Yoda1 | CRET Signal

Piezo1 acts upstream of TRPV4 to induce pathological changes in endothelial cells due to shear stress

Abstract
The ion channels Piezo1 and TRPV4 have both, independently, been implicated in high venous pressure- and fluid shear stress-induced vascular hyperpermeability in endothelial cells. However, the mechanism by which Piezo1 and TRPV4 channels execute the same function is poorly understood. Here we demonstrate that Piezo1 regulates TRPV4 channel activation in endothelial cells and that Piezo1- mediated TRPV4 channel opening is a function of the strength and duration of fluid shear stress. We first confirmed that either fluid shear stress or the Piezo1 agonist, Yoda1, led to an elevation in intracellular calcium ([Ca2+]i), and that application of the Piezo1 antagonist, GsMTx4, completely blocked this change. We discovered that high and prolonged shear stress caused sustained [Ca2+]i elevation which was blocked by inhibition of TRPV4 channel opening. Moreover, Piezo1 stimulated TRPV4 opening through activation of phospholipase A2. TRPV4-dependent sustained [Ca2+]i elevation was responsible for fluid shear stress- and Piezo1-mediated disruption of adherens junctions and actin remodeling. Blockade of TRPV4 channels with the selective TRPV4 blocker, HC067047, prevented the loss of endothelial cell integrity and actin disruption induced by Yoda1 or shear stress and prevented Piezo1-induced monocyte adhesion to endothelial cell monolayers. These findings demonstrate that Piezo1 activation by fluid shear stress initiates a calcium signal that causes TRPV4 opening which in turn is responsible for the sustained phase calcium elevation that triggers pathological events in endothelial cells. Thus, deleterious effects of shear stress are initiated by Piezo1 but require TRPV4.

Introduction
Endothelial cells are under constant mechanical force due to blood pressure and flow in both the arterial and venous systems. Blood flowing across endothelial cells within blood vessels generates shear stress.Under normal physiological conditions, a dynamic balance between mechanical shear stress and biological responses maintains endothelial integrity (1- 5). Shear stress induces the release of endothelial vasodilatory factors such as nitric oxide, prostacyclin, and cytochrome P-450 metabolites of arachidonic acid that are required for surrounding smooth muscle relaxation (6-8). Endothelial Ca2+-mediated mechanosensing is required for normal flow-mediated dilation (4,5). Perturbation of endothelial shear stress that occurs with hypertension or excessive flow leads to vascular remodeling through the disruption of cytoskeletal proteins and vascular dysfunction involving the loss of endothelial integrity, increased endothelial cell stiffness, altered vasorelaxation properties, and leukocyte adhesion (2,3,9-13).Clinically, high venous pressure is a major cause of pulmonary edema and mortality in patients with congestive heart failure (10,11). Elevatedvascular pressure can lead to endothelial barrier disruption and hyperpermeability due to loss of adherens junctions (AJs) between endothelial cells (3,11). It has recently been demonstrated that the mechanosensitive ion channel Piezo1 mediates pressure-induced disruption of AJs and endothelial barrier breakdown in pulmonary vessels (11,14). Piezo1 is activated by cell membrane tension caused by high pressure, shear stress and membrane stretching which allow the influx of cations, mainly Ca2+, and triggers downstream calcium signaling (15-18).

These processes are important for maturation of the vasculature as deletion of Piezo1 impaired vascular development in mice and also blocked sprouting angiogenesis in response to shear stress (16).However, endothelial Piezo1 mediates pathological responses to pressue and is involved in atherosclerosis progression and inflammatory signaling (19).Like Piezo1, the endothelial cell-expressed, calcium-permeable transient receptor potential vanilloid subfamily 4 (TRPV4) channel is expressed in various tissues and cells that are also pressure- sensitive (e.g., vascular endothelium, urinary bladder, and airway epithelium) (9,20-22). TRPV4 has been linked to several physiological functions including epithelial ciliary activity, regulation of blood flow, and shear-induced vasodilation and angiogenesis, and pathological processes that involve endothelial dysfunction and actin disruption (4,23-25). Blockade of TRPV4 channels protects against pulmonary edema and hyperpermeability induced by high pressure (10). Experimentally it has been shown that TRPV4 channels are activated by high shear stress, membrane stretching, and hypotonic cell swelling although they do not have true mechanoreceptor properties (4,7,26- 31). Therefore, how TRPV4 in endothelial cells senses physical force is not fully understood.It was demonstrated previously that blood flow-mediated shear stress activates phospholipase A2 (PLA2) generating 5′,6′-epoxyeicosatrienoic acid (5′,6′-EET) from arachidonic acid (6,28). Importantly, 5′,6′-EET has the ability to activate TRPV4.However, how shear stress activates PLA2 in endothelial cells is unknown.We recently observed that stimulation of Piezo1 in pancreatic acinar cells is responsible for pressure-induced pancreatitis (32) and is linked to TRPV4 (33). Therefore, we postulated that Piezo1 signaling coupled to TRPV4 activation may also account for the effects of shear stress on endothelialcells. Here we demonstrate that high shear stress activates Piezo1 and causes an initial increase in [Ca2+]i that triggers activation of TRPV4 in human endothelial cells (HUVECs) and HEK293T cells expressing both Piezo1 and TRPV4. Activation of TRPV4 causes a sustained [Ca2+]i elevation leading to loss of endothelial cell contacts, actin disruption, and endothelial cell monocyte adhesion.

