2.1. Shear stress

coordinated changes in arterial diameter. Endothelial cells respond to vasodilatory stimuli by releasing diffusible mediators such as nitric oxide (NO) and prostacyclin (PGI2) and by initiating membrane hyperpolarization that spreads to surrounding smooth muscle cells via myoendothelial gap junctions (MEGJs) to inhibit contractility, a mechanism termed endothelium-dependent hyperpolarization (EDH) [1–3]. NO and PGI2 are local mediators that diffuse to surrounding smooth muscle cells to cause relaxation. Once initiated, EDH spreads to surrounding smooth muscle cells to affect relaxation but conduction of hyperpolarization longitudinally through the endothelial layer means that EDH also contributes to coordination of changes in blood flow in multiple arterial segments within a vascular bed [4]. Thus, the ability of a stimulus to engage diffusible mediators versus EDH determines whether it's effects on arterial diameter and thus blood flow, are restricted to the local area

Increases in endothelial intracellular Ca2+ concentration ([Ca2+]i) drive these vasodilator pathways; NO is synthesized from L-arginine by the Ca2+-calmodulin-dependent enzyme NO synthase (NOS) [3], PGI2 is generated by the actions of cyclooxygenase on arachidonic acid released by the actions of Ca2+-dependent phospholipase A2 on membrane phospholipids [5, 6], and opening of Ca2+-activated K+ (KCa) channels causes hyperpolarization [3, 7]. Global changes in endothelial [Ca2+]i have been widely studied [8, 9], but development of new technologies such as high-speed, high-resolution confocal Ca2+ imaging and generation of transgenic mice expressing genetically encoded Ca2+ indicators has allowed resolution of a wide range of transient Ca2+ events within endothelial cells of intact arteries to provide a growing body of support for the concept of stimulus-specific engagement of effectors underpinned by spatially and temporally discrete Ca2+ signaling patterns that occur independently of changes in bulk endothelial

Pulsars [10] and wavelets [11] are spontaneous, short-lived, (<0.03 s duration) spatially fixed Ca2+ events originating from distinct clusters of inositol 1,4,5-trisphosphate (InsP3) receptors on the membrane of endoplasmic reticulum (ER). First identified in mouse mesenteric artery and hamster skeletal muscle arteriolar endothelial cells, these events predominantly occur close to endothelial projections that abut or form MEGJs with smooth muscle cells [10, 11] and exert a basal vasodilator influence through activation of intermediate conductance (IKCa) Ca2+-activated K+ channels. Their dependence on InsP3 provides a mechanism by which pulsars are linked to and regulated by G protein-coupled receptor (GPCR) signaling. Elevation of InsP3 by endothelium-dependent vasodilators [10] or by flux of InsP3 from smooth muscle cells following stimulation of α1-adrenoceptors [11] increases pulsar size and/or frequency through recruitment of new sites and a reduction in the interval between pulsars at a given site. In porcine coronary arteries, InsP3-dependent Ca2+ events similar to pulsars propagate into longer lasting Ca2+ waves (>8 s duration) facilitated by the longitudinal arrangement of ER/InsP3 receptors to promote directional Ca2+-induced Ca2+ release along the endothelial cell

Sparklets are generated by spatially restricted Ca2+ influx through members of the transient receptor potential (TRP) ion channel family [14, 15]. Sparklets were first identified in mouse mesenteric arteries under experimental conditions in which InsP3-mediated pulsars were

axis and are associated with activation of both NOS and KCa channels [12].

or can impact blood flow at the level of the vascular bed.

[Ca2+]i [10–13].

44 Calcium and Signal Transduction

In vivo, endothelial sensing of laminar shear stress, the tangential frictional force exerted by blood flowing across the cell surface, plays a dominant role in acute modulation of vascular tone and therefore, tissue perfusion [19–21]. In the majority of resistance arteries, increases in blood flow stimulate endothelium-dependent relaxation of surrounding smooth muscle cells and increase arterial diameter, a response termed flow-mediated dilatation. Flow also influences gene expression and structural remodeling with areas of disturbed flow and reduced shear stress is associated with development of atherosclerotic plaques [22]. Measurement of acute responses to increases in shear stress is the most widely used clinical index of endothelial function and vascular health with attenuation of flow-induced dilation associated with increased risk of cardiovascular diseases [23, 24]. Indeed, reductions in shear stress are a likely mechanism by which endothelial function is altered with inactivity, an effect which can be overcome by exercise interventions [25, 26].

