Abstract
Blood flow profoundly varies throughout the vascular tree due to its pulsatile nature and to the complex vessel geometry. While thrombus formation has been extensively studied in vitro under constant flow, and in vivo under normal blood flow conditions, increased attention has been paid to the impact of complex hemodynamics such as flow acceleration found in stenosed arteries. We investigated the effect of flow acceleration, characterized by shear rate gradients, on the function of platelets adhering to fibrinogen, a plasma protein which plays a key role in hemostais and thrombosis. While we confirmed that under constant flow, fibrinogen only supports single platelet adhesion, we observed that under shear rate gradients, this surface becomes highly thrombogenic, supporting efficient platelet aggregation leading to occlusive thrombus formation. Interestingly, this phenomenon is general as it occurs on other weak adhesive matrices including laminins and thrombospondin-1. This shear rate gradient-driven thrombosis is biphasic with an initial step of slow platelet recruitment supported by direct plasma von Willebrand factor (VWF) adsorption to immobilized fibrinogen and followed by a second phase of explosive thrombosis initiated by VWF fiber formation on platelet monolayers. In vivo experiments confirmed that shear rate gradients accelerate thrombosis in a VWF-dependent manner. Together, this study characterizes a process of plasma VWF-dependent accelerated thrombosis on weak adhesive proteins such as, fibrinogen in the presence of shear rate gradients.
Introduction
It has long been recognized that hemodynamics play important roles in hemostasis and thrombosis.1 A study coupling intravital microscopy to hydrodynamic studies provided evidence that shear gradients found at the site of vessel stenosis enhance thrombus formation in the post-stenotic area.2 The rheology-driven thrombi were essentially composed of discoid platelets as they formed independently of soluble agonists. Exacerbated platelet function and thrombosis in the poststenotic area was confirmed in another study, which proposed a role for von Willebrand factor (VWF) in this process.3 To date, the mechanism by which VWF exacerbates platelet activation and thrombosis under shear gradients has not been established. In addition to VWF, atherosclerotic plaque rupture exposes many other adhesive proteins including fibrinogen, which is known to support platelet adhesion and activation under low laminar blood flow conditions.4 However, whether this protein initiates and contributes to atherothrombosis under profoundly altered flow remains unknown.
VWF is a well-studied adhesive protein for platelets that is central in both hemostasis and arterial thrombosis.5 VWF is found in the subendothelium, in Weibel-Palade bodies of endothelial cells, in α-granules of platelets and in the plasma. Upon vascular injury, plasma VWF becomes rapidly adsorbed to several adhesive glycoproteins found at the site of injury, including collagen, laminins, thrombospondin, fibrin and fibronectin.6 Immobilized VWF then unfolds under the action of shear forces and exposes sites for the GPIb-IX-V complex supporting the recruitment of flowing platelets. VWF has the unique ability amongst all adhesive proteins to recruit platelets under elevated wall shear rate (WSR) conditions (>1,500 s-1).7-9 It has also been shown that unfolding of VWF is facilitated in the presence of shear gradients and elongational flow and can form a network of fibers which supports stable adhesion of several individual platelets.10-14
Fibrinogen is a soluble plasma glycoprotein which plays a pivotal role in hemostasis. In suspension, activation of platelets results in a change of the conformation of integrin αIIbβ3 which supports fibrinogen binding, allowing the formation of inter-platelet bonds, i.e, platelet aggregation. 15 When immobilized on a surface, fibrinogen supports attachment of resting platelets which is limited to low blood flow conditions (<1,000 s-1), as fibrinogen is not recognized to allow plasma VWF adsorption.7 The adhesive properties of fibrinogen under disturbed hemodynamic conditions remains completely unexplored. Understanding the effect of such flows on platelet adhesion to fibrinogen will help to better understand the mechanism underlying thrombosis since this pathological process is intimately linked to severely disturbed blood flow patterns.
This study evaluated the effect of shear rate gradients (SRG) such as those found at the entrance of a vessel stenosis, on platelet function on fibrinogen. A major finding is that fibrinogen becomes a highly thrombogenic surface under elevated SRG allowing the formation of occlusive thrombi. We identified and characterized a process of SRG-accelerated thrombosis that is bi-phasic with an initial step of slow platelet recruitment initiated through the ability of fibrinogen to adsorb plasma VWF, followed by a second stage during which VWF fibers of a couple of hundred microns form and initiate a very rapid accumulation of highly activated platelets to promote occlusive thrombosis. This process is general as it can be observed on other weak adhesive proteins such as laminins and thrombospondin- 1.
