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Division of Nephrology, University of Maryland School of Medicine, Baltimore, Maryland 21201-1595
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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We tested the hypothesis that constriction
of descending vasa recta (DVR) is mediated by voltage-gated calcium
entry. K+ channel blockade with BaCl2 (1 mM) or
TEACl (30 mM) depolarized DVR smooth muscle/pericytes and constricted
in vitro-perfused vessels. Pericyte depolarization by 100 mM
extracellular KCl constricted DVR and increased pericyte intracellular
Ca2+ ([Ca2+]i). The
KATP channel opener pinacidil
(10
7-104 M) hyperpolarized resting
pericytes, repolarized pericytes previously depolarized by ANG II
(108 M), and vasodilated DVR. The DVR vasodilator
bradykinin (107 M) also reversed ANG II depolarization.
The L-type Ca2+ channel blocker diltiazem vasodilated ANG
II (108 M)- or KCl (100 mM)-preconstricted DVR, and the
L-type agonist BayK 8644 constricted DVR. The plateau phase of the
pericyte [Ca2+]i response to ANG II was
inhibited by diltiazem. These data support the conclusion that DVR
vasoreactivity is controlled through variation of membrane potential
and voltage-gated Ca2+ entry into the pericyte cytoplasm.
medulla; kidney; microcirculation; patch clamp; fura-2; KCl
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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BLOOD FLOW TO THE MEDULLA of the kidney is supplied by descending vasa recta (DVR). These vessels arise from juxtamedullary efferent arterioles and either traverse the center of outer medullary vascular bundles to supply blood flow to the inner medulla or branch from the bundle periphery to supply the outer medullary interbundle region (12). Thus DVR might have a role to regulate the relative distribution of blood flow to the outer vs. inner medulla of the kidney. In addition to endothelial expression of aquaporin 1 and facilitated urea transport, smooth muscle remnants known as pericytes impart a contractile function to the DVR wall (25, 26). The signaling pathways that mediate and modulate DVR vasoreactivity are largely unexplored and would be expected to play a role in the regulatory functions of the renal medulla, including urinary concentration and the control of salt and water excretion (5, 20, 21).
Calcium influx through voltage-gated channels mediates contraction of many types of smooth muscle (11, 29). In the kidney, it is generally accepted that afferent arteriolar smooth muscle responds to ANG II stimulation by depolarizing and activating L-type calcium channels. Studies in the efferent arteriole have yielded mixed results, most often failing to identify a role for depolarization and activation of voltage-gated calcium entry pathways (1, 2, 4, 7, 10, 14-17). Hansen et al. (9) recently shed new light on this subject by identifying expression of both L- and T-type calcium channels in juxtamedullary but not cortical efferent arterioles. Also, we recently showed that DVR pericytes respond to ANG II by depolarizing (23, 35), an event that is expected to presage voltage-gated calcium entry into the pericyte cytoplasm. In this study we tested whether vasoconstriction and vasodilation of DVR is accompanied, in parallel, by depolarization and hyperpolarization of pericyte membrane potential. The results confirm that depolarization by K+ channel blockers or high KCl induces mild vasoconstriction and that the vasodilators pinacidil and bradykinin repolarize ANG II-treated pericytes. Finally, a role for voltage-gated calcium entry pathways was confirmed because the L-type calcium channel blocker diltiazem relaxes ANG II- or KCl-constricted DVR and prevents ANG II-induced calcium entry into the pericyte cytoplasm.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Isolation of DVR. Kidneys were harvested from Sprague-Dawley rats (70-150 g; Harlan) that had been anesthetized by an intraperitoneal injection of thiopental (50 mg/kg body wt). Tissue slices were placed in buffer and maintained at 4°C. Individual DVR were dissected from outer medullary vascular bundles and transferred to the stage of an inverted microscope for fluorescence imaging or microperfusion studies as previously described (22-24, 27). The solution used for dissection, microperfusion, and measurement of vasoreactivity contained (in mM) 140 NaCl, 10 Na acetate, 5 KCl, 1.2 MgSO4, 1.2 Na2HPO4, 1 CaCl2, 5 HEPES, 5 L-alanine, 5 D-glucose, and 0.5 g/dl bovine albumin. The pH was adjusted to 7.55 at room temperature using NaOH to yield a pH of ~7.4 at 37°C. When patch clamp studies were performed, tissue was stored in physiological saline solution (PSS). PSS also served as the extracellular solution during membrane potential recordings. PSS contained (in mM) 145 NaCl, 5 KCl, 1 MgCl2, 1 CaCl2, 10 HEPES, 10 glucose, pH 7.4 at room temperature.
