Angiotensin II enhances beta -adrenergic receptor-mediated vasorelaxation in aortas from young but not old rats

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Angiotensin II enhances $beta$ -adrenergic receptor-mediated vasorelaxation in aortas from young but not old rats

William E. Schutzer¹, Hong Xue², John F. Reed¹, Jean-Baptiste Roullet², Sharon Anderson¹^,², and Scott L. Mader¹^,²

¹ Research Service, Portland Veterans Affairs Medical Center, and ² Oregon Health Sciences University, School of Medicine, Portland, Oregon 97201

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

$beta$ -Adrenergic receptor ( $beta$ -AR)-mediated (cAMP-dependent) vasorelaxation declines with advancing age. It has been shown thatangiotensin II (ANG II), a potent vasoconstrictor, enhances cAMP-mediatedvasorelaxation. Therefore, we questioned whether ANG II couldreverse age-related, impaired $beta$ -AR-mediated vasorelaxation andcAMP production. Pretreatment of aortic rings from 6-wk-old or6-mo-old male Fischer 344 rats with ANG II significantly enhancedvasorelaxation induced by isoproterenol (Iso), a $beta$ -AR agonist,and forskolin, a direct activator of adenylyl cyclase, but notdibutyryl-cAMP or isobutylmethylxanthine. The ANG II effect wasblocked by losartan but not PD-123319 and was not observed inthe aortas from 12- and 24-mo-old animals. Iso-stimulated cAMPproduction in the aorta was enhanced in the presence of ANG IIin the 6-wk-old and 6-mo-old age groups only. Results suggestANG II cannot reverse the age-related impairment in $beta$ -AR-dependentvasorelaxation. We conclude aging may affect a factor common toboth ANG II-receptors and $beta$ -AR signaling pathways or aging mayimpair cross-talk between these two receptorpathways.

cAMP; Fischer 344; forskolin; hypertension; isoproterenol

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

AGING IS ASSOCIATED with a number of specific physiological and metabolic changes affecting several organs and systems. Theaged cardiovascular system exhibits diminished responsivenessto $beta$ -adrenergic receptor ( $beta$ -AR) stimulation in the rat aorta (5),the mesenteric and pulmonary arteries (10, 16), the rabbitand guinea pig aorta (26), and the human dorsal hand veins (31).Multiple mechanisms have been implicated in this phenomenon, includingchanges in the affinity of $beta$ -AR (40), coupling efficacy of Gproteins such as G_s (25, 34), function of effector enzymessuch as adenylyl cyclase (24), and/or activity of $beta$ -AR-receptorkinases (15, 33). However, at this time, the exact natureof the age-induced impairment of the $beta$ -AR pathway remainsunknown.

Vascular tone is produced via a complex interaction among a variety of vasoactive agents that affect vascular smooth musclecells. These vasoactive agents activate (or deactivate) an elaboratenetwork of signal transduction pathways that modulate blood pressure(41). Agents such as isoproterenol (Iso) activate $beta$ -ARs thatstimulate adenylyl cyclase to increase intracellular cAMP, whichactivates protein kinase A (PKA) and ultimately elicits vasorelaxation(29). In contrast, agents such as angiotensin II (ANG II) elicitincreases in intracellular calcium, which lead to activation ofmyosin light chain kinase and thus vasoconstriction (37).

A recent study (2) has shown a novel action of ANG II in that it enhanced cAMP-mediated vasorelaxation via ANG II type1 (AT₁) receptors. This enhancement was endothelium independentand was also observed when other receptors, besides $beta$ -AR, upstreamfrom adenylyl cyclase were activated (prostaglandin I₂ receptor).However, ANG II did not enhance the relaxant effect of dibutyryl-cAMP.This suggests that this effect of ANG II is upstream from PKAin the $beta$ -AR signaling cascade and points to cAMP production asthe amplification mechanism by which ANG II exerts its effecton vasorelaxation. This hypothesis is further supported by invitro studies, which have shown that ANG II enhances $beta$ -AR-mediatedcAMP production in cultured aortic vascular smooth muscle cells(22, 30, 43) as well as in preglomerular microvascular smoothmuscle cells (19, 27).