In animals and humans, acute shear stress-induced vasodilation can be mediated by both NO and EDH [27–31]. Although endothelial cells express both SKCa and IKCa channels, data from isolated arteries indicate that it is SKCa channels that play a predominate role in mediating the EDH component of this response. Deletion of SKCa but not IKCa channels impaired both NO and EDH-mediated dilation to shear stress stimulation in mouse isolated carotid arteries [32]. In rat isolated perfused mesenteric beds, shear stress-induced modulation of sympathetic vasoconstriction was prevented by both the NOS inhibitor L-NG-nitroarginine methyl ester (L-NAME) and apamin, a selective blocker of SKCa channels, but not by the IKCa channel inhibitor TRAM-34 [33]. Similarly, shear stress-evoked dilation of mouse isolated coronary arteries was inhibited by apamin [34] and L-NAME [35].

Mechanotransduction, the conversion of increases in shear stress into changes in arterial diameter, is reliant upon rises in endothelial [Ca2+]i mediated by Ca2+ entry. In vitro studies have identified multiple candidates as potential endothelial mechanosensors including integrins [36], tyrosine kinase receptors [37], intercellular junction proteins [38], and P2X4 receptors which are cation channels activated by adenosine triphosphate (ATP) [39]. Work with transgenic mice has implicated GPR68, a proton-sensing rhodopsin-like GPCR [40], inwardly rectifying K<sup>+</sup> channels [41] and PIEZO1, a Ca2+-permeable, non-selective cation channel [42, 43]. However, recently, it is the role of TRPV4 in endothelial responses to increases in shear stress that has received particular attention. This Ca2+ permeable channel can be directly activated by shear stress [34, 44] via membrane deformation or through a lever-like action involving cytoskeletal linkages to molecules embedded in the glycocalyx [45, 46], the layer of proteoglycans and glycoproteins that covers the luminal surface of the endothelium, or indirectly through upstream production of arachidonic acid metabolites [47]. Genetic deletion of TRPV4 results in blunted flow-mediated dilation of mouse carotid and mesenteric arteries [31, 47, 48] and pharmacological inhibition of these channels blocked flow-evoked increases in endothelial [Ca2+]i in isolated mouse mesenteric, human coronary, and rat carotid and gracilis arteries [31, 49–51]. In bovine coronary endothelial cells block of TRPV4 inhibited both shear stress-evoked increases in [Ca2+]i and activation of SKCa channels [34], indicating that there may be a direct link between TRPV4-mediated Ca2+ influx and SKCa channel activity. This idea is supported by the demonstration that in rat pulmonary arteries, vasodilation to the TRPV4 agonist GSK1016790A was mediated by activation of SKCa channels [52]. In the same vessels, and in mouse small pulmonary arteries, shear stress-stimulated TRPV4 activity was also linked to NO production [17] suggesting a further link between TRPV4 and NOS.

> within a signaling microdomain to selectively activate SKCa channels and NOS to elicit vasodilation (Figure 1). However, a number of questions remain to be addressed. Shear stress increases PGI2 production in bovine coronary and human umbilical vein endothelial cells [34, 61] and rabbit isolated femoral arteries [62], and hydrogen peroxide (H2O2) contributes to flow-mediated dilation in coronary arterioles from patients with heart disease [63] but the functional role of these factors in acute flow-mediated vasodilation has not fully been explored. A significant component of flow-induced dilation remained in isolated mesenteric arteries of mice lacking TRPV4 [31] which could indicate that, as suggested in earlier reports, Ca2+-independent processes may also contribute to this response [64] or the involvement of another route for Ca2+ influx. The possibility that flow-induced increases in endothelial cell [Ca2+]i are stimulated by localized release endothelium-derived paracrine mediators such as ATP, substance P or acetylcholine, first proposed over 30 years ago [65, 66], has recently received renewed support with the demonstration that endothelial organic cation transporters release acetylcholine in response to increases in shear stress in rat isolated carotid arteries [67]. The same study suggests that InsP3-mediated Ca2+ release from ER stores and Ca2+ entry through TRPC but not TRPV4 contributes to flow-induced endothelial Ca2+ signaling in these vessels. This finding highlights the fact that further work is required to elucidate the differential signaling networks underlying endothelial responses to acute increases in shear stress in