Results
Fluid shear stress-induced [Ca2 +]i overload is force and time dependentShear stress is a physiological activator of mechanical ion channels in endothelial cells. In endothelial cells, shear stress regulates levels of intracellular calcium ([Ca2+]i) and downstream calcium signaling (24,34- 36). We evaluated the magnitude and duration of shear stress forces that affected [Ca2+]i in human umbilical vein endothelial cells (HUVECs) by applying shear stresses at physiological level ( 5 dyne/cm2) and pathological levels (37,38). Shear stresses of 4 and 12 dyne/cm2 applied for 1 min increased peak [Ca2+]i (Fig. 1A, and B). Applying a force of 12 dyne/cm2 for 1 min caused a sustained elevation in [Ca2+]i (intensity calculated at 8 min after initiation of force) but the same force applied for a shorter time (12 dyne/cm2 for 5 seconds) or lower shear stress (4 dyne/cm2) for 1 min elicited only a transient [Ca2+]i rise and did not produce prolonged elevation in [Ca2+]i (Fig. 1A, B and C).Endothelial cells express the mechanically sensitive, calcium-permeable ion channel, Piezo1(14,17). As an initial step in evaluating its role, we utilized the Piezo1 agonist, Yoda1. Yoda1 (2 M and 5 M), in a dose-dependent manner, increased peak [Ca2+]i, and caused sustained [Ca2+]i elevations (fluorescence intensity calculated at 8 min after Yoda1 application) (Fig. 1D, E and F). Thus, the level of [Ca2+]i produced by Piezo1 activation in HUVECs was dependent upon the Yoda1 concentration (Fig. 1D, E and F). To determine if Piezo1 was responsible for shear stress-induced calcium influx, we used the mechanoreceptor blocker, GsMTx4 (39). GsMTx4 (10 M) completely inhibited the shear stress (12 dyne/cm2)-induced elevation in [Ca2+]i (Fig 1G, H and I).

We observed that a higher dose of Yoda1 (10 M) or GsMTx4 (10 M) applied for up to 11 minutes did not affect the cell viability as all cells treated with Yoda1 or GsMTx4 responded to the calcium ionophore, ionomycin (1 M) (Sup-Fig. 1A, B, C and D).TRPV4 is responsible for the Piezo1-induced sustained [Ca2+]i elevation in HUVECs Although Piezo1 directly senses mechanical force (18), its fast inactivation kinetics and low single channel conductance (15), render it unlikely to be directly responsible for the sustained elevation in[Ca2+]i seen with higher shear forces. It is notable that endothelial cells also express another calcium- permeable ion channel – TRPV4 (4,35). Even though cells expressing TRPV4 exhibit mechanosensitivity, direct channel activation by mechanical force has not been demonstrated (9,27,28). Therefore, the ability of shear stress to activate TRPV4 channels seems to be indirect. To evaluate the contribution of TRPV4 to sense shear force, we tested 1 M HC067047 (HC067), a concentration that has been reported to completely block TRPV4 channel activity (21).HC067 slightly reduced the initial rise in [Ca2+]i produced by shear force applied at 12 dyne/cm2 for 1 min but completely blocked the sustained calcium elevation (Fig. 2A, B and C). This observation demonstrates that activation of the TRPV4 channel is responsible for the secondary, sustained elevation in [Ca2+]i produced by shear force. Addtionally, HC067 (1 M) completely blocked the Yoda1-induced sustained elevation in [Ca2+]i without affecting the initial rise in [Ca2+]i confirming that the Yoda1- and shear stress-induced secondary [Ca2+]i phase is due to activation of TRPV4 and the initial transient [Ca2+]i rise occurs through activation of Piezo1 (Fig. 2D, E and F).