Methods
Preparation of microfluidic devices
Microfluidic devices were made from poly-dimethylsiloxane (PDMS) by standard soft lithography techniques according to published methods.16 Briefly, a patterned photoresistant-based mold was made by standard soft lithography techniques. The liquid prepolymer PDMS and its curing agent were mixed thoroughly at a volumetric ratio of 10:1, placed in a vacuum chamber to degas and poured onto the mold followed by curing at 70° C for 2 hours. The polymerized PDMS channels were then carefully peeled away from the mold and holes were punched at both extremities. Finally, the irreversible bonding of PDMS to glass coverslips was performed upon exposure of both surfaces to an oxygen plasma. We made a chamber containing: 5 cm long straight rectangular channels with a 1 mm width and 0.1 mm height constant section (Figure 1A; straight channel) and; stenosed channels with identical dimensions in addition to a symmetric stenosis showing a 90% lumen reduction in the central part of the channel (Figure 1A; stenosed channel). This symmetric two sided stenosed channel is composed of a constricted central part (zone 3) connected on both sides to rectangular sections similar to straight channel (zones 1 and 5) through linearly varying sections (zones 2 and 4). Finally, we made a chamber containing square section channels with a width of 0.1 mm, a height of 0.1 mm and a length of 5 cm.
Computational modeling of VWF dynamics
VWF dynamics was described with a model reported in.14 In order to reduce computational complexity, hydrodynamic correlations were not taken into account. The VWF dimer was treated as a sphere with a 70 nm radius. The polymer chain was represented as the chain of interconnected spheres, joined with Hookean springs. The interaction parameters were taken from.14 In order to infer conformational dynamics of VWF molecules within different flow lines of the chamber (flow lines lying within the central z-x plane were considered), the corresponding flow velocity profiles were taken from the computational fluid dynamic (CFD) simulation results. The local velocity gradient tensor was computed from polynomial interpolation of velocity profiles obtained from CFD simulations. In order to reduce the computational burden we considered VWF dynamics along the 1 mm of flow lines corresponding to stenosis entrance region (as far as this region possesses the highest values of elongational velocity gradients). VWF elongation d for a given moment of time was determined as maximum linear size of VWF molecule divided by the length of fully unfolded molecule. Values of VWF elongation exceeding unity correspond to flow-mediated extension of linear unfolded molecule. In case VWF elongation exceeded unity, the molecule was considered to be fully unfolded. In order to obtain a relative value of unfolding events we considered flow lines with different heights above fibrinogen surface: 1, 5, 10, 15 and 20 µm. For each height above the surface, 100 VWF trajectories were analyzed to infer the mean relative number of VWF unfolding events. The maximum relative number of unfolding events were analyzed for each flow line. Analysis was performed for long (n=80 dimers) VWF multimers.
In vivo FeCl3 thrombosis and stenosis
FeCl3-induced thrombosis was performed as previously described17–19 with some modifications. Briefly, 8-10 week-old mice were anesthetized by intraperitoneal injection of a mixture of xylasine (100 mg/kg) and ketamine (20 mg/kg). DiOC6 (0.4 µL of a 100 µM solution/g of body weight) was injected into the jugular vein to label the thrombus. The carotid artery was injured by lateral external application of a filter paper containing a 4% FeCl3 solution for 2.5 minutes (min). Four min after vessel injury, a 80% stenosis of the carotid or no stenosis (control) was obtained by compression with a micro-manipulator (Eppendorf Transferman, Hamburg, Germany). Thrombus formation was monitored with a fluorescent macroscope (Macrofluo®, Leica Microsystems, Rueil- Malmaison, France). Ethics approval for animal experimentation was obtained from the French Ministry of Research in accordance with the European Union Guidelines as defined by European laws.
Detailed methods are described in the Online Supplementary Materials and Methods.