It has been suggested that the ANG II enhancement of agonist-induced cAMP production and subsequent augmented vasorelaxationmay preserve vascular smooth muscle from the provasoconstrictiveand proproliferative effects of ANG II (27). Therefore, thisregulatory mechanism, if malfunctioning, could contribute to cardiovasculardiseases such as hypertension and atherosclerosis (19). Indeed,it is conceivable that ANG II could possibly correct the age-relateddecline in vascular $beta$ -AR function. Such a finding could have importantclinical implications and may provide new therapeutic options.Also, understanding whether cross-talk between ANG II signalingcascades and $beta$ -AR signaling cascades changes with age would yieldcritical information about the molecular basis of aging in thecardiovascularsystem.

Consequently, we examine the interaction among aging, $beta$ -AR-mediated vasorelaxation, and ANG II. We question whether the provasorelaxingeffect of ANG II is preserved during aging. The experiments areconducted with aortas from young (6 wk and 6 mo) and old (12 and24 mo) male Fischer 344 rats, an animal model widely used in experimentalaging research (9).

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Materials. Chemicals were obtained from Sigma (St. Louis, MO) unless indicated. All vasoactive chemicals were diluted in deionized water.Composition of phosphate-buffered saline (PBS) is as follows (inmM): 114 NaCl, 4.7 KCl, 1.15 KH₂PO₄, 1.1 Na₂HPO₄, 1.18 MgSO₄,15 NaHCO₃, 1.25 CaCl₂, and 5.0glucose.

Animals. Male Fischer 344 rats in four age groups (6 wk and 6, 12, and 24 mo old) were obtained from Harlan Sprague Dawley (Indianapolis,IN). Rats were euthanized by pentobarbital sodium sedation andexsanguination in accordance with the procedures approved by theInstitutional Animal Care and Use Committee at the Portland VAMedical Center. Thoracic aortas were quickly removed and cleanedof the adhering fat and connective tissue in ice-cold PBS gassedwith 95% O₂-5% CO₂.

Vascular reactivity studies. Isometric tension development was determined as described (5). Aortic rings (3-4 mm wide) were suspended between a fixedsupport and a Grass Instruments (Quincy, MA) FT.03 force transducerin a muscle bath system containing PBS at 37°C. Rings were stretchedto their optimal length and allowed to equilibrate for 90 min.After equilibration, the aortic rings were challenged three timeswith 45 mM KCl to confirm responsiveness before testing. Ringsthat responded to KCl were used to create a dose-response relationship(1 nM-10 µM) to phenylephrine (PE) by cumulative addition. Afterwashout and if experimental conditions dictated, we added losartan(10 µM; an AT₁-receptor antagonist) and/or PD-123319 (10 µM; anAT₂-receptor antagonist). Vessels were then precontracted to 70%of the maximum level of PE by addition of appropriate dose ofPE (~0.3 µM). Once a stable level of precontraction was achieved,0.05 µM isobutylmethylxanthine (IBMX; a nonspecific phosphodiesteraseinhibitor) was added. This low dose of IBMX did not alter tension.Subsequently, either 0.1 µM ANG II or appropriate control wasadded. ANG II evoked a transient contraction that returned tothe initial level of PE-induced tension after ~15 min. Thereafter,a dose-response relationship was determined for Iso, forskolin(FSK; a direct adenylyl cyclase activator), IBMX, or dibutyryl-cAMP(a nonhydrolyzable, cell-permeable cAMP analog). Figure 1 showsthe complete experimental paradigm.