Measurement of DVR diameter.
Vasoactivity was monitored in DVR perfused in vitro as previously
described (22). Vessels were recorded on videotape
(Panasonic WV-BL90) and diameters were analyzed during playback. The
inverted microscope supporting the chamber was equipped with a beam
splitter and a side port with a C-mount for attachment of a video
camera. DVR luminal diameter was observed with a ×40 dry objective;
the final magnification on the videoscreen was ×1,300. Internal
diameters were measured using calipers at the location of maximal
constriction. Diameter changes are expressed as percentage
constriction, given by [1 
(D/D0)] × 100, where D
is experimental diameter and D0 is initial baseline
diameter. The effects of KCl- and TEACl-induced depolarization were
tested by isosmolar substitution of NaCl to yield the desired KCl or
TEACl concentration. In some protocols, either 100 mM KCl or ANG II
(108 M) was substituted into the bath to preconstrict
vessels and permit assessment of the subsequent effects of vasodilators.
Isolation of pericytes from the DVR wall. Small wedges of renal medulla were separated from kidney slices by dissection and transferred to CaCl2-free PSS containing collagenase 1A (0.45 mg/ml, Sigma), protease XIV (0.4 mg/ml, Sigma), and albumin (1.0 mg/ml) (23, 35). These were incubated at 37°C for 22 min and then transferred back to CaCl2 (1 mM) containing PSS and held at 4°C in a petri dish. At intervals, vessels were isolated from the digested renal tissue by microdissection and transferred to a perfusion chamber on an inverted microscope (Nikon Diaphot). In the chamber, DVR were captured and aspirated into a microperfusion-style collection pipette with an opening of 5-10 µm. As previously described and illustrated (32), during the aspiration, pericytes strip from the abluminal surface of the vessel. Once the vessel has been completely drawn into the pipette, a preparation of isolated pericytes remains suspended in the bath, adherent to the pipette tip, available for fura-2 loading and intracellular calcium ([Ca2+]i) measurements.
Measurement of [Ca2+]i. Pericytes were loaded with fura-2 by incubating them with the fura-2 AM ester (10 µM, Molecular Probes, Eugene, OR) for 20 min at 37°C in the presence of probenecid (1 mM). This yields a strong fluorescent signal because the anion transport inhibitor probenecid prevents leakage of de-esterified fura-2 from the cytoplasm (32). A photon-counting photomultiplier assembly was employed to measure the fluorescent emission of fura-2 at 510 nm. Excitation was provided by a 75-W xenon arc lamp using a 350/380 nm wavelength combination isolated with a computer-controlled monochrometer (PTI, Lawrenceville, NJ). Fluorescent emission was isolated with a 510WB40 bandpass filter (Omega Optical, Brattleboro, VT) and collected with a Nikon CF fluor ×40 oil immersion objective (1.3 numerical aperture). The background-subtracted ratio of fluorescent emission (R350/380) was converted to the equivalent intracellular calcium concentration assuming a dissociation constant of 224 nM for fura-2 at 37°C. Rmax and Rmin were measured by exposing vessels to buffer containing 5 mM CaCl2 or 0 CaCl2, 0.5 mM EGTA, respectively, along with 10 µM ionomycin (24).
Whole cell patch clamp recording.
Membrane potential (
m) was monitored by patch clamp
recording from pericytes at room temperature. To accomplish this, DVR were digested with the same enzyme treatment described above for pericyte isolation (23, 35). Patch clamp studies of
pericytes were always done on intact vessels, i.e., pericytes isolated
by stripping were used for [Ca2+]i
measurements but not for electrophysiological studies. Patch pipettes
were made from borosilicate glass capillaries (PG52151-4, external
diameter 1.5 mm, internal diameter 1.0 mm; World Precision Instruments,
Sarasota, FL), using a two-stage vertical pipette puller (Narshige
PP-830) and heat polished. To obtain electrical access for whole cell
perforated patch clamp recording, nystatin was used as the pore-forming
agent. The pipette solution contained (in mM) 120 Kaspartate, 20 KCl,
10 NaCl, 10 HEPES, pH 7.2, and nystatin (100 µg/ml with 0.1% DMSO)
in ultrapure water. Nystatin in DMSO was kept frozen at 20°C and
renewed weekly. Each day, the nystatin stock was thawed, dispensed into
the Kaspartate pipette solution at 37°C by vigorous vortexing for 1 min, and subsequently protected from light. Pipettes were backfilled
with nystatin-containing electrode solution via a 0.2-µm filter.
