifications for these events in settings where hemostasis, inflammation, and infection processes are triggered.

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The Impact of Blood Shear Rate On Arterial Thrombus Formation

Cited by 185 publications

References 53 publications

In vitro studies show synergistic effects of a procoagulant bispecific antibody and bypassing agents

In vitro studies show synergistic effects of a procoagulant bispecific antibody and bypassing agents

In vitro flow based systems to study platelet function and thrombus formation: Recommendations for standardization: Communication from the SSC on Biorheology of the ISTH

Proteolytic processing of platelet receptors

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