To determine if selective activation of TRPV4 channels can reproduce the sustained [Ca2+]i elevation, we tested the effects of theTRPV4 agonist, GSK1016790A (GSK101) and the endogenous TRPV4 agonist 5′,6′-epoxyeicosatrienoic acid (5,6 – EET). Both GSK101 (50 nM) and 5,6 -EET (5 M)produced sustained [Ca2+]i elevations in HUVECs (Fig. 2G, H and I) however, the kinetics of the [Ca2+]i elevations were somewhat different. GSK101 caused a more rapid rise and subsequent decline in [Ca2+]i rise than 5, 6-EET. A detailed study of the gating mechanisms, binding affinity and half-lives of GSK101 and 5, 6-EET and their dose-dependent effects on TRPV4 activation will be needed to fully explain these changes. Along these lines, we observed that a lower concentration of 5, 6-EET reduced both the maximum and sustained [Ca2+]i elevations in HUVECs (Sup-Fig. 2A, B and C).Intracellular signals including PLA2 have been shown to activate TRPV4 (6), and we and others have previously reported that shear stress can increase PLA2 activity (33,40). Therefore, to determine theintracellular process that is responsible for the effects of Piezo1 on TRPV4 channel opening, we applied PLA2 blockers and measured the effects of high shear stress and the selective Piezo1 agonist, Yoda1, on [Ca2+]i in HUVECs. Exposure of HUVECs to Yoda1 throughout the period of imaging or high shear stress (12 dyne/cm2) for 1 min induced a prolonged increase in [Ca2+]i (Fig. 3) raising the possibility that Piezo1 activation is coupled to TRPV4 channel opening.

Treatment with the cytoplasmic PLA2 blocker AACOCF3 (30 μM) (41) and secretory PLA2 blocker YM26734 (10 μM) (42) significantly inhibited the Yoda1- and shear stress-induced sustained elevations in [Ca2+]i (Fig. 3), indicating that Piezo1 regulates PLA2 activity, which is responsible for the subsequent activation of TRPV4.Additionally, we demonstrated that the TRPV4 antagonist, HC067 blocked the 5, 6-EET-mediated [Ca2+]i elevation in HUVECs confirming that 5,6-EET is the endogenous activator of TRPV4 channel (Sup- Fig. 2D, E and F). Consistent with the idea that TRPV4 is activated by PLA2-generated signaling molecules, we found that the cocktail of PLA2 blockers AACOCF3 (30 μM) and YM26734 (10 μM) did not affect the 5, 6-EET- and GSK101-stimulated elevation in [Ca2+]i (Sup-Fig. 2G, H, I and J).Piezo1 is required for shear stress-induced TRPV4 activation in HEK293T cellsHaving demonstrated that TRPV4 is responsible for the Piezo1-induced sustained [Ca2+]i elevation in HUVECs, we next established a cell system in which the effects of Piezo1 and TRPV4 could be evaluated independently. Here we used HEK293T cells in which endogenous Piezo1 was deleted (43). We then induced transient expression of Piezo1, TRPV4 and Piezo1+TRPV4. Except for nontransfected cells, tdTomato cDNA was co-transfected with other genes to mark the positively transfected cells for calcium imaging. We observed that ~98% of tdTomato- positive cells responded to respective ion channel agonists indicating high co-transfection efficiency. As expected, nontransfected cells did not respond to Yoda1 or shear stress (12 dyne/cm2 for 1 min), and cells expressing TRPV4 responded to GSK101 (100 nM), but not to Yoda1 (5 µM) (Figure 4A, B and C).

In cells expressing Piezo1, Yoda1 produced asignificant but transient [Ca2+]i elevation. However, in cells expressing both Piezo1 and TRPV4, Yoda1 produced brisk and sustained [Ca2+]i elevations; the latter was completely blocked by the TRPV4 antagonist HC067 (Figure 4D, E and F). Shear stressproduced effects similar to Yoda1 on HEK293T cells expressing Piezo1, TRPV4 and Piezo1+TRPV4 (Figure 5). These results confirm that the initial transient increase in [Ca2+]i induced by Yoda1 and shear stress is caused by activation of Piezo1 and the secondary sustained phase of [Ca2+]i elevation resulted from activation of TRPV4. In approximately 10% of non- transfected and TRPV4-expressing cells, shear stress produced a transient (30 sec) spike in [Ca2+]i raising the possibility that other mechanically-sensitive ion channels may exist in HEK293T cells.Piezo1-induced adherens junction (AJ) disruption is the consequence of TRPV4 activationAJs consist of α-catenin, β-catenin, and p120-catenin and the transmembrane adhesive protein VE-cadherin (11,44). Activation of Piezo1 disrupts vascular AJs and increases vascular permeability (11). To determine if this disruption occurs through Piezo1 on vascular endothelial cells, we treated monolayer HUVEC cells with Yoda1 (2 M) for 30 min and observed a reduction in VE-cadherin expression at AJs (Fig. 6A). The overall apparent width of VE-cadherin at AJs was decreased significantly with Yoda1 (2 M) (Fig. 6C). A higher concentration of Yoda1 (5 M) decreased the accumulation of VE-cadherin and disrupted HUVEC integrity (Fig. 6A and B).

