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HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
From the Australian Centre for Blood Diseases,
Department of Medicine, Monash Medical School, Australia.
The adhesion and aggregation of platelets at sites of vascular
injury is dependent on the initial binding of the GP Ib/V/IX receptor
complex to immobilized von Willebrand factor (VWF). Under flow
conditions, this interaction supports platelet translocation that is
characteristically stop-start in nature. High resolution imaging of
platelets during surface translocation on immobilized VWF revealed that
thin membrane tethers (length: 0.91 µm-47.90 µm) were pulled from
the surface of these cells. Membrane tethers were dynamic structures
that extended from small, localized adhesion contacts under the
influence of flow. Perfusion of platelets in the presence of blocking
antibodies against integrin The formation of stable adhesion contacts between
circulating blood cells, such as platelets and leukocytes, and the
injured vessel wall requires specialized adhesion mechanisms capable of withstanding the mechanical forces generated by flowing blood. It has
recently become apparent that platelets and leukocytes utilize a
similar multistep adhesion mechanism, albeit through entirely different
ligand-receptor pairs,1,2 that enables efficient cell
adhesion under flow. In the initial stages of platelet and leukocyte
adhesion, receptor-ligand interactions with inherently rapid bond
kinetics support cell tethering onto the vessel wall. These bonds are
reversible, such that tethered cells subjected to hydrodynamic drag
forces roll or translocate over the injured vessel wall. Rolling is
indispensable for normal platelet and leukocyte function as it serves
to decelerate cell movement relative to flowing blood, allowing
receptors with slower bond kinetics (ie, integrins) to engage adhesive
ligands and mediate firm cell adhesion.3,4
The molecular basis of cell rolling has been primarily determined from
in vitro and in vivo studies on leukocytes. In rolling cells, adhesive
bond formation between selectin family members and their corresponding
carbohydrate ligands is balanced by continuous bond breakage. This
process is facilitated by the clustering of selectins and their ligands
(eg, L-selectin, PSGL-1) at the tips of microvilli.5-7 In
support of this, disruption of these membrane structures with
cytochalasin B, or redistribution of L-selectin from microvilli to the
body of the cell, are associated with decreased leukocyte adhesion and
rolling.8,9 Adhesion of leukocytes via these microvilli is
thought to result in the formation of a cluster of tethered bonds that
when subjected to tensile forces, results in the elongation of
microvilli into thin membrane tethers. Tether formation has been
proposed to account for the 2 distinct behaviors observed in rolling
leukocytes, where tether stretching represents the slow, smooth rolling
phase and release of membrane tethers represents the intermittent
stepwise or jerky phases.10
The formation of membrane tethers has been extensively studied in
erythrocytes, using micropipette techniques to extend the membrane into
thin, elongated membrane tethers.11,12 During this
process, the plasma membrane is thought to flow from the cell body over
the underlying cytoskeletal layer, forming a hollow cylinder of lipid
bilayer. In this model, the rigid membrane skeleton is unable to deform
from its original state, causing it to become either fragmented or
completely separated from the lipid bilayer.13 A similar
response has also been described in neutrophils, whereby applying a
pulling force to surface microvilli results in membrane tether
extrusion.14 More recently, membrane tether formation has
been directly observed in neutrophils interacting with adherent platelets as well as immobilized P-selectin.15 The
extension of membrane tethers during neutrophil rolling may be
important for reducing the level of stress experienced by individual
receptor-ligand interactions, thereby increasing the likelihood of
rolling cells forming stable adhesion contacts.
Like leukocytes, platelets have also been observed to roll in
vitro4,16 and at sites of vascular injury in
vivo.17 Platelet rolling not only occurs on the injured
vessel wall but also on the surface of thrombi, and is mediated by the
interaction between the A1 domain of immobilized von Willebrand factor
(VWF) with the platelet glycoprotein (GP) Ib/V/IX receptor complex.
This rolling interaction is characteristically stop-start in nature, wherein transient stationary adhesion contacts are interspersed by
periods of rapid translocation. Our recent studies have demonstrated that platelets undergo changes in morphology during surface
translocation, converting from disc-shaped cells into irregular spheres
extending multiple filopodia16; however, to date there are
no reports of membrane tether formation during platelet translocation.