> Figure 1. Model of localized endothelial Ca2+ signaling evoked by increases in shear stress. Shear stress-evoked Ca2+ influx through TRPV4 channels on the luminal surface of endothelial cells leads to spatially-restricted Ca2+ sparklets

The Endothelium: The Vascular Information Exchange http://dx.doi.org/10.5772/intechopen.79897 47

within a signaling microdomain to selectively activate SKca channels and endothelial NOS (eNOS).

Many endogenous and exogenous chemicals bind to GPCRs leading to stimulation of EDH and production of NO, PGI2 and other diffusible mediators such as epoxyeicosatrienoic acids and H2O2, to cause vasodilation [1, 2, 68]. Measurements of bulk endothelial [Ca2+]i established

different arteries.

2.2. Agonists at endothelial GPCRs

Building on these findings, several lines of evidence now support the notion that acute increases in shear stress cause Ca2+ influx through TRPV4 channels to selectively activate both SKCa channels and NOS, and that this pathway is enabled by organization of TRPV4, NOS, SKCa channels and the caveolae scaffold protein caveolin-1 into microdomains within caveolae, flask-shaped structures on the endothelial cell surface rich in signaling proteins [34, 53, 54]. SKCa channels are localized to the luminal membrane of endothelial cells in rat mesenteric arteries [55] and SKCa channel protein was co-immunoprecipitated with caveolin-1 from endothelial cells of the same arteries and from porcine coronary arteries [56]. It is well established that endothelial NOS is localized to caveolae where it is negatively regulated through its interaction with caveolin-1 [57]. Increases in [Ca2+]i promote recruitment of Ca2+ calmodulin to displace caveolin-1 from NOS thereby activating it [53]. In bovine coronary and human microvascular endothelial cells, SKCa channels were co-localized with caveolin-1, NOS and TRPV4 channels within microdomains at the luminal endothelial cell surface [34, 57, 58]. Furthermore, in mesenteric arteries from mice lacking caveolin-1, endothelial TRPV4 channel activity was impaired indicating that a direct interaction between TRPV4 and caveolin-1 may be functionally important for Ca2+ entry in response to shear stress [57]. Caveolin-1 has been shown to initiate downstream signaling in response to increases in shear stress [59] leading to the suggestion that caveolae act as mechanosensors to elicit a cascade of events that promote vasodilation. In line with this proposal, shear stress-induced dilation is defective and endothelial SKCa current reduced in coronary and carotid arteries of mice lacking caveolin-1, an effect rescued by re-introduction of endothelial specific caveolin-1 [58, 60].

Together these findings, gathered using a range of approaches and from a number of different arteries, support an elegant model in which shear stress-evoked Ca2+ influx through TRPV4 channels on the luminal surface of endothelial cells leads to spatially-restricted Ca2+ sparklets

Figure 1. Model of localized endothelial Ca2+ signaling evoked by increases in shear stress. Shear stress-evoked Ca2+ influx through TRPV4 channels on the luminal surface of endothelial cells leads to spatially-restricted Ca2+ sparklets within a signaling microdomain to selectively activate SKca channels and endothelial NOS (eNOS).