We proposed that these changes were due to Piezo1- triggered TRPV4 activation causing secondary calcium overload. To determine if the effect of Yoda1 on VE-cadherins was due to activation of TRPV4, we evaluated the action of HC067 (1 M). Treatment with HC067 stabilized the VE-cadherin at AJs and also protected the integrity of HUVECs in monolayer culture (Fig. 6A and B). These findings indicate that Yoda1-induced loss of AJs is through the combined actions of Piezo1 and TRPV4. We observed that a high concentration of Yoda1 (10 M) caused cell retraction and produced paracellular gaps in monolayer cultures (Fig. 6F and Movie 1).Paracellular gaps were the consequence of the reduction in the cell surface area. Cellular disruption due to Yoda1 was absent when the TRPV4 blocker HC067 was added to the media (Fig. 6F and Movie 1).Subjecting HUVEC monolayers to 12 dyne/cm2 for 10 min reduced VE-cadherin at AJs and decreased the apparent width of individual cells.Knowing that through Piezo1, shear stress triggers TRPV4 activation which is responsible for producing high levels of [Ca2+]i , we postulated that blocking TRPV4 would protect against the loss of VE-cadherin caused by Yoda1. Thus, if TRPV4 was responsible forthe sustained [Ca2+]i elevation that causes the loss of VE-cadherin, then blocking TRPV4 would be expected to protect against disruption of AJs. We observed that HC067 blocked shear stress-mediated loss of VE-cadherin at AJs (Fig. 6D) and preserved the apparent width of VE-cadherin (Fig. 6E).Inhibition of Piezo1 channels protected against shear stress-induced actin disorganization Cytoskeleton remodeling in response to the physiological levels of shear stress is necessary for endothelial cell migration and maintaining vascular integrity (1,45).

However, shear stress generated under conditions of high vascular pressure or turbulence has adverse effects on the cytoskeleton which can lead to increased endothelial cell stiffness, vascular permeability, and transmigration of leukocytes (1,11,46,47). We analyzed F-actin fiber distribution using F-actin plot profiling and measured the F-actin orientation and intensity at cytosolic and peripheral regions of the cell (Fig. 7A, B, C and D). We observed that high shear stress (25 dyne/cm2 for 10 min) disrupted the orientation of F-actin in HUVECs in contrast to lower shear force (4 dyne/cm2 for 10 min) (Fig. 7 A and B). High shear stress triggered the formation of F-actin bundles indicative of fiber polymerization (Fig. 7 A and B). The F-actin intensity frequency distribution predicted that high shear stress caused F-actin fibers to translocate from the peri- nuclear region of the cell to the periphery where a high-density of uneven clusters appeared (Fig. 7 A, B, C and D). The uniform thickness of F-actin fibers generally observed under low shear stress conditions was lost and extensive polymerization of thick F-actin bundles appeared at the periphery of cells subjected to high shear stress (Fig. 7 A, B, C and D). These effects of high shear forces were prevented in cells treated with GsMTx4 confirming that high shear stress- mediated F-actin disorientation required Piezo1 channel activation (Fig. 7).Piezo1 mediated F-actin disruption depends on TRPV4 activationTo determine if activation of Piezo1 can affect the F- actin disorganization and might be the mechanism through which shear stress causes cytoskeletal remodeling, we applied the Piezo1 agonist, Yoda1 (10M) for 10 min to HUVECs.