In this study, we have examined platelet morphologic changes during the
initial interaction of platelets with immobilized VWF under shear
conditions, using high-resolution differential interference contrast
microscopy. We demonstrate that platelets extend membrane tethers
during surface translocation on immobilized VWF. Tether formation in
rolling platelets does not require changes in either the actin or
microtubular components of the cytoskeleton and occurs independently of
calcium mobilization and other platelet activation events. We show that
tether formation occurs as a function of shear rate and plays a
potentially important role in modulating the dynamics of the
platelet-VWF interaction.
Materials
Preparation of washed platelets
Flow studies and analysis of tether formation Flow assays were performed according to a modified method of Yap et al.21 Rectangular glass microcapillary tubes (Microslides; Vitro Com, Mountain Lakes, NJ) were coated with either human VWF (100 µg/mL) or an isolated 39/34 kd fragment of VWF (174 µg/mL) overnight at 4°C and subsequently blocked with 10% heat-inactivated human serum (containing 50 µg/mL phenylmethylsulfonyl fluoride) at room temperature for 60 minutes. Platelets in PWB (3 × 108/mL) were perfused through VWF-coated microcapillary tubes at 150 s 1 to
enable platelet interaction with the VWF matrix. Activation inhibitors
were removed by subsequent perfusion of modified Tyrode buffer (10 mM
HEPES, pH 7.4, 12 mM NaHOC3, 137 mM NaCl, 2.7 M KCl, 5 mM
glucose, 1 mM CaCl, and 1 mM MgCl) through the microcapillary tubes.
Tether formation in translocating platelets was visualized by
differential interference contrast microscopy (DMIRB Leica microscope;
×100 objective) and 10 random fields video-recorded for offline
analysis. In some experiments, platelets were pretreated with the
anti-integrin  IIb 3 c7E3 Fab (20 µg/mL)
or peptidomimetic Aggrastat (0.25 µg/mL) for 10 minutes to block
ligand binding to integrin IIb3. VWF
binding to GP Ib/V/IX was blocked by pretreating platelets with the
anti-GP Ib antibody, AK2 (5 µg/mL). In experiments examining the
effect of increasing shear on the rate and stability of tether
formation, platelets were initially perfused through the microcapillary
tubes at either 600 s1, 1800 s1, 5000 s1, or 10 000 s1. The flow was
subsequently reduced to 150 s1 for 5 seconds (to bring
platelets in close proximity to the VWF surface) and the wall shear
rate was subsequently increased back to its original rate. Under these
conditions platelets were not observed to interact with the VWF surface
at 150 s1; however, upon increasing the wall shear rate,
platelets were observed to rapidly interact and translocate across the
VWF surface. In these experiments, platelet translocation velocity was
determined by measuring the distance traveled (displacement) per unit
time recorded. The video monitor was calibrated using a 0.01-µm stage micrometer (Olympus, Tokyo, Japan). Images were digitized using the Microcomputer Imaging Device (MCID) software (Imaging Research, Ontario, ON, Canada). To investigate the frequency of tether formation under high shear conditions (600 s1, 1800 s1, 5000 s1, or 10 000 s1),
the flow assay was modified slightly. We have previously established that perfusing platelets through microcapillary tubes at high shear, in
the absence of red blood cells, leads to minimal platelet-VWF interaction.16 In contrast, perfusing platelets through
the capillary tubes at low flow rates, allowing the cells to come into
close contact with the matrix under the influence of gravity, then
suddenly exposing the cells to rapid increases in shear (ie, from 150 s1 up to 10 000 s1) resulted in platelets
rapidly and efficiently tethering to the VWF surface. In other studies,
platelets in PWB were preincubated with prostaglandin E1
(0.5 µg/mL), vinblastine (10 µg/mL), or paclitaxel (2 µM) for 20 minutes prior to perfusion, or cytochalasin D (5 µM) for 10 minutes
prior to perfusion. In studies examining the role of intracellular
calcium in tether formation, platelets in PWB were treated with
DM-BAPTA BAPTA (70 µM) for 30 minutes at 37°C. Platelets were
subsequently pelleted at 2000g and resuspended in PWB in the
presence of EGTA/Mg2+ (1 mM each) prior to perfusion
through VWF-coated microcapillary tubes.
Immunofluorescence studies Translocating platelets were fixed by perfusion of 4% formaldehyde in modified Tyrode buffer through microcapillary tubes for 2 minutes. Adherent cells were permeabilized with 2% Triton X-100 and stained with fluorescein isothiocyanate (FITC)-conjugated phalloidin or a monoclonal anti--tubulin antibody. Cells were washed with
phosphate-buffered saline (PBS) prior to incubation with a
CY5-conjugated anti-mouse antibody and imaged by confocal microscopy.