within a signaling microdomain to selectively activate SKCa channels and NOS to elicit vasodilation (Figure 1). However, a number of questions remain to be addressed. Shear stress increases PGI2 production in bovine coronary and human umbilical vein endothelial cells [34, 61] and rabbit isolated femoral arteries [62], and hydrogen peroxide (H2O2) contributes to flow-mediated dilation in coronary arterioles from patients with heart disease [63] but the functional role of these factors in acute flow-mediated vasodilation has not fully been explored. A significant component of flow-induced dilation remained in isolated mesenteric arteries of mice lacking TRPV4 [31] which could indicate that, as suggested in earlier reports, Ca2+-independent processes may also contribute to this response [64] or the involvement of another route for Ca2+ influx. The possibility that flow-induced increases in endothelial cell [Ca2+]i are stimulated by localized release endothelium-derived paracrine mediators such as ATP, substance P or acetylcholine, first proposed over 30 years ago [65, 66], has recently received renewed support with the demonstration that endothelial organic cation transporters release acetylcholine in response to increases in shear stress in rat isolated carotid arteries [67]. The same study suggests that InsP3-mediated Ca2+ release from ER stores and Ca2+ entry through TRPC but not TRPV4 contributes to flow-induced endothelial Ca2+ signaling in these vessels. This finding highlights the fact that further work is required to elucidate the differential signaling networks underlying endothelial responses to acute increases in shear stress in different arteries.

#### 2.2. Agonists at endothelial GPCRs

integrins [36], tyrosine kinase receptors [37], intercellular junction proteins [38], and P2X4 receptors which are cation channels activated by adenosine triphosphate (ATP) [39]. Work with transgenic mice has implicated GPR68, a proton-sensing rhodopsin-like GPCR [40], inwardly rectifying K<sup>+</sup> channels [41] and PIEZO1, a Ca2+-permeable, non-selective cation channel [42, 43]. However, recently, it is the role of TRPV4 in endothelial responses to increases in shear stress that has received particular attention. This Ca2+ permeable channel can be directly activated by shear stress [34, 44] via membrane deformation or through a lever-like action involving cytoskeletal linkages to molecules embedded in the glycocalyx [45, 46], the layer of proteoglycans and glycoproteins that covers the luminal surface of the endothelium, or indirectly through upstream production of arachidonic acid metabolites [47]. Genetic deletion of TRPV4 results in blunted flow-mediated dilation of mouse carotid and mesenteric arteries [31, 47, 48] and pharmacological inhibition of these channels blocked flow-evoked increases in endothelial [Ca2+]i in isolated mouse mesenteric, human coronary, and rat carotid and gracilis arteries [31, 49–51]. In bovine coronary endothelial cells block of TRPV4 inhibited both shear stress-evoked increases in [Ca2+]i and activation of SKCa channels [34], indicating that there may be a direct link between TRPV4-mediated Ca2+ influx and SKCa channel activity. This idea is supported by the demonstration that in rat pulmonary arteries, vasodilation to the TRPV4 agonist GSK1016790A was mediated by activation of SKCa channels [52]. In the same vessels, and in mouse small pulmonary arteries, shear stress-stimulated TRPV4 activity was also

46 Calcium and Signal Transduction

linked to NO production [17] suggesting a further link between TRPV4 and NOS.

rescued by re-introduction of endothelial specific caveolin-1 [58, 60].

Building on these findings, several lines of evidence now support the notion that acute increases in shear stress cause Ca2+ influx through TRPV4 channels to selectively activate both SKCa channels and NOS, and that this pathway is enabled by organization of TRPV4, NOS, SKCa channels and the caveolae scaffold protein caveolin-1 into microdomains within caveolae, flask-shaped structures on the endothelial cell surface rich in signaling proteins [34, 53, 54]. SKCa channels are localized to the luminal membrane of endothelial cells in rat mesenteric arteries [55] and SKCa channel protein was co-immunoprecipitated with caveolin-1 from endothelial cells of the same arteries and from porcine coronary arteries [56]. It is well established that endothelial NOS is localized to caveolae where it is negatively regulated through its interaction with caveolin-1 [57]. Increases in [Ca2+]i promote recruitment of Ca2+ calmodulin to displace caveolin-1 from NOS thereby activating it [53]. In bovine coronary and human microvascular endothelial cells, SKCa channels were co-localized with caveolin-1, NOS and TRPV4 channels within microdomains at the luminal endothelial cell surface [34, 57, 58]. Furthermore, in mesenteric arteries from mice lacking caveolin-1, endothelial TRPV4 channel activity was impaired indicating that a direct interaction between TRPV4 and caveolin-1 may be functionally important for Ca2+ entry in response to shear stress [57]. Caveolin-1 has been shown to initiate downstream signaling in response to increases in shear stress [59] leading to the suggestion that caveolae act as mechanosensors to elicit a cascade of events that promote vasodilation. In line with this proposal, shear stress-induced dilation is defective and endothelial SKCa current reduced in coronary and carotid arteries of mice lacking caveolin-1, an effect