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Fig. 1. Representative tracing of isolated ring preparation. Aortic rings were precontracted with phenylephrine (PE; 70% of maximal effect of PE), and, after the PE-induced contraction reached plateau, 0.05 µM isobutylmethylxanthine (IBMX) was applied. Five minutes after the addition of IBMX, ANG II (0.1 µM) was added, which induced a transient (~15 min) contraction that returned to the initial level of PE-induced tone. Subsequently, a dose-response relationship to isoproterenol (Iso; 0.001 µM-10 µM) was achieved via cumulative addition. If experimental design dictated, losartan (LO; 10 µM) or PD-123319 (PD; 10 µM) were added as indicated.

cAMP determination. Aortas were collected from rats of each age group (n = 7 rats/age group) and cut into five equal-sized rings. Each ring wasplaced into a gas-tight tube containing gassed PBS and allowedto equilibrate for 10 min at 37° C. Each ring was then exposedto a different treatment cumulatively as follows (see Fig. 3B):1) Basal treatment (vehicle only for 30 min); 2) IBMX treatment(1 µM IBMX for 30 min); 3) IBMX + ANG II treatment (IBMX for 30min and then 0.1 µM ANG II starting 10 min after the additionof IBMX and continuing through 30 min); 4) IBMX + Iso treatment(IBMX for 30 min and then 1 µM Iso 20 min after the addition ofIBMX and continuing through 30 min); and 5) IBMX + ANG II + Isotreatment (IBMX for 30 min, ANG II starting 10 min after the additionof IBMX, and Iso 20 min after the addition of IBMX and continuingthrough 30 min). Immediately after treatment, rings were immersedinto ice-cold 0.1 N HCl, finely minced, and then homogenized ina glass-glass motor-driven Kontes tissue homogenizer. Homogenateswere centrifuged at 500 g for 15 min at 4°C, and the resultingcleared supernatant was analyzed for cAMP content with a commerciallyavailable enzyme-immunoassay kit per the manufacturer's instructions(Assay Designs, Ann Arbor, MI). The protein concentration of thepellet was determined using the bicinchoninic acid method (PierceChemical, Rockford, IL). Concentration of cAMP is expressed aspicomoles of cAMP per milligrams ofprotein.

Statistical analysis. Results are expressed as mean values ± SE. The experimental unit was the number ofanimals.

In vascular reactivity studies, matched rings from each animal were utilized for each test. Two-way ANOVA (± ANG II treatmentby a dose-relaxing agent) with Bonferroni's post hoc comparisonwas performed to assess the interaction between ANG II and theefficacy of the relaxing agent. Efficacy was determined two ways:via the concentration of the relaxing agent that produced 50%of maximal response (ED₅₀) and via the concentration of the relaxingagent that produced maximal effect (ED_max). Both ED₅₀ and ED_maxwere determined by computer nonlinear regression using a four-parameterlogistic equation (GraphPad Software, San Diego, CA). Subsequently,age-related differences in ED₅₀ and ED_max were determined againby two-way ANOVA (± ANG II vs. age) with Bonferroni's post hoccomparison to assess the interaction between ANG II and age-relatedchanges in the efficacy of the relaxing agent. Statistical significancewas considered at P < 0.05.

For cAMP accumulation, differences were assessed using two-way ANOVA (treatment by age) with Bonferroni's post hoc comparisonwith P < 0.05 consideredsignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Effect of ANG II on Iso-stimulated vasorelaxation in young and old rats. We examined the influence of ANG II on Iso-induced relaxation in 6-wk-old and 6-, 12-, and 24-mo-old animals to determinethe effect of age on this phenomenon. A representative tracingis shown in Fig. 1. Isolated rings achieved a sustained contraction~7 min after exposure to PE. Addition of a low dose of IBMX (0.05µM) after the PE-mediated contraction reached plateau had no effect.Subsequent addition of ANG II (0.1 µM) evoked further contractionover that produced by PE. However, the ANG II effect was transient,and tension returned to that produced by PE by ~15 min. Controlaortic rings were time matched and received ANG II vehicle (deionizedH₂O). Neither the amplitude nor the time course of the contractionproduced by ANG II were significantly different among age groups(data not shown). Cumulative addition of Iso (1 nM-10 µM) produceddose-dependent vasorelaxation. Regardless of presence or absenceof ANG II, age-related differences were detected in Iso-ED₅₀ andIso-ED_max (Table 1). The presence of ANG II significantly reducedIso-ED₅₀ in 6-wk-old and 6-mo-old animals but not 12- or 24-mo-oldanimals (Fig. 2). ANG II also significantly enhanced the ED_maxeffect of Iso in 6-mo-old animals. Iso-ED₅₀ was reduced in theaortas from 6-wk-old and 6-mo-old animals by 43.7 ± 1.1 and 28.1± 1.5%, respectively, but increased by 9.1 ± 1.1 and 2.9 ± 0.9%in 12- and 24-mo-old animals, respectively. The ED_max effect ofIso was enhanced in 6-mo-old animals only (Table 1).