Results
Development and characterization of a microfluidic device to study the effect of SRG on platelet adhesion to fibrinogen
We developed a PDMS-based microfluidic chamber with a 90% narrowing in its central region (zone 3) in order to generate SRG, similar to those found in pathological settings (Figure 1A). Micro-particle imaging velocimetry (microPIV) measurements performed while perfusing a 40/60 glycerol/PBS mixture to mimic the blood viscosity, at a flow rate of 30 µL/min, showed terminal acceleration of the flow at the end of zone 2 and the entry of the stenosis (zone 3), (Figure 1B-C). The maximal flow velocity of 0.115 m/s measured in the centerline of the stenotic area (Figure 1C) is very close to the expected 0.113 m/s computed from the mass flow rate conservation through the model and to that of the straight channel (data not shown). In agreement, the value of the absolute average of WSR (4,750±300 s-1) of zone 3 is also very close to the 4,800 s-1 for which the stenosed channel was designed. Reynolds numbers (Re) based on maximum centreline velocity and hydraulic diameter were characteristic of a laminar flow in all sections of the flow chamber (zone 1-5: Re=0.46; zone 3: Re=3.36) indicating the absence of turbulence. This laminar flow behavior was confirmed by the velocity profiles that can be inferred from the flow field measurements in the different sections of zone 3 (Figure 1D). In agreement with the microPIV measurements, computational fluid dynamic analysis indicated that the WSR were symmetrically distributed within the stenosed channel and of similar values (for 30 µL/min: zone 3 of 4,800 s-1) (Figure 1E-F). Finally, analytical solution of Navier-Stokes equation for infinitely long squareshaped channels20 with a corresponding volumetric flow rate gives a WSR value in the center line of zone 3 of 4,792 s-1, which is in line with CFD and microPIV results.
Effect of SRG on the function of platelet adhering to fibrinogen and other weak adhesive proteins
In agreement with previous reports,7 perfusion of hirudinated whole blood over immobilized fibrinogen in channels with a constant section results in a modest platelet adhesion under low WSR (300 s-1), and no platelet recruitment under high WSR (4,800 s-1), (Figure 2A-B). In sharp contrast, in zone 3 of the 90% narrowed channel, we observed that numerous platelets adhered at 4,800 s-1, and formed aggregates (Figure 2C-D). Control experiments indicated that this adhesion was specific as no platelet adhesion was observed in any region of the channel in the absence of coating or when the chamber was passivated with albumin (data not shown). The efficient platelet accumulation on fibrinogen in zone 3 did not rely on local geometry, since no platelet adhesion was observed at similar WSR (4,800 s-1) in a straight fibrinogen coated channel with identical dimensions as those of zone 3 (Online Supplementary Figure S1 and Figure 2E-F). We therefore concluded that the efficient adhesion on fibrinogen at high WSR (4,800 s-1) observed in zone 3, results from flow acceleration occurring upstream (exit of zone 2) which generates SRG (Figure 1C). At early time points, we observed a modest 34.3% increase in Ca2+ signaling of platelets adhering to zone 3 compared to those attaching in zone 1 (Figure 2G). In contrast, at later stages, numerous platelets were Annexin-V positive in zone 3 (4,800 s-1), but not in zone 1 (300 s-1), suggesting that the level of platelet activation increases over time and that SRG favor procoagulant platelet formation (Figure 2H-I). In agreement, a signal for fibrin was detected in zone 3 when recalcified citrated human blood was perfused (Figure 2J-K). When different SRG were used, we observed single platelets adhering at 2.5 s-1/m and 4.9 s-1/m, platelet aggregates started to form at 7.4 s-1/ m and became massive resulting in channel occlusion at 9.8 s-1/m and 12.2 s-1/m (Figure 2LM and Online Supplementary Video S1). Of importance, this phenomenon appears general as it also occurred on other weak adhesive proteins including vascular laminins and thrombospondin-1 (Online Supplementary Figure S2). Together, these results indicate that SRG can enhance platelet function on weak adhesive proteins, such as fibrinogen resulting in occlusive thrombosis.
Thrombus formation on fibrinogen under SRG is bi-phasic
To further characterize the SRG-mediated process of platelet aggregation on fibrinogen, video-microscopy experiments were conducted. Real-time analysis of the flow experiments revealed a stepwise process of in vitro thrombus formation on fibrinogen, with an initial phase characterized by a slow and heterogeneous recruitment of individual platelets, followed by a stage of very rapid platelet aggregation visualized after 180 seconds (s) (Online Supplementary Video S2 and Figure 3A). Importantly, platelet adhesion and thrombus growth occur at the entrance of zone 3. Quantification of the surface coverage confirmed the bi-phasic nature of platelet accumulation on fibrinogen in zone 3 (Figure 3B). This bi-phasic process contrasted with platelet adhesion in zone 1 within the same channel which was linear (Figure 3B). The second phase (180-360 s) led to a very marked acceleration of platelet accumulation, with a 3-fold slope increase when compared to early time points (<210 s) (Figure 3B-C). This bi-phasic platelet accumulation is original since platelet aggregation under flow is recognized to be linear over a very wide range of WSR in the classical model of “in vitro thrombus formation” when whole blood is perfused over collagen (data not shown).
Characterization of the first step of platelet adhesion to fibrinogen in the stenosed region
We next analyzed the mechanism involved in platelet adhesion to fibrinogen in zone 3. Two clinically used αIIβb3 blockers, ReoPro® and Integrilin®, completely prevented platelet adhesion in the straight control channel at 300 s-1, as well as in zone 3 of the stenosed channel (4,800 s-1), (Figure 4A-B). Blockade of GPIbα or VWF exhibited a similar effect in zone 3, but not in the control channel at 300 s-1 (Figure 4C-F). These results suggested that plasma VWF becomes adsorbed to fibrinogen under SRG. This was confirmed by VWF immunostaining in zone 3 after perfusion of platelet-poor plasma (PPP) through the channel (Figure 4G). VWF staining was also detected in zone 1 but the signal was much weaker when compared to zone 3 further demonstrating that VWF binds to fibrinogen (Figure 4H). Direct interaction between VWF and fibrinogen was demonstrated in a purified assay under static conditions showing a specific and dose-dependent binding of soluble VWF to immobilized fibrinogen (Figure 4I). The increased VWF adsorption observed in zone 3 might be the result of VWF unfolding. A computational modeling approach of VWF dynamics, indicated that SRG similar to those occurring in transition from zone 2 to zone 3, especially 9.8 s-1/ m and 12.2 s-1/ m, favored unfolding of VWF molecules (Figure 4J and Online Supplementary Video S3), while this was not the case under flow conditions found in zone 1 at 300 s-1 and zone 3 at 4,800 s-1 (Online Supplementary Figure S3). We observed a 27.5% reduction of VWF deposition in zone 3 when PPP was perfused in the absence of red blood cells, suggesting that these cells contribute to this process (Figure 4K). Together, these results demonstrate that platelet adhesion observed on fibrinogen in zone 3 relies on integrin αIIbβ3, the GPIb-IX complex, and on plasma VWF adsorption which is the result of its unfolding due to SRG.
Characterization of the second step of accelerated platelet aggregation in the stenosed region: a role for VWF fibers
Real-time video-microscopy showed that aggregates presented an unusual extended shape in the flow direction and contained VWF fibers (Figure 5A-B and Online Supplementary Video S2 and S4). The fibers were particularly long reaching several hundred microns. Confocal microscopy confirmed the presence of VWF fibers and showed that they did not form directly on the fibrinogen surface but rather on top of platelet monolayers (Figure 5C). Interestingly these fibers appeared concomitantly to the initiation of the accelerated thrombosis, suggesting a role for them in this process (Online Supplementary Video S4). This role was confirmed in an experiment in which blockade of the GPIbα/VWF axis with OS-1, once a platelet monolayer on fibrinogen had already formed, prevented the second phase of accelerated thrombosis (Figure 5D). Computational fluid dynamic simulation (CFD) of the flow around single adhered platelets in zone 3 demonstrates a very strong increase in shear at their surface (>10,000 s-1), suggesting that events of VWF unfolding are very likely to occur (Figure 5E). Moreover, computational analysis of VWF dynamics at different heights shows SRG-dependent increase of VWF unfolding with an increase of height above the fibrinogen surface, reaching a maximum at 10 µm above the surface (Figure 5F). This result provides an explanation for acceleration of thrombus growth due to SRG-mediated unfolding of VWF molecules, which might trigger VWF fiber formation. Besides, CFD also shows significant streamline contraction effects on a second layer of platelets (Figure 5G) which might be responsible for the observed increase in the rate of VWF and platelet transport to the surface of growing aggregates as illustrated in Figure 5H. Thus, enhanced VWF unfolding and fiber formation combined with streamline contraction effects might explain the observed acceleration of thrombus formation in zone 3.
SRG accelerate in vivo thrombus growth in a VWF-dependent manner
To evaluate whether SRG accelerate thrombus growth in vivo, an experimental thrombosis approach was used. A 4% FeCl3 solution was applied to the carotid artery of adult mice to injure the vessel wall, and once a monolayer of platelets had formed (~270 s), the artery was severely stenosed (>80%) with a micromanipulator to generate SRG. Measurements of blood flows in the mouse carotid with a Doppler probe combined to CFD analysis indicated that the SRG generated in such a setting were very similar to those we applied in vitro as they were reaching 8.6 s-1/m (Figure 6A). Intravital microscopy showed that thrombus formation occurred much earlier in a stenosed vessel compared to the control (Figure 6B and Online Supplementary Video S5). Quantification confirmed that thrombus formation was more rapid in the presence of a stenosis (Figure 6C-D). As expected thrombus formation was severely impaired in VWF-deficient mice under normal conditions (Figure 6E-F). Interestingly, even though a tendency of increased thrombosis could be observed in the presence of a stenosis in VWF-/- mice, no significant difference in the time of thrombus formation was observed in these mice in the presence or absence of a stenosis (Figure 6E-F). This result confirms that VWF plays a central role in the accelerated thrombosis that occurs under conditions of blood flow acceleration and SRG.
Discussion
In this study, we describe and characterize a process of bi-phasic thrombus formation on weak adhesive proteins such as fibrinogen taking place under blood flow acceleration which can be found in the vicinity of an atherosclerotic plaque. This process is original and differs from thrombus formation in perfusion assays occurring under physiological or pathological hemodynamic conditions by several features including: i) its occurrence on several weak adhesive surfaces such as fibrinogen, laminins or thrombospondin-1 which are well-known to support only single platelet attachment; ii) its bi-phasic nature with a first step of slow platelet recruitment followed by a second phase of very rapid platelet aggregation; iii) its high reactivity that results in rapid channel occlusion; iv) its crucial dependence on VWF, which is not only key in the first step of platelet recruitment to the surface, but is also required to initiate the second step of platelet aggregation through VWF fiber formation on pre-adherent platelets. The elevated reactivity of the thrombotic process occurring under SRG, was not only evidenced by the ability of platelets to adhere at high shear, but also by their increased activation, their pro-coagulant activity and by fibrin deposition resulting in occlusive thrombosis. This SRG-enhanced thrombus growth was also evidenced in vivo, after mechanically inducing a severe stenosis of a FeCl3-injured carotid artery. Our results are in line with the pioneer work of Nesbitt and co-authors who showed that shear rate gradients promote thrombus formation.2 While they proposed that this mechanism was largely independent of soluble agonists, we propose that the formation of highly reactive VWF fibers could promote enough activation to support platelet aggregation.
Our results are in line with previous reports7 showing that under normal blood flow conditions, immobilized fibrinogen recruits single platelets under low WSR with a threshold around 1,000 s-1 above which platelets fail to attach.7 The reason for the lack of attachment above 1,000 s-1 relies in the limited affinity of integrin αIIbβ3 for its ligand. 7 We were therefore surprised by the capacity of platelets to attach to immobilized fibrinogen at a high shear (4,800 s-1) in the restricted area of a 90% stenosed channel. This response is not due to the local square geometry of the microfluidic device (zone 3), since it is not observed in a straight channel with similar dimensions. Instead, this effect is most likely the result of profoundly altered flow conditions resulting from the stenosis which generates SRG. Numerical studies indicated that the SRG found in the transition from zone 2 to zone 3 favor unfolding of VWF multimers, a phenomenon known to increase its adsorption to adhesive substrates.9 This likely explains the significant increase of VWF binding to fibrinogen that we observed in zone 3. Moreover, VWF unfolding dissociates the A1/A2 region and thereby unblocks the binding site of GPIb-IX complex which explains platelet recruitment to immobilized fibrinogen observed in zone 3 at 4,800 s-1.21
A major observation of this work is the description of a physical and direct interaction between fibrinogen and VWF in a purified system. We show that VWF binds to fibrinogen both under static and flow conditions, however, the binding is markedly increased in conditions of SRG, which could be explained by an increased VWF unfolding. The reason why this interaction has been overlooked so far most likely relies in the fact that in the absence of SRG, the amount of fibrinogen-bound VWF is insufficient to support platelet recruitment at high shear. We observed that under SRG the amount of VWF adsorption to fibrinogen increases (zone 3), which explains platelet recruitment at high shear. The underlying mechanism probably relies in SRG-mediated VWF unfolding which favors its adsorption. Moreover, we propose that the streamline contraction effects taking place after platelet adhesion may participate as these effects favor VWF transport to the surface. We also observed that red blood cells modestly contribute to this process, potentially by shear diffusion-mediated transport of VWF.