Together these findings, gathered using a range of approaches and from a number of different arteries, support an elegant model in which shear stress-evoked Ca2+ influx through TRPV4 channels on the luminal surface of endothelial cells leads to spatially-restricted Ca2+ sparklets Many endogenous and exogenous chemicals bind to GPCRs leading to stimulation of EDH and production of NO, PGI2 and other diffusible mediators such as epoxyeicosatrienoic acids and H2O2, to cause vasodilation [1, 2, 68]. Measurements of bulk endothelial [Ca2+]i established the role of InsP3-mediated Ca2+ release and subsequently store-operated Ca2+ entry (SOCE) in this process [9]. The mechanism underlying endothelial SOCE has been controversial but recent evidence supports a model in which Ca2+ store depletion allows spatial reorganization of Ca2+ sensor protein stromal interaction molecules (STIMs) so that they can aggregate into clusters that physically interact with Ca2+-selective Orai channels at the ER-plasma membrane junction [69–72]. TRPC and TRPV4 can also interact with STIMs [73] and studies of knock-out mice have provided evidence for a role for TRPC4 in acetylcholine-evoked SOCE in aortae [74] and for TRPV4 in SOCE in mesenteric [75] and carotid arteries [76]. A receptor-operated Ca2+ entry mechanism can also be mediated by DAG-induced activation of TRPC and TRPV channels. For example, in human umbilical vein endothelial cells, bradykinin stimulated both translocation of DAG-sensitive TRPC6 to the cell membrane and Ca2+ influx [77, 78]. Expression of mRNA for another ER Ca2+ release channel, the ryanodine receptor (RyR), has been detected in endothelial cells of human mesenteric arteries [79], and RyRs have been suggested to mediate Ca2+ oscillations in cultured bovine aortic and human umbilical vein endothelial cells [80] but to date, ryanodine has been shown to have no effect on endothelial Ca2+ signaling or vasodilation [12, 81]. There is significant variation in the reported contribution of EDH, NO and other mediators to agonist-evoked dilation, both in terms of differences between agonists and arteries. Thus, for the purposes of this chapter we will limit our discussion to three agents commonly used to stimulate endothelium-dependent vasodilation in experimental studies, acetylcholine, ATP and substance P.

regions associated with MEGJs in which ER membrane, InsP3 receptors, gap junction connexins, TRPC3 and TRPV4 have also been identified [10, 11, 14, 55, 90–93]. In mouse and rat mesenteric arteries, acetylcholine increased the frequency and number of InsP3-dependent Ca2+ pulsars in this region which were linked to activation of IKCa channels to evoke EDH [10, 93] (Figure 2). TRPC3 may support this process by providing Ca2+ entry for refilling of InsP3-sensitive ER stores, and/or direct activation of both SKCa and IKCa channels [91, 94]. However, in other reports acetylcholine exclusively stimulates TRPV4 in the vicinity of MEGJs to generate Ca2+ sparklets and which in turn activate IKCa channels in mouse mesenteric arteries [14, 95]. This occurs via a mechanism dependent on the anchoring protein AKAP, and is consistent with deletion of TRPV4 resulting in blunting of acetylcholine-evoked increases in endothelial [Ca2+]i and loss of EDH in mouse mesenteric arteries [75, 76]. TRPV3 [96] and TRPA1 [97] are also expressed in endothelial cells and activators of these channels can certainly initiate increases in Ca2+ signaling and EDH in cerebral arteries, but a role for these channels in agonist-stimulated EDH has yet to