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Table 1. Age-related differences in Iso-ED₅₀ and Iso-ED_max

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Fig. 2. Effect of ANG II on Iso-mediated vasorelaxation in 6-wk-old (A), 6-mo-old (B), 12-mo-old (C), and 24-mo-old (D) animals. Aortic rings were contracted with PE, incubated in ANG II (0.1 µM;

) or vehicle (

), and then relaxed with a cumulative addition of Iso after the ANG II-mediated contraction returned to its initial tone. Data are expressed as a percentage of PE-induced contraction versus dose of Iso. Each point represents the mean response to Iso ± SE (n = 12 animals/age group). *P < 0.05 via 2-way ANOVA (± ANG II by dose of Iso) with Bonferroni's post hoc comparison. The efficacy of Iso alone (solid bars) versus ANG II + Iso (open bars) effect on the concentration of the relaxing agent (Iso) producing a 50% maximal effect (Iso-ED₅₀; E) and the concentration of the relaxing agent (Iso) producing a maximum effect (Iso-ED_max; F) is also shown. ANG II significantly decreased the Iso-ED₅₀ in 6-wk-old and 6-mo-old animals, whereas ANG II increased the ED_max effect of Iso in 6-mo-old animals. *P < 0.05 via 2-way ANOVA (± ANG II by age) with Bonferroni's post hoc comparison.

Effect of ANG II on Iso-stimulated cAMP accumulation in young and old rats. To establish a mechanism for ANG II-Iso interaction, aortic rings from 6-wk-old and 6-, 12-, and 24-mo-old animals (n = 7rats/age group) were treated as illustrated in Fig. 3B, and cAMPaccumulation was determined. There were no age-related differencesin either basal, IBMX-, or IBMX + ANG II-stimulated cAMP accumulation(Fig. 3A). A significant decline in IBMX + Iso-stimulated cAMPaccumulation was observed with age (275.3 ± 34.1, 165.5 ± 17.8,125.6 ± 16.8, and 95.3 ± 19.7 pmol/mg for 6-wk-old and 6-, 12-,and 24-mo-old animals, respectively). Finally, ANG II significantlyaltered the stimulatory effect of Iso on cAMP accumulation in6-wk-old and 6-mo-old animals but not in 12- or 24-mo-old animals(+44.6 ± 3.1, +63.6 ± 7.5, $-$ 6.4 ± 1.3, and $-$ 7.3 ± 3.3%, respectively,for each age group; Fig. 3A).

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Fig. 3. Effect of ANG II (0.1 µM) on Iso (1 µM)-mediated cAMP production in aortas (n = 7 rats/age group) from 6-wk-old and 6-, 12-, and 24-mo-old animals (A) as stimulated in the protocol depicted in B. An age-related decline in cAMP production was detected in response to Iso. ^aP < 0.05 compared with 6 wk old; ^bP < 0.05 compared with 6 mo old. ANG II (0.1 µM) enhanced the effect of Iso on cAMP production in aortas from 6-wk-old and 6-mo-old animals only. *P < 0.05 compared with the effect of Iso alone to ANG II + Iso. Results determined by 2-way ANOVA (±ANG II by age) with Bonferroni's post hoc comparison. Notice discontinuous ordinate. EQUILIB, equilibrium.