Scanning electron microscopy Translocating platelets were fixed by perfusion of 2% gluteraldehyde in scanning electron microscopy buffer (100 mM Na2HPO4/NaH2PO4, pH 7.4) through microcapillary tubes for 2 minutes. The upper surface of the rectangular glass microcapillary tube was removed by scoring the glass with a diamond pen; the lower surface was retained. Adherent cells were dehydrated and critical point dried as described previously,22 then mounted on scanning electron microscopy stubs and coated with gold. Stubs were stored under desiccation until imaging on a Hitachi S570 scanning electron microscope (Tokyo, Japan) at 15 kV accelerating voltage.Statistical analysis Significant differences were determined using a Student t test using the Prism software package (GraphPAD Software for Science, San Diego, CA).
Tether formation during platelet translocation on VWF To examine the morphology of platelets during surface translocation on VWF, initial studies were performed on washed platelets under low shear conditions (150 s1). We have
previously established that these conditions allow high-resolution
imaging of platelets in the absence of other blood cells.16 As demonstrated in Figure
1A, platelets initially tethered to VWF
as flat-disc shaped cells and translocated in a continuous stop-start
manner over the VWF surface, as described previously.4,16 In some cases, platelets underwent prolonged periods of stationary adhesion (> 10 seconds) that resulted in the development of single elongated membrane extensions (tethers) at the trailing edge of the
cell (Figure 1A). These membrane tethers developed from small, localized adhesion contacts formed between the cell body and VWF matrix. The formation of adhesion contact points caused a slight teardrop-shaped deformation of the platelet membrane as the cell body
gradually pulled away in response to the drag forces created by flow
(Figure 1A). As a result, long, thin membrane tethers were seen to
extend between the attachment point and the cell body (Figure 1A). In
this regard, they were distinct from filopodia, as tethers were always
aligned parallel to the direction of flow, with the tether attachment
point facing upstream and the cell body downstream. In contrast,
filopodia did not form as a result of a direct interaction between the
membrane and VWF matrix, but tended to randomly extend out from the
cell body in all directions as freely mobile membrane protrusions. The
formation of membrane tethers was not dependent on VWF engagement of
integrin IIb3, as pretreating platelets
with the integrin IIb3 antagonists, c7E3
Fab, or Aggrastat had no inhibitory effect on tether formation. Further
evidence that membrane tethers were primarily induced by the VWF-GP
Ib/V/IX interaction was obtained from studies using the 39/34
proteolytic fragment of VWF, containing the GP Ib binding domain (A1 domain). Translocation of platelets on isolated A1 domain
resulted in the formation of membrane tethers that were similar in
length and morphology to those observed on full-length VWF (Figure 1A).
The extension of tethers on A1 domain was specific to GP Ib as
platelet adhesion was fully blocked with the anti-GP Ib antibody
ALMA12 (20 µg/mL).
Analysis of tethers by scanning electron microscopy revealed that the
majority of membrane tethers formed at 150 s Real-time analysis of tether formation at low wall shear rates
(150 s
Effect of shear on tether formation and stability in translocating platelets The strength of the tether attachment point was examined more closely by assessing the effect of increasing shear force on its ability to resist detachment and maintain stable platelet adhesion to immobilized VWF. As demonstrated in Figure 3A, a stably adherent platelet developed a membrane tether over a 60-second time period, after which the tether length increased slowly. This plateau in tether growth rate after initial tether formation was a consistent finding in all platelets examined under low shear conditions. Incremental increases in the wall shear rate from 150 s1 to 600 s1 to 1800 s1 resulted in a corresponding increase in tether length
from 5.4 µm to 12.9 µm to 23.3 µm, respectively. However, at 1800 s1 the tether contact points were unable to sustain
stationary platelet adhesion. This shear-induced conversion of tethered
platelets from stably adherent to rolling cells involved releasing the
tether contact point from the matrix. At no stage was the membrane
tether observed to detach from the cell body (data not shown). Instead, the tether participated in the translocation process along with the
cell body (Figure 4A), or alternatively,
retracted back into the cell (Figure 4B). The retraction process
involved contraction of the tether into small membrane blebs along the
length of the tether, gradually receding back into the cell
(Figure 4B,C).