A striking result of this work is the very rapid platelet aggregation occurring on platelet monolayers under SRG. Real-time video-microscopy showed that this event was concomitant to the formation of VWF fibers of several hundred microns long, which could represent a trigger. This was shown in vitro, since blockade of the GPIb/VWF interaction once the monolayer had already formed, completely prevented the rapid platelet aggregation process. Similar results were obtained in vivo as the acceleration of thrombosis occurring under SRG was also markedly reduced in VWF-deficient mice. Interestingly, the fibers did not form directly on the surface of the channels, but rather at a distance on top of adherent platelets or small aggregates. The reason why VWF fibers formed in the restricted region is the result of a combination of factors. Firstly, this process occurred under SRG which efficiently promote VWF unfolding that is a prerequisite for VWF self-association and fiber formation.14 Secondly, fiber formation took place several microns above the surface where numerical studies of the flow surrounding adherent platelets predicted extremely high shear rates (>10,000 s-1) which also favors VWF unfolding and fiber formation. Thirdly, simulation of VWF dynamics confirmed that VWF unfolding was maximal at 10 microns above the surface. Finally, CFD indicates streamline contraction effects at such sites which facilitate recruitment of plasma VWF and therefore fiber formation.
This study identified a process of bi-phasic thrombosis on weak adhesive surfaces. Such a process was previously reported on fibrillar collagen in a stenosed channel.22 In both cases the bi-phasic process occurred when the blood flow is accelerated. Acceleration is found throughout the vasculature due to the pulsatile nature of the blood flow and the complex geometry of the vessels. However, the bi-phasic thrombosis leading to vessel occlusion described herein was achieved only for elevated values of SRG. Interestingly, despite simple hemodynamic conditions in our microfluidic system (laminar and constant blood flow), the disturbance of flow caused by the stenosis results in a complex phenomena, including accelerated thrombosis. Therefore, we propose that this process observed in the microfluidic-scale system is most likely relevant to pathological flows which can be found in the vicinity of an evolved atherosclerotic plaque presenting a severe stenosis. This has been shown by the accelerated thrombosis that occurred in an injured carotid artery when a 80% stenosis was applied with a micromanipulator. Whether such thrombi contain large VWF fibers and whether such fibers represent a major trigger for occlusive thrombosis still needs to be demonstrated. Based on our observations it is tempting to speculate that blockade of VWF fiber formation could efficiently reduce the accelerated thrombosis occurring when the flow accelerates. In agreement with this view, it has recently been proposed that blockade of VWF self-association could represent a potential strategy to prevent arterial thrombosis, highlighting the therapeutic potential of interfering with SRG driven thrombosis.23 Marked flow acceleration also takes place in extracorporeal circulation systems notably at the site of tubing-connector junctions where sharp 90° angles are particularly prone to generate elevated SRG.24 Such devices were shown to adsorb plasma proteins including fibrinogen and to expose a surface to becoming thrombogenic under SRG, therefore explaining the occurrence of large thrombi notably in extracorporeal membrane oxygenation systems.24 Future studies should be conducted to determine the structure of these thrombi and evaluate whether they contain VWF fibers.
In summary, we describe and characterize a mechanism of bi-phasic thrombus formation that is initiated on immobilized fibrinogen, relies on VWF and occurs specifically under SRG. This process is general as it can be triggered on several weak adhesive surfaces, such as fibrinogen, laminins or thrombospondin-1, which become thrombogenic when they are subjected to blood flow acceleration generating SRG and elongational flow. Under such hemodynamic conditions, plasma VWF molecules become adsorbed to the surface allowing a modest recruitment of circulating platelets. This process is amplified on adherent platelets forming reactive VWF fibers that enhance platelet adhesion and activation, promote the procoagulant function of platelets, allow fibrin deposition and result in intense platelet aggregation and occlusive thrombosis (Figure 7).
Supplementary Material
Acknowledgments
We would like to thank Christophe Dubois for providing the anti-fibrin antibody.
Funding Statement
Funding This work was supported by ARMESA (Association de Recherche et Développement en Médecine et Santé Publique).
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