Determination of ANG II receptor type involved in enhanced Iso-stimulated vasorelaxation. Two receptor types for ANG II have been identified: AT₁ and AT₂, both of which have been found in vascular tissue, includingthe rat aorta (39). Accordingly, both AT₁ and AT₂ receptorshave distinct signal transduction pathways and subsequent physiologicaleffects (reviewed in Ref. 17). To establish whether AT₁ and/orAT₂ receptor stimulation was responsible for ANG II/Iso enhancementof vasorelaxation, aortic rings from 6-wk-old and 6-, 12-, and24-mo-old animals (n = 8 rats/age group) were examined in thepresence or absence of losartan and/or PD-123319. Losartan blockedthe contractile effect of ANG II in each age group. However, PD-123319did not significantly change the force or duration of ANG II-mediatedvasoconstriction in any age group (data not shown). The enhancingeffect of ANG II (in terms of reduced Iso-ED₅₀ and increased Iso-ED_max)was blocked by losartan in 6-wk-old and 6-mo-old animals, whereasPD-123319 did not significantly alter Iso-ED₅₀ or Iso-ED_max whenANG II was present. Neither losartan nor PD-123319 affected Iso-ED₅₀or Iso-ED_max in 12- or 24-mo-old animals (Fig. 4).

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Fig. 4. Effect of LO and or PD-123319 on Iso-ED₅₀ (A) and Iso-ED_max (B) on ANG II-enhanced, Iso-stimulated vasorelaxation in 6-wk-old and 6-, 12-, and 24-mo-old animals (n = 8/age group). *P < 0.05 compared with Iso alone within each age group.

Effect of ANG II on FSK-, dibutyryl-cAMP-, or IBMX-stimulated vasorelaxation in young and old rats. Experiments were performed to localize the signal transduction targets in the ability of ANG II to enhance agonist-inducedvasorelaxation. Aortic rings from 6-wk-old and 12-mo-old animals(n = 10/age group) were treated as shown in Fig. 1 except vesselswere relaxed with either FSK (1 nM-10 µM), dibutyryl-cAMP (5 µM-1mM), or IBMX (1 nM-10 µM). ANG II significantly enhanced the effect(both ED₅₀ and ED_max) of FSK in 6-wk-old but not 12-mo-old animals(Fig. 5). In 6-wk-old animals, the ED₅₀ for FSK was reduced 48.6± 6.5% by ANG II pretreatment (35.4 ± 5.6 vs. 18.8 ± 4.1 nM).The maximal effect of FSK was enhanced 9.1 ± 0.8% via ANG II pretreatmentin 6-wk-old animals (100.2 ± 1.1 vs. 110.9 ± 1.5%). In 12-mo-oldanimals, the ED₅₀ was 33.5 ± 6.9 versus 29.9 ± 6.2 nM, whereasthe ED_max was 106.3 ± 1.3 versus 104.5 ± 1.3% with and withoutANG II pretreatment, respectively. Efficacy of dibutyryl-cAMPand IBMX were not altered with ANG II pretreatment (data not shown).Finally, no age-related changes were detected in the efficacyof either FSK (Fig. 5) or IBMX (data not shown).

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Fig. 5. Effect of ANG II on forskolin (FSK)-mediated vasorelaxation in 6-wk-old (A) and 12-mo-old (B) animals. Aortic rings were contracted with PE, incubated in ANG II (0.1 µM;

) or vehicle (

), and then relaxed with a cumulative addition of FSK after the ANG II-mediated contraction returned to its initial tone. Data are expressed as a percentage of PE-induced contraction versus dose of FSK. Each point represents the mean response to FSK ± SE (n = 10 animals/age group). *P < 0.05 via 2-way ANOVA (± ANG II by dose FSK) with Bonferroni's post hoc comparison. Efficacy of FSK alone (solid bars) versus ANG II + FSK (open bars) effect on FSK-ED₅₀ (C) and FSK-ED_max (D). ANG II significantly decreased FSK-ED₅₀, whereas ANG II increased the FSK-ED_max in 6-wk-old animals only. *P < 0.05 via 2-way ANOVA (±ANG II by age) with Bonferroni's post hoc comparison.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The present study examines the effect of ANG II on agonist-induced vasorelaxation and cAMP production in the aortas from ratsof different ages. Our results show that this effect of ANG IIon agonist-induced vasorelaxation is limited to young (6 wk old)or adult (6 mo old) rats and is absent in aged (12 and 24 mo old)animals. In addition, ANG II only enhances vasorelaxation to agoniststhat function upstream of PKA in the $beta$ -AR signaling cascade, suchas Iso and FSK. ANG II does not enhance the vasodilatory effectof IBMX or dibutyryl-cAMP. With agents that ANG II enhances efficacy,the effect appears to be mediated by AT₁ receptors because itis blocked by losartan but not PD-123319. ANG II appears to amplifyvasorelaxation in the aortas from 6-wk-old and 6-mo-old animalsvia enhanced production of cAMP. The mechanism(s) surroundingthis phenomenon are discussed below and presented schematicallyin Fig. 6.