In further studies, we examined whether translocating platelets were
able to form membrane tethers at shear rates of more than 150 s
Analysis of individual platelets during surface translocation at high
wall shear rates (5000 s
Effect of tether formation on platelet translocation To gain insight into the potential role of tether formation in regulating the dynamics of the platelet-VWF interaction, we examined the velocity of platelet translocation before, during, and after tether formation. As demonstrated in Figure 7, platelets translocated in a stop-start manner over a broad range of shear conditions (150 s1-5000 s1). At low
shear rates (150 s1), the formation of a membrane tether
(shaded region) resulted in a sudden cessation in platelet movement
followed by a slight increase in the displacement of the cell centroid
over time as the tether gradually lengthens. At the point in which the
tether attachment point is unable to maintain stable adhesion with the matrix (124"), the platelet reinitiates surface translocation. It
should be noted that not all stationary phases were associated with
membrane tether formation (eg, see Figure 7; 18-28 seconds and 134-146 seconds), raising the possibility that additional mechanisms regulate
the dynamics of the platelet-VWF interaction. In contrast to low shear,
at 1800 s1 and 5000 s1 tether development
was far more rapid (occurring over a few seconds) and continuous, with
multiple tethers forming during translocation (shaded regions in Figure
7). In most cases, the development of tethers at these higher wall
shear rates correlated with the short periods of stationary adhesion or
the "stop" phase of the translocation process, whereas the
"start" phase of translocation was a result of the tether releasing
its contact point from the matrix. However, when extremely long
membrane tethers developed rapidly (eg, Figure 7; first tether at 1800 s1 [18 seconds]), a significant difference in
translocation velocity prior to and during tether formation was
not observed.
Role of the cytoskeleton in regulating platelet tether formation In further studies, we examined the role of the platelet cytoskeleton in promoting membrane tether formation. Initially we examined for the presence of actin filaments and/or microtubular structures within membrane tethers. As demonstrated in Figure 8A, staining of the actin cytoskeleton with FITC-conjugated phalloidin revealed that all cells exhibited a diffuse pattern of staining within the cell body and membrane tether. In contrast, immunofluorescent analysis of the same cells using a-tubulin antibody revealed a distinct microtubule ring around the
circumference, with no staining of microtubules within the membrane
tether (Figure 8A). In contrast, filopodial projections in
translocating platelets stained strongly for both actin filaments and
microtubules (Figure 8Aii), further highlighting the structural
differences between filopodia and membrane tethers.
To investigate the potential importance of the actin cytoskeleton in
regulating tether formation and retraction, platelets were pretreated
with the actin polymerisation inhibitor, cytochalasin D. Under all
shear conditions (150 s
Role of platelet activation and calcium in regulating tether dynamics We have recently demonstrated that VWF engagement of GP Ib induces increases in cytosolic calcium and reorganization of actin filaments, via signaling processes sensitive to the inhibitory effects of cAMP.16 To investigate the ability of elevated levels of cAMP to inhibit the formation of membrane tethers, platelet translocation studies were performed in the presence of the cAMP phosphodiesterase inhibitor, theophylline. Interestingly, perfusion of platelets under these conditions had no effect on the rate, extent, or morphology of tethers pulled from the surface of translocating platelets (data not shown). Furthermore, combining theophylline with a stimulator of adenylyl cyclase, prostaglandin E1, also had no effect on tether formation. Chelating cytosolic calcium, by pretreating platelets with DM-BAPTA, did not inhibit tether formation; however, these tethers were longer (Figure 9A) and finer (data not shown), similar to those observed with cytochalasin D. However, unlike cytochalasin D, DM-BAPTA did not induce the formation of unstable tethers. Reducing cytosolic calcium with DM-BAPTA did not affect the retraction of membrane tethers but did have a significant effect on the shear-dependent decrease in tether lifetime observed in control platelets (Figure 9B). As a result, the average lifetime of tethers was significantly shorter at 150 s1, 600 s1,
and 1800 s1 (4.86 sec, 1.52 sec, and 1.51 sec,
respectively) than in untreated controls (270.0 sec-13.07 sec).