The Endothelium: The Vascular Information Exchange http://dx.doi.org/10.5772/intechopen.79897 49

In contrast to IKCa channels, SKCa channels are associated with caveolae and are diffusely distributed across the cell membrane with a higher level expression at endothelial-endothelial cell borders [12, 55, 90, 93]. Also, unlike IKCa channels, evidence is lacking for a direct link between agonist-evoked, InsP3-mediated Ca2+ events and SKCa channel activity. Instead, it

Figure 2. Schematic showing discrete Ca2+ signaling events elicited by agonists at endothelial GPCRs. InsP3-dependent Ca2+ pulsars are linked to activation of IKCa channels to evoke EDH whereas Ca2+ influx through DAG-activated TRPC

channels is the primary source of Ca2+ for agonist stimulation of endothelial SKCa channels and eNOS.

be demonstrated.

The first evidence that differential endothelial Ca2+ signaling underlies agonist-evoked EDH and NO came from a study of rat isolated middle cerebral arteries in which EDH-dependent vasodilation to purinergic agonists required a larger increase in [Ca2+]i than for NO [82]. Measurements of global [Ca2+]i indicated that different sources of Ca2+ contributed to agoniststimulated production of NO and EDH; NO production is associated with SOCE [83] whereas EDH is linked to both InsP3-mediated Ca2+ release and SOCE [84]. Similarly, both agonist evoked SOCE and NO production are suppressed in isolated aortae from mice lacking STIM1, the primary endothelial STIM [85]. Building on these findings, data accrued over the past 15 years from functional, histological, Ca2+ imaging and immunohistochemical studies of intact arteries and endothelial-smooth muscle co-cultures support agonist-evoked EDH and NO release being mediated by distinct Ca2+ signaling within specialized domains.

#### 2.2.1. EDH

EDH is mediated by opening of both IKCa and SKCa channels but their relative contribution to agonist-evoked vasodilation, based on the effects of selective pharmacological inhibitors, displays significant variation between agonists and arteries. Simultaneous block of both IKCa and SKCa channels is required to inhibit acetylcholine-evoked EDH in mesenteric arteries from rats and mice, and guinea-pig coronary arteries [86–88] whereas in rat cerebral and human mesenteric arteries the same response is largely reliant on IKCa channels [89, 90].

IKCa and SKCa channels display a differential spatial distribution within endothelial cells and their contribution to agonist-evoked EDH appears to be mediated by different signaling pathways. In mesenteric arteries from rats, mice and humans, IKCa channels are localized within regions associated with MEGJs in which ER membrane, InsP3 receptors, gap junction connexins, TRPC3 and TRPV4 have also been identified [10, 11, 14, 55, 90–93]. In mouse and rat mesenteric arteries, acetylcholine increased the frequency and number of InsP3-dependent Ca2+ pulsars in this region which were linked to activation of IKCa channels to evoke EDH [10, 93] (Figure 2). TRPC3 may support this process by providing Ca2+ entry for refilling of InsP3-sensitive ER stores, and/or direct activation of both SKCa and IKCa channels [91, 94]. However, in other reports acetylcholine exclusively stimulates TRPV4 in the vicinity of MEGJs to generate Ca2+ sparklets and which in turn activate IKCa channels in mouse mesenteric arteries [14, 95]. This occurs via a mechanism dependent on the anchoring protein AKAP, and is consistent with deletion of TRPV4 resulting in blunting of acetylcholine-evoked increases in endothelial [Ca2+]i and loss of EDH in mouse mesenteric arteries [75, 76]. TRPV3 [96] and TRPA1 [97] are also expressed in endothelial cells and activators of these channels can certainly initiate increases in Ca2+ signaling and EDH in cerebral arteries, but a role for these channels in agonist-stimulated EDH has yet to be demonstrated.

the role of InsP3-mediated Ca2+ release and subsequently store-operated Ca2+ entry (SOCE) in this process [9]. The mechanism underlying endothelial SOCE has been controversial but recent evidence supports a model in which Ca2+ store depletion allows spatial reorganization of Ca2+ sensor protein stromal interaction molecules (STIMs) so that they can aggregate into clusters that physically interact with Ca2+-selective Orai channels at the ER-plasma membrane junction [69–72]. TRPC and TRPV4 can also interact with STIMs [73] and studies of knock-out mice have provided evidence for a role for TRPC4 in acetylcholine-evoked SOCE in aortae [74] and for TRPV4 in SOCE in mesenteric [75] and carotid arteries [76]. A receptor-operated Ca2+ entry mechanism can also be mediated by DAG-induced activation of TRPC and TRPV channels. For example, in human umbilical vein endothelial cells, bradykinin stimulated both translocation of DAG-sensitive TRPC6 to the cell membrane and Ca2+ influx [77, 78]. Expression of mRNA for another ER Ca2+ release channel, the ryanodine receptor (RyR), has been detected in endothelial cells of human mesenteric arteries [79], and RyRs have been suggested to mediate Ca2+ oscillations in cultured bovine aortic and human umbilical vein endothelial cells [80] but to date, ryanodine has been shown to have no effect on endothelial Ca2+ signaling or vasodilation [12, 81]. There is significant variation in the reported contribution of EDH, NO and other mediators to agonist-evoked dilation, both in terms of differences between agonists and arteries. Thus, for the purposes of this chapter we will limit our discussion to three agents commonly used to stimulate endothelium-dependent vasodilation in experimental studies,

The first evidence that differential endothelial Ca2+ signaling underlies agonist-evoked EDH and NO came from a study of rat isolated middle cerebral arteries in which EDH-dependent vasodilation to purinergic agonists required a larger increase in [Ca2+]i than for NO [82]. Measurements of global [Ca2+]i indicated that different sources of Ca2+ contributed to agoniststimulated production of NO and EDH; NO production is associated with SOCE [83] whereas EDH is linked to both InsP3-mediated Ca2+ release and SOCE [84]. Similarly, both agonist evoked SOCE and NO production are suppressed in isolated aortae from mice lacking STIM1, the primary endothelial STIM [85]. Building on these findings, data accrued over the past 15 years from functional, histological, Ca2+ imaging and immunohistochemical studies of intact arteries and endothelial-smooth muscle co-cultures support agonist-evoked EDH and

NO release being mediated by distinct Ca2+ signaling within specialized domains.

teric arteries the same response is largely reliant on IKCa channels [89, 90].

EDH is mediated by opening of both IKCa and SKCa channels but their relative contribution to agonist-evoked vasodilation, based on the effects of selective pharmacological inhibitors, displays significant variation between agonists and arteries. Simultaneous block of both IKCa and SKCa channels is required to inhibit acetylcholine-evoked EDH in mesenteric arteries from rats and mice, and guinea-pig coronary arteries [86–88] whereas in rat cerebral and human mesen-

IKCa and SKCa channels display a differential spatial distribution within endothelial cells and their contribution to agonist-evoked EDH appears to be mediated by different signaling pathways. In mesenteric arteries from rats, mice and humans, IKCa channels are localized within

acetylcholine, ATP and substance P.

48 Calcium and Signal Transduction

2.2.1. EDH

In contrast to IKCa channels, SKCa channels are associated with caveolae and are diffusely distributed across the cell membrane with a higher level expression at endothelial-endothelial cell borders [12, 55, 90, 93]. Also, unlike IKCa channels, evidence is lacking for a direct link between agonist-evoked, InsP3-mediated Ca2+ events and SKCa channel activity. Instead, it

Figure 2. Schematic showing discrete Ca2+ signaling events elicited by agonists at endothelial GPCRs. InsP3-dependent Ca2+ pulsars are linked to activation of IKCa channels to evoke EDH whereas Ca2+ influx through DAG-activated TRPC channels is the primary source of Ca2+ for agonist stimulation of endothelial SKCa channels and eNOS.

appears that Ca2+ influx through TRP channels is the primary source of Ca2+ for agonist stimulation of endothelial SKCa channels [94, 98]. In mouse cerebral artery, ATP caused rapid trafficking of TRPC3 to the plasma membrane to provide Ca2+ influx to selectively activate SKCa channels to cause EDH [98] (Figure 2). As described earlier, TRPV4 are also associated with caveolae and are a source of Ca2+ for SKCa channel activation in response to increases in shear stress but whether this relationship accounts for engagement of SKCa channels by agonists has not been explored.