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Fig. 6. Schematic representation of discussed interacting signal transduction pathways. $beta$ -Adrenergic receptors ( $beta$ -AR) are activated by Iso, which induces coupling between the G protein (G_s) and adenylyl cyclase (AC). Upon activation by G_s, AC catalyzes the conversion of ATP to cAMP. cAMP activates protein kinase A (PKA), which ultimately promotes vasorelaxation. ANG II activates ANG II type 1 receptors (AT₁-R), which couple to G_q and result in activation of phospholipase C (PLC), which promotes increases in intracellular calcium and vasoconstriction. Calcium also activates protein phosphatase 2b (PP2b). Pathways 1, 2, and 3 represent hypothetical interactions that may explain the ability of ANG II to enhance $beta$ -AR-mediated responses and are reviewed in DISCUSSION.

Aging is associated with a pronounced decline in $beta$ -AR-stimulated cAMP production and subsequent function (6, 10, 16,23-25, 34). Generally, there is an age-related decrease in $beta$ -ARresponsiveness in the blood vessels, heart, brain, parotid gland,and lung to both circulating and pharmacological $beta$ -AR agonists(21, 26). Experiments with human vessels, including in vivostudies of the dorsal hand vein and in vitro studies of the saphenousvein, found decreased $beta$ -AR-mediated relaxation with age (18,31).

The aortas from Fischer 344 rats exhibit impaired $beta$ -AR-mediated vasorelaxation with age, whereas FSK-mediated relaxation isnormal (5). $beta$ -AR density in whole artery preparations is unaltered(40) or declines only very slightly with age (16), suggestingthat age-impaired vasorelaxation is not related to $beta$ -AR downregulation.However, Gurdal et al. (16) reported a complete loss of high-affinityreceptors with age. The age-related loss of vasorelaxation appearsto be explained by a deficiency in cAMP production but not PKAactivity. Tissue cAMP accumulation to Iso stimulation is proportionalto relaxation in young and old age groups, and both FSK and dibutyryl-cAMPrelax both ages of vessels normally (6, 10, 20). Together,these data suggest that the age-related decline in $beta$ -AR-mediatedsignaling may be due in part to changes in the $beta$ -AR affinity stateand, therefore, changes in the ability of $beta$ -ARs to transduct signalwith increasing age. The results of the present study confirmthat there are age-related declines in cAMP production (Fig. 3)and $beta$ -AR-mediated vasorelaxation (Fig. 2). The results furtherconfirm that FSK- and IBMX-mediated vasorelaxation are unaffectedby advancing age (Fig. 5).

The age-related effects of ANG II signaling are equivocal (11). Some investigators (4) have shown decreased vascularresponsiveness with increasing age. Conversely, others (13)have shown an increased contractile effect to ANG II with increasingage. Still others (3) have reported no differences across ageto the constrictor effect of ANG II. The differences in thesereports may be explained by preparation differences (the aorta,cardiac artery, or saphenous vein), species differences (dogs,rats, rat strains, or humans), or analytical techniques (in vivo,in vitro and organ bath with tension development, or in vitroand perfused pressure development). The present study found noage-related changes in the time course or the maximal contractileeffect of a single dose of ANGII.