The studies presented here demonstrate a new platelet phenomenon, the shear-dependent elongation of membrane tethers during surface translocation on immobilized VWF. Membrane tethers are dynamic structures that extend from small, localized adhesion contacts under the influence of hydrodynamic shear stress. Interestingly, all aspects of tether dynamics, including tether growth rate and dimensions, lifetime of adhesive contact with the matrix, and retractile dynamics are influenced by the shear conditions experienced by the cell. Tether formation appears to regulate, at least in part, the stop-start nature of platelet translocation on VWF, raising the interesting possibility that tether formation represents a previously hitherto unrecognized mechanism regulating platelet adhesion under flow. Recent studies have demonstrated that neutrophils also form membrane
tethers during surface translocation,15 although in these
cells, tether formation is dependent on the interaction between PSGL-1
and immobilized P-selectin. In contrast to the VWF-GP Ib interaction,
PSGL-1-P-selectin bonds can only support neutrophil tethering and
rolling under low shear conditions (50 s It is of interest that less than 5% of platelets at low shear
developed membrane tethers during surface translocation. This low
frequency of tether formation is not due to the presence of a distinct
subpopulation of "tether-forming" platelets, as increasing the wall
shear rate up to 10 000 s The results presented here demonstrate for the first time that the
VWF-GP Ib/V/IX interaction can support prolonged stationary cell
adhesion (> 10 seconds) under physiologic flow conditions, independent
of integrin The low percentage of platelets forming tethers under low shear
conditions suggests that this phenomena is unlikely to play a major
role in regulating platelet translocation velocity in the venous
circulation. However, at high shear the vast majority of platelets
develop membrane tethers, raising the interesting possibility that
tether formation is a key step in the platelet adhesion process under
high shear. These observations may not be surprising given that tether
formation has been proposed to reduce the level of force exerted on
adhesive bonds.14 As demonstrated in Figure
10, in the case of reversible adhesive
interactions, such as those formed between VWF and GP Ib/V/IX,
hydrodymanic forces generated by flowing blood rapidly undermine the
formation of stationary adhesion contacts. By forming tethers, adhesive bonds more effectively oppose shear forces by increasing the moment arm
(see Figure 10 legend for detailed explanation). Thus platelets, as
well as leukocytes, appear to have evolved tethering mechanisms that
serve to retard the velocity of cell translocation, albeit transiently,
thereby increasing the probability of receptors with intrinsically slow
kinetics (ie, integrins) forming irreversible adhesion contacts.
We thank Prof Michael Berndt and Dr Francois Lanza for helpful suggestions and the generous donation of monoclonal antibodies.
Submitted April 17, 2001; accepted August 27, 2001.
Supported by grants from the National Health and Medical Research Council of Australia, National Heart Foundation of Australia, and the Welcome Trust (London, UK).
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Shaun P. Jackson, Australian Centre for Blood Diseases, Monash Medical School, Box Hill Hospital, Box Hill, Victoria 3127, Australia; e-mail: shaun.jackson{at}med.monash.edu.au.
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© 2002 by The American Society of Hematology.
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 J. M. Auger and S. P. Watson Dynamic Tyrosine Kinase-Regulated Signaling and Actin Polymerisation Mediate Aggregate Stability Under Shear Arterioscler Thromb Vasc Biol, August 1, 2008; 28(8): 1499 - 1504. [Abstract] [Full Text] [PDF]
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S. P. Jackson The growing complexity of platelet aggregation Blood, June 15, 2007; 109(12): 5087 - 5095. [Abstract] [Full Text] [PDF]
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K. J. Clemetson How complex is the platelet GP Ib complex? Blood, January 15, 2007; 109(2): 393 - 394. [Full Text] [PDF]
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A. J. Reininger, H. F. G. Heijnen, H. Schumann, H. M. Specht, W. Schramm, and Z. M. Ruggeri Mechanism of platelet adhesion to von Willebrand factor and microparticle formation under high shear stress Blood, May 1, 2006; 107(9): 3537 - 3545. [Abstract] [Full Text] [PDF]
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J. M. Dyson, A. D. Munday, A. M. Kong, R. D. Huysmans, M. Matzaris, M. J. Layton, H. H. Nandurkar, M. C. Berndt, and C. A. Mitchell SHIP-2 forms a tetrameric complex with filamin, actin, and GPIb-IX-V: localization of SHIP-2 to the activated platelet actin cytoskeleton Blood, August 1, 2003; 102(3): 940 - 948. [Abstract] [Full Text] [PDF]
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S. M. Schoenwaelder, S. C. Hughan, K. Boniface, S. Fernando, M. Holdsworth, P. E. Thompson, H. H. Salem, and S. P. Jackson RhoA Sustains Integrin alpha IIbbeta 3 Adhesion Contacts under High Shear J. Biol. Chem., April 19, 2002; 277(17): 14738 - 14746. [Abstract] [Full Text] [PDF]
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Top
Abstract
Introduction
(where 
, to which it is applied at the adhesive
surface. Tether formation increases the horizontal component of
Fb (Fbcos