Without Yoda1 administration (control), the F-actin fibers were parallel in orientation and evenly distributed.Application of Yoda1 (10 M) caused a drastic change in HUVEC morphology with apparent cell contraction and reduction in cell surface area, complete loss of F-actin fiber distribution, and accumulation of high- density clusters of F-actin fibers at the periphery of cells and loss of F-actin fibers in the cytosolic region of the cells (Fig. 8). These Yoda1-induced changes were significantly reduced by the TRPV4 blocker, HC067 (1M), confirming that Piezo1 mediated F- actin disorganization required TRPV4 activation (Fig. 8). We determined that arachidonic acid (10 M), an endogenous mediator of TRPV4 activation, triggered the same pattern of F-actin disorganization and gathering of high-density clusters of F-actin fibers in the periphery of HUVECs all of which were inhibited by HC067 (Fig. 8). These findings signify that TRPV4 activation can cause cytoskeleton damage, and that shear stress-triggered remodeling of F-actin and disruption of F-actin fibers results from the combined actions of Piezo1 and TRPV4.Blockade of TRPV4 inhibits Piezo1-mediated monocyte adhesion to endothelial monolayers Disruption of normal cell-to-cell contacts in the vascular endothelium accompanies excessive shear force and leads to an inflammatory response characterized by monocyte adhesion (3,36). Having demonstrated that shear force activates Piezo1 which can disrupt AJs and form paracellular gaps in confluent monolayers, we next evaluated the effects of Piezo1 on endothelial cell activation and adhesion protein expression, which are two of the early processes in atherosclerosis (48). Exposing endothelial cells to Yoda1 (1 M) for 10 h increased expression of the adhesion protein VCAM1 and stimulated the attachment of monocytes (THP-1 cells) (Fig. 9). THP-1 attachment was prevented by the TRPV4 antagonist HC067 (Fig. 9A and B). These findings indicate that the adverse effects of Piezo1- induced changes in endothelial cell adhesion led to the attraction of inflammatory cells and were mediated by TRPV4.

Discussion
Calcium signaling in endothelial cells is a highly regulated process (36). Under physiological conditions, the amplitude and frequency of [Ca2+]i oscillations in endothelial cells maintaincellular integrity, but stimulation by inflammatorymediators such as histamine, bradykinin and thrombin increases intracellular calcium up to 10 fold (36).High sustained [Ca2+]i, leading to calcium overload, alters normal calcium signaling pathways and causes cytoskeletal disorganization and AJs disassembly.Together these processes facilitate transendothelial migration of leukocytes.High blood pressure and shear stress also have been associated with endothelial dysfunction (1,3,13,36,49). High blood pressure or shear stress-mediated calcium overload contributes to cytoskeletal disorganization, AJs disassembly and leukocyte transendothelial migration (2,10,11,17,34,47). However, the severity of damage is endothelium-dependent, as the sensitivity to shear stress differs between the arterial and venous systems (50). Endothelial cells sense pressure and shear forces through calcium permeable mechanosensitive ion channels that convey extracelluar signals to maintain cellular integrity. The extent of calcium influx depends upon the strength of blood flow shear stress (51) and the number of mechanosensitive ion channels in the particular endothelium. We demonstrated in HUVECs that prolonged high shear stress produced a sustained elevation in [Ca2+]i in contrast to low levels of shear stress or transient high shear stress.

HUVECs are typical of other endothelial cells and express two types of mechanosensitive ion channels, Piezo1 and TRPV4, which have been implicated in vascular pathophysiological conditions (10,11,17,52,53).Either Piezo1 or TRPV4 may contribute to abnormallyhigh [Ca2+]i and may even initiate pathological events in endothelial cells (53-55).Piezo1 has a low single-channel conductance of approximately 22 pS and is a fast inactivating channel (15). Therefore, it seemed unlikely that Piezo1 alone could produce the prolonged elevation in [Ca2+]i to induce a calcium overload state necessary to disrupt endothelial cell integrity. This led us to search for another calcium signaling pathway or calcium permeable ion channel that might be involved.TRPV4 was a likely candidate due to its slow inactivation kinetics and high single-channel conductance of approximately 60 pS (56). However, unlike Piezo1, TRPV4 does not appear to possess direct mechanosensing properties (7,27-29,40).Although under certain experimental conditions, TRPV4 has been shown to become activated by physical forces, such as shear stress, osmotic pressure, and mechanical stretching (4,23,26,27,57,58), the mechanical gating of TRPV4 has not been described. In whole cell systems such as Xenopus oocytes transfected with TRPV4 and TRPV4-expressing endothelial cells, hypotonicity and mechanical forces increased TRPV4 activity (4,34,58). However, in cell- free systems (e.g., inside-out membrane patches or lipid bilayers) similar responses have not been studied.In analogous experiments, in cells TRPV4 was sensitive to to changes in temperature but the same sensitivity was not seen in cell-detached, inside-out patches (56,59). These findings suggest that mechano- and temperature-sensing may not be inherent properties of TRPV4 itself.The mechanosensitive nature of the TRPV4 channel has been controversial.

Urothelial cells which express endogenous TPPV4 and Xenopus oocytes transfected with TRPV4, but not TRPV4-expressing HEK293T cells were activated by membrane stretch (26,27,31,58). In the absence of confounding factors, if TRPV4 directly senses mechanical force, one would expect all TRPV4-expressing cells to respond to mechanical stimuli. Our observation that deletion of Piezo1 in TRPV4-expressing HEK293T cells eliminated their ability to respond to shear force supports the concept that Piezo1 but not TRPV4 is mechanosensitive and that TRPV4 activation is downstream to Piezo1 activation. It is likely that the level of Piezo1 expression and the number of Piezo1 channel openings affect the extent of the TRPV4 channel opening and may explain, at least in part, the heterogeneous response of TRPV4-expressing cells to mechanical forces.During shear stress, TRPV4 is activated by 5,6-EET, an endogenous ligand derived from arachidonic acid through the activation of PLA2 (28,33).Recently, we discovered that high pressure activated Piezo1, PLA2, and TRPV4 in pancreatic acinar cells producing a sustained [Ca2+]i elevation. However, in acinar cells from TRPV4 knockout mice, high pressure caused only a transient elevation in [Ca2+]i (33).HUVECs sense mechanical force in a similar manner.In HUVECs, shear stress stimulates TRPV4 channel opening through Piezo1-stimulated activation of PLA2. A cocktail of PLA2 blockers (YM26734 and AACOCF3) significantly inhibited the sustained [Ca2+]i elevation produced with Yoda1 and shear stress, while the TRPV4 antagonist HC067 completely blocked the sustained calcium influx suggesting other signaling pathways might be operating along with PLA2 to activate TRPV4. Binding of calcium ion to PLA2 accelerates enzyme activity, which initiates 5,6 – EET production and TRPV4 channel activation.

It appears that a threshold level of peak [Ca2+]i was necessary to induce PLA2 activation. It is likely that peak [Ca2+]i is controlled by the number of Piezo1 channel openings. It could be that brief shear stress activated only a subset of Piezo1 channels resulting in submaximal [Ca2+]i elevation which was insufficient toactivate PLA2 in endothelial cells. In contrast, Yoda1 which would be expected to activate most Piezo1 channels, mimicked the effects of prolonged high shear stress-mediated [Ca2+]i elevation. Like HUVECs, Yoda1 and high shear stress caused sustained [Ca2+]i elevation in HEK293T cells expressing both Piezo1 and TRPV4. Cells expressing TRPV4 alone were nonresponsive to Yoda1 and high shear stress, and cells expressing only Piezo1 exhibited only transient calcium elevations confirming that Piezo1 and TRPV4 coupling during high mechanical force is a generalized process.Basal endothelial calcium levels control vascular permeability and contraction. Notably, basal calcium levels are altered in hypertension and high shear stress, which leads to disruption of the cell-cell junctional protein VE-cadherin and loss of endothelial barrier function. Impaired endothelial barrier function contributes to atherosclerosis which is a major cause of mortality among patients with hypertension. It was recently reported that blocking Piezo1 or TRPV4 prevented hypertension-associated vascular hyperpermeability but the underlying mechanisms or possible interactions were not uncovered (10,11).Nevertheless, our findings demonstrate how TRPV4 may contribute to micro-endothelial permeability (10,34).

It has been shown that TRPV4 knockout mice are protected from lung vascular hyperpermeability in response to high pulmonary venous pressure (PVP) (20,57,60,61). Similarly, pharmacological blockade with the TRPV4 antagonist GSK2193874 also protected against pulmonary venous pressure (PVP)- induced permeability of the lung (10). It was recently reported that Piezo1 senses high vascular pressures at the lung endothelial surface and is responsible for vascular hyperpermeability and pulmonary edema(11). Thus, it appears that the high PVP-mediated vascular hyperpermeability is due to both Piezo1 and TRPV4. Our results demonstrated that Piezo1 activation caused the loss of VE-cadherin at the cell- cell junction and disrupted endothelial barrier integrity which were prevented by TRPV4 blockade. Moreover, TRPV4 was responsible for Piezo1- initiated cell retraction and paracellular gap formation in monolayer cultures. Thus, the combined actions of both Piezo1 and TRPV4 may contribute to the endothelial vascular barrier dysfunction inhypertension. Shear stress also accompanies increased viscosity of blood which is a risk factor for deep vein thrombosis (23,62,63). It will be interesting todetermine if targeting Piezo1 or TRPV4 channels can improve either of these clinical conditions.Fluid shear stress caused by blood flow is a major determinant of vascular remodeling and arterial tone and can lead to the development of atherosclerosis (36,47). High shear stress-mediated calcium signaling activates endothelial cells, cytoskeleton remodeling, and production of inflammatory cytokines and chemokines which facilitate leukocyte rolling, adhesion, and transendothelial migration (36).