ANG II has been shown to potentiate the effect of agents that elevate cAMP, including Iso, which is a $beta$ -AR agonist. To ourknowledge, the first report of this interesting phenomenon wasfrom Nabika et al. (30) in a cultured vascular smooth musclecell model. ANG II, functioning through activation of G_q-linkedreceptors, stimulates the activation of protein kinase C (PKC)and release of intracellular calcium (12). Kubalak and Webb(22) showed that when cultured vascular smooth muscle cellswere exposed to ANG II before treatment with Iso, the ANG II-exposedcells had enhanced cAMP generation. This effect was partiallyblocked by staurosporine (an inhibitor of PKC), 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraaceticacid (BAPTA, an intracellular calcium chelator), and W-7 (a calmodulininhibitor), suggesting that ANG II exposure enhanced Iso-mediatedcAMP production through either PKC, calmodulin, or changes inintracellular calcium. In a subsequent study, Zhang et al. (43)extended these results to another G_q-linked receptor agonist,arginine vasopressin, thus establishing the importance of theG_q-linked receptor pathway rather than an effect of a specificagonist. Finally, Brizzolara-Gourdie and Webb (2) tested thisparadigm in whole vascular tissue and studied vasorelaxation.Their data show that when vessels were initially exposed to ANGII and then treated with G_s-linked receptor agonists, Iso,or iloprost (prostaglandin receptor agonist), there was enhancedvasorelaxation. Enhanced vasorelaxation occurred regardless ofthe precontracting agent (KCl, PE, or endothelin) and was notaffected by the presence or absence of the endothelium. Furthermore,ANG II had no effect on relaxation stimulated bynitroprusside.

Cross-talk between G_q-linked receptors and $beta$ -ARs have been studied by others. Winstel et al. (42) found that activationof PKC by G_q-linked agonists directed G protein receptorkinases (GRKs) to the membrane, enhancing $beta$ -AR phosphorylation.Also, it has been shown that GRK-2 is more effective at desensitizing $beta$ -ARs after its activation by PKC (8). Finally, Shih and Malbon(35) used antisense technologies to knockout PKC expressionand function and determined that this manipulation produced enhanced $beta$ -AR agonist-induced desensitization rather than the expectedattenuation result. They also found that this effect was linkedto phosphatase activity (36). These findings suggest that PKCmight also be involved with $beta$ -AR resensitization through interactionwith a phosphatase. Therefore, phosphorylation/dephosphorylationand desensitization/resensitization of $beta$ -ARs can be induced froma number of stimuli and certainly through ANG II-mediated signaling.Determining how the aging may affect the phosphorylation processisnecessary.

Mechanisms of action to explain the effect of ANG II on $beta$ -AR signaling are equivocal. One explanation for the effect of ANGII on $beta$ -AR-mediated signaling is provided by Zhang et al. (43),as discussed above, and by Fig. 6 (pathway 1). They suggest thatANG II, functioning through AT₁ receptors, elicits increases inintracellular calcium, which activates calcium-dependent adenylylcyclases that produce more cAMP upon $beta$ -AR activation. The presentdata (Fig. 5) and the literature (6) suggest that there areno age-related differences in adenylyl cyclase function with aging.FSK-stimulated cAMP production or FSK-mediated vasorelaxationare unaffected with advancing age (5). However, this adenylylcyclase hypothesis could explain the results of the present studyif there were an age-related shift in the ratio of calcium-sensitiveto noncalcium-sensitive cyclases. In the aortas from 6-wk-oldanimals, there was enhanced FSK-mediated relaxation with ANG IIpretreatment. This effect of FSK disappears in the aortas from12-mo-old animals (Fig. 5). An age-related change in adenylylcyclase subtypes is supported in the literature. Tobise et al.(38) found that concentrations of cardiac type V adenylyl cyclaseremained constant, whereas type IV adenylyl cyclase declined withadvancingage.

Likewise, ANG II could somehow modify the function of the G protein G_s (Fig. 6, pathway 2). Kubalak and Webb (22) foundthat ANG II potentiates the ability of not only cholera toxin(directly activates G_s) but also prostaglandin I₂, adenosine,and vasopressin (all of which activate G_s-linked receptors)to stimulate cAMP accumulation in cultured vascular smooth musclecells. Certainly, the vascular reactivity results of Brizzolara-Gourdieand Webb (2) suggest that G_s could be the target of ANGII in that Iso as well as iloprost (both of which activate G_s-linkedreceptors) yield enhanced vasorelaxation with ANG II pretreatment.G_s has been a target protein of interest in the field ofaging in that it has been shown that cholera toxin treatment ofthe aortas from aged rats produced significantly less cAMP accumulationcompared with younger rats (21). Mader et al. (25) have shownthat cholera toxin-induced labeling of G_s decreases withage in rat aortic membranes, whereas Western blotting showed nodifference in G_s protein levels. Chapman et al. (5) havealso shown that cholera toxin-induced vasorelaxation likewisedeclines with age in rataortas.

Another hypothesis put forth in the literature that may explain the effect of ANG II on $beta$ -AR signaling is through phosphataseactivity (Fig. 6, pathway 3). Calcineurin (protein phosphatase2B) is a calcium/calmodulin-regulated phosphatase that has beenrecently implicated in cardiovascular pathology (28). Baukalet al. (1) found that the effect of ANG II on agonist-inducedcAMP production could be blocked by FK-506 and cyclosporin A,both of which are inhibitors of calcineurin. Furthermore, Shihand Malbon (36) showed that calcineurin was directly involvedin $beta$ -AR resensitization. In their model, calcineurin dephosphorylatedand, therefore, resensitized $beta$ -AR to agonist signaling. Therefore,the ANG II effect on $beta$ -AR may be via a calcineurin action on the $beta$ -AR itself. Age-related changes in calcineurin itself or in ANGII-mediated activation of calcineurin are, to our knowledge,unexplored.

A final hypothesis in understanding the effect of ANG II on $beta$ -AR signaling is through ANG II-mediated effects on GRKs. $beta$ -AR-phosphorylationcauses profound decreases in the ability of the receptor to transducesignals in response to agonist binding (14). GRKs are a superfamilyof kinases that phosphorylate and desensitize G protein-linkedcoupled receptors (32). Three GRKs, GRK-2, GRK-3 (also knownas $beta$ -AR kinase 1 and 2), and GRK-5, rapidly phosphorylate anddesensitize not only $beta$ -ARs but also many other G_s-linkedreceptors upon agonist binding in numerous tissues, includingthe cardiovascular system (7). GRKs have been shown to be regulatedby agents that elevate PKC activity, such as ANG II. Taken together,the available data suggest that activation of GRKs by ANG II woulddecrease receptor-mediated responses. Thus a GRK hypothesis couldexplain the deficiency in the stimulatory effect of ANG II on $beta$ -AR-mediated vasorelaxation in old animals, because they haveupregulated GRK expression and activity (33). However, GRK activationwould not be involved in the stimulatory mechanism of ANG II onIso-mediated signaling observed in the aortas from younganimals.

In summary, ANG II enhances $beta$ -AR-mediated cAMP production and vasorelaxation in young but not old animals. It is well establishedthat there is an age-related decline in $beta$ -AR signaling that involvesa mechanism associated with $beta$ -AR function and/or coupling to adenylylcyclase. The mechanisms involved with ANG II enhanced, $beta$ -AR-mediatedsignaling are unknown but may involve adenylyl cyclase, G_s,or calcineurin. We suggest that aging may affect a factor commonto both ANG II receptors and $beta$ -AR signaling pathways, or agingmay impair cross-talk between these two receptorpathways.

	ACKNOWLEDGEMENTS

The authors thank Terry T. Oyama for technical expertise and Dr. Radko Komers (Division of Nephrology, Oregon Health SciencesUniversity) for editorialcomments.

	FOOTNOTES

This work was supported by the Research Service, the Department of Veterans Affairs (to S. L. Mader), the Medical ResearchFoundation of Oregon (to S. L. Mader), and US Public Health ServiceGrant AG-14699 (to S.Anderson).

A portion of these data were presented at the 2000 Experimental Biology Meeting, San Diego, California, April 15-18.

Address for reprint requests and other correspondence: S. L. Mader, Portland VA Medical Center, Research Service, R&D 26,3710 SW US Veterans Hospital Rd., Portland, OR 97201 (E-mail:scott.mader{at}med.va.gov).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate thisfact.

Received 7 April 2000; accepted in final form 28 June 2000.

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Angiotensin II enhances -adrenergic receptor-mediated vasorelaxation in aortas from young but not old rats

Angiotensin II enhances $beta$ -adrenergic receptor-mediated vasorelaxation in aortas from young but not old rats