[32]. In rat mesenteric arteries, block of SKCa and IKCa channels reduces agonist-evoked, NOmediated vasorelaxation and NO release [101]. Conversely, activators of endothelial KCa channels can enhance NO release from cultured endothelial cells, enhance ATP-induced increases in cytosolic Ca2+ concentration and NO synthesis in rat cremaster arterioles, and elicit NO-

The Endothelium: The Vascular Information Exchange http://dx.doi.org/10.5772/intechopen.79897 51

Lacking voltage-operated Ca2+ channels, endothelial Ca2+ influx is mediated by TRP channels and so membrane hyperpolarization may be required to maintain an appropriate electrochemical driving force for agonist-induced Ca2+ influx and also to prevent channel inactivation and/ or reduction in unitary conductance [105, 106]. Membrane depolarization does inhibit both agonist-induced increases in [Ca2+]i and NO release in cultured endothelial cells [107, 108], and in rat isolated basilar arteries, endothelial depolarization was associated with a reduction in NO-mediated relaxation to acetylcholine [109]. Nonetheless, the ability of hyperpolarization to regulate Ca2+ entry by increasing the electrical driving force is controversial. The large concentration gradient (20,000-fold for extracellular versus intracellular) [110] and driving force for Ca2+ entry raising the question of whether a small amplitude hyperpolarization will be insufficient to modulate Ca2+ entry. In rat mesenteric and cerebral arteries, that certainly appeared to be the case as changes in global endothelial [Ca2+]i were independent of changes membrane potential [89, 111]. However, more recent work with endothelial cell tubes isolated from resistance arteries has provided renewed support for hyperpolarization enhancing acetylcholine-evoked Ca2+ influx through TRPV4 [112] and indicate that pharmacological activation of SKCa and IKCa channel may not only enhance Ca2+ entry to further amplify KCa channel activity, but also boost NO production [113]. In mouse mesenteric arteries, acetylcholine-evoked TRPV4-dependent Ca2+ signaling was inhibited in arteries from mice lacking IKCa channels indicating that in these arteries, endothelial stimulation drives sufficient IKCa-dependent Ca2+ entry through TRPV4 to enhance dynamics [13]. IKCa channel activity modestly augmented Ca2+ event amplitude but the most notable impact was in recruiting new Ca2+ firing sites as well as increasing firing frequencies at pre-existing sites. In the same study, increasing or decreasing SKCa expression had little additional effect on the occurrence of Ca2+ events but did promote increased amplitudes and durations indicating that SKCa channels may play a role in positive feedback Ca2+ regulation by shaping the size and time course of individual events. In porcine coronary arteries stimulation of NOS by InsP3-dependent, large amplitude-low frequency Ca2+ waves [12], exactly the types of events which were lost in mesenteric arteries from mice with an endothelial specific knockout of SKCa channels [114], suggests that SKCa channels are required for their development. As mentioned above, deletion of SKCa channels impaired NO-mediated dilation to acetylcholine [32] and together, these findings support the notion that their role in protraction of Ca2+ events may be important in

The sympathetic nervous system regulates total peripheral resistance and is a key modulator of resistance artery diameter through release of noradrenaline and co-transmitters such as ATP and neuropeptide Y [115]. Noradrenaline causes vasoconstriction through activating α1 adrenoceptors on vascular smooth muscle cells, a process which is limited by engagement of

mediated relaxation in mesenteric arteries [102–104].

stimulation NOS.

2.3. Myoendothelial feedback