Our results suggest that all of these effects can be initiated by Piezo1 activation. Therefore, loss of endothelial barrier integrity and monocyte adhesion which are integral to atherosclerosis may be directly related to Piezo1 (19,55). Although our findings provide insight into the relationship between Piezo1 activation and deleterious effects on endothelial cells, it is important to note that development of atherosclerosis is a chronic process and is best studied in animals. Therefore, the relationship between Piezo1 and TRPV4 in the endothelium and initiation and perpetuation of atherosclerosis is more complicated than what can be studied in vitro. Nevertheless, the effects of Piezo1 on endothelial cell integrity may be an early step in the disease.Piezo1 initiated the remodeling in our in vitro system. It is possible that a similar mechanism occurs under conditions of elevated shear stress in vivo. Due to the rate of blood flow, the endothelium in the arterial system is exposed to higher shear stress forces compared to the venous endothelium. In addition, transient or pulsatile shear stress is beneficial in the arterial system (2). In our experiments, using cells of venous origin, high shear stress of 25 dyne/cm2 for minutes at a time caused adverse effects. Regional distribution of both Piezo1 and TRPV4 throughout the vascular endothelium has not been extensively evaluated. It is possible that deleterious effects of high pressure do not occur in some vascular beds due to the absence of coexpression of Piezo1 and TRPV4 in the same cell. Our findings suggest that cells lacking either Piezo1 or TRPV4 would be protected from high shear stress-induced changes in cytoskeleton, cell retraction, and inflammatory cell adhesion.

Similarly, pharmacological blockade of either Piezo1 or TRPV4 would be expected to prevent the deleterious effects of shear stress in endothelium. However, identification and functional chacterization of both Piezo1 and TRPV4 throughout the vascular endothelium would be needed before considering therapeutics forcardiovascular diseases directed against these ion channels.The deleterious effects of shear stress in endothelial cells are secondary to sustained Ca2+ influx through TRPV4 channels. Therefore, the extent of Ca2+ influx could be influenced by several factors including the strength and duration of mechanical force, the level of PLA2 activity, and TRPV4 abundance. Our findings suggest that Piezo1 or TRPV4 alone is not sufficient to transduce mechanical force into pathological events. We have previously demonstrated that coupling of Piezo1 with TRPV4 is responsible for the effects of high pressure in pancreatic acinar cells (33). If functional coupling between Piezo1-TRPV4 is a generalized process in which TRPV4 translates the mechanical force sensed by Piezo1 into pathological events, then other organ systems like urinary bladder and bone tissue where Piezo1and TRPV4 are coexpressed (21,64-67), may also be amenable to targeting Piezo1 or TRPV4 to prevent adverse effects of pressure or shear stress.Cell Culture and expression of Piezo1 and TRPV4 Primary human umbilical vein endothelial cells (HUVECs) (CC-2519) were obtained from Lonza. Cells were cultured with Endothelial Cell Growth Media (Cell Applications; 211-500) in a humidified incubator at 37°C and 5% CO2 (68). Cells were fed every two days and were not allowed to grow to confluence unless required for a specific experiment.

Cells were used for experiments between passage numbers 2 to 5. HUVECs were passaged with 0.025% Trypsin/EDTA solution (TE, #R001100, Thermo Fischer Scientific). THP-1 cells, a monocyte cell line, were obtained from ATCC; TIB-202 (69). The suspension culture of THP-1 was grown in RPMI 1640+ sodium pyruvate (1 mM) + HEPES (10 mM) + glucose (10 mM) + 10% FBS + 0.05 mM beta- mercaptoethanol in a humidified incubator at 37°C and 5% CO2. Like HUVECs, THP-1 cells were fed every two days and during culture, the cell number was not allowed to exceed 1 x 106. Primocin (InvivoGen) at a concentration of 100 g/mL was added to cell culture media.Piezo1 deleted HEK293T cells were transiently transfected with pcDNA3.1 plasmids containing mouse Piezo1 or human TRPV4 (15,22) alone or together using Lipofectamine 3000 (Invitrogen) according to the manufacturer’s protocol.A plasmid containing tdTomato was co-transfected with targeted cDNA at a 1:8 molar ratio for the selection of positively transfected cells. Calcium imaging in the transfected cells was performed 36– 48 h post-transfection.HUVECs were plated on a thin layered Matrigel coated plate for 1 h to allow cells to attach. The cells were then loaded with Calcium 6-QF (Molecular Devices) in a Minimum Essential Medium:Hanks’ balanced salt solution (MEM:HBSS; 1:1) for 30 min at 37°C in a CO2 incubator (32). The cells were washed gently with HBSS buffer with 2 mM Ca2+.

The cells were imaged by using a Zeiss Axio observer Z1 with a 20x objective and images were captured at 400 ms intervals. HBSS buffer with 2 mM Ca2+ was used during imaging. The intracellular calcium elevation of individual cells was analyzed with MetaMorph software (Molecular Devices). Cells overloaded with dye or only faintly fluorescent were excluded from analysis. The chemicals used in calcium imaging experiments included: Yoda1 (Tocris; 5586), GsMTx4 (Abcam; ab141871), 5, 6- eicosatrienoic acid (Santa Cruz Biotechnology; sc-221066), arachidonic acid (Sigma; A3611), HC067047 (Tocris; 4100), GSK1016790A (Sigma; G0798), AACOCF3 (Tocris; 1462), YM26734 ( Tocris; 2522).Monocyte-endothelial cell adhesion assayTo evaluate Yoda1-induced monocyte (THP-1 cells) adhesion to HUVECs, confluent HUVEC monolayers were pretreated with DMSO (vehicle control), Yoda1 (1 M), Yoda1 (1 M) + HC067 (1M), or TNF-α (10 ng/mL), (CELL BIOLAB. INC;Catalog; CBA210) for up to 10 hours in a humidified incubator at 37°C and 5% CO2. After treatment, the media were removed and THP-1 cells were added to HUVEC monolayers for 1 hour at 37°C to allow attachment (70). Before THP-1 cells were added to HUVEC monolayers, the THP-1 cells were harvested and prepared in a cell suspension at 1.0 x 106 cells/mL in serum free media and loaded with LeukoTracker (a live cell imaging dye) from CELL BIOLAB. INC; CBA210) as per manufacturer instructions. The non- attached THP-1 cells were cleared by gently washing three times with serum-free media. The remaining adherent THP-1 cells loaded with LeukoTracker dye were imaged using a Zeiss Axio observer Z1 with a 4x objective. Adherent cells were counted using FIJI software.

The average number of THP-1 cells werecalculated from five image frames. The data presented are representative of three independent experiments.HUVEC cells were washed with PBS (pH 7.4) and then fixed with 4% PFA for 10 min at room temperature. The fixed cells were treated with 0.1% Triton X-100 in PBS (pH 7.4) for 15 min at room temperature then blocked with 1% bovine serum albumin (BSA) for 1 h at room temperature. Cells were incubated with antibodies against VE-cadherin (Santa Cruz Biotechnology; sc9989) overnight at 2- 8°C or antibodies against VCAM1 (abcam; ab134047) for 1 h at room temperature (71). Secondary goat anti- rabbit or secondary goat anti-mouse IgG Alexa Fluor 594 (Jackson ImmunoResearch) was used after each step for 1 h at room temperature. Immunostaining of F-actin was performed on fixed cells using Alexa Flour 488TM Phalloidin (Thermo Fisher scientific; A12379) for 1 h at room temperature. Cells were then washed three times with PBS for 10 min and incubated with Nunc Blue (Thermo Fisher scientific; R37606) and then mounted onto microscope slides with ProLong® Gold antifade reagent (Invitrogen). Images of immunostained cells were taken with a Zeiss Axio observer Z1 with a 40x objective or a Leica SP5 inverted confocal microscope with a 40x oil objective. The images were processed initially with MetaMorph software (Molecular Devices) or Leica LAS AF lite software and then the intensity of F-actin and width of VE-cadherin were measured with ImageJ software (11). To measure the F-actin fiber distribution we used the plot profile from the analysis section of the ImageJ software (25). A line was drawn at the widest part of the cell perpendicular to the F- actin orientation across which the intensity of phalloidin 488 was measured.

The length of the line drawn perpendicular to F-actin orientation was calculated by converting the length from pixel to µm (1 pixel = 0.1570 µm) according the Cool SNAP ES2 camera (Photometrics) specification with a 40x objective. Laminar flow shear stress was generated using parallel-plate fluid flow chambers fromIbidi, GmbH. Two types of flow chambers were used in the experiments. A μ-Slide I 0.4 Luer flow chamber was used to achieve 12 dyne/cm2 or lower shear stress. A μ-Slide I 0.2 Luer flow chamber was used for forces of 25 dyne/cm2 (17,33). The constant fluid flow rate with shear stress (τ) was determined as follows: τ = η ᵡ104.7 φ for μ-Slide I 0.4 Luer and τ = η ᵡ 330.4 φ forμ-Slide I 0.2 Luer, where η = viscosity of the medium and φ = flow rate (according to the manufacturer’s instructions, Ibidi).Results are expressed as Yoda1 mean ± SD. Mean differences between 2 groups were analyzed by 2- tailed Student’s t-test, and mean differences between multiple groups were analyzed by 1-way ANOVAwith Tukey’s multiple comparison post-test (GraphPad Prism 8). P values of less than 0.05 were considered significant and ‘ns’ represents non-significant.