m was measured using a CV201AU headstage and Axopatch 200A amplifier
(Axon Instruments, Foster City, CA) in current clamp mode
(I = 0) at a sampling rate of 10 Hz. m was recorded
with pipettes of 8-15 M
resistance. Lower resistance pipettes
proved technically difficult to use and led to premature loss of seals. Pipettes with nystatin-containing electrode solution were inserted into
the bath under positive pressure, positioned near the cell, and the
offset of the amplifier was adjusted to null the junction and electrode
potentials. The final approach to the cell was controlled with a
piezoelectric drive (Burleigh PCS-5000). Gigaseals were established by
pressing the pipette tip against the cell and applying light suction.
After seal formation, the appearance of the cell capacitance transient
and the access resistance were monitored using a Digidata
analog-to-digital converter and Clampex 7.0 (Axon Instruments, Union
City, CA) with 10-mV pulses at a holding potential of 70 mV. Final
access resistance was generally between 15 and 40 M. A 3 M KCl agar
bridge was used as the bath electrode. Junction and Donnan potential
corrections were applied as previously described (22).
Reagents.
ANG II, bradykinin (BK), probenecid, pinacidil, diltiazem, ionomycin,
bovine serum albumin (A2153, Cohn fraction V), nystatin, collagenase
1A, and protease XIV were from Sigma (St. Louis, MO). ANG II, BK,
pinacidil, and diltiazem were stored in water in 200-µl aliquots at
20°C and diluted 1:100 or 1:1,000 on the day of the experiment. The
enzyme digestion solution was prepared in 50-ml batches, frozen in 2-ml
aliquots, and thawed daily as needed. Fura-2 (Molecular Probes) was
stored at 1 mM in anhydrous DMSO. Reagents were thawed once and the
excess was discarded at the end of the day.
Statistics. Data in the text and figures are given as means ± SE. The significance of differences between means was calculated using Student's t-test (paired or unpaired, as appropriate) and analysis of variance. Where sampling rates were high, the majority of error bars were suppressed to clarify display of data.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Vasoconstriction by K+ channel
blockers.
We verified that the K+ channel blockers BaCl2
and TEACl were effective to depolarize DVR pericytes. During
I = 0 current clamp recording of m,
BaCl2 (1 mM) or TEACl (30 mM) was introduced into the bath
for 5 min and then washed out. BaCl2 depolarized pericytes
from 56.2 ± 2.8 to 36.0 ± 4.5 mV (n = 7, P < 0.05, Fig. 1,
A and B). TEACl depolarized pericytes from
62.0 ± 2.4 to 35.8 ± 4.3 mV (Fig. 1, C and
D, n = 7, P < 0.05). Having
established that these agents depolarize the pericyte cell membrane, we
tested whether they would also constrict in vitro-perfused DVR. After 2 min of baseline recording, either BaCl2 (Fig.
2A) or TEACl (Fig. 2B) was added to the bath for 10 min and then washed out.
BaCl2 decreased luminal diameter from 12.9 ± 0.8 µm
to a minimum of 11.9 ± 0.6 µm, whereas TEACl constricted from
13.4 ± 0.6 to 11.6 ± 0.6 µm. Despite similar degrees of
depolarization (Fig. 1, B and D), TEACl was a
more effective constrictor of DVR than BaCl2 (P < 0.05, 6-14 min, %constriction, ordinate,
Fig. 2, A and B). We speculate that TEA was a
better constrictor because Ba2+ can compete for
Ca2+ influx pathways and Ca2+-dependent
intracellular signaling processes. Subsequent to washout of
BaCl2 and TEACl, to verify contractility of the vessels and compare their effectiveness to a biological constrictor, ANG II (108 M) was added to the bath. ANG II reduced luminal
diameter to 8.6 ± 0.5 and 8.7 ± 0.5 µm for
BaCl2 and TEACl groups, respectively. Thus both
BaCl2 and TEACl constricted DVR but were substantially less
effective than ANG II.
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KCl-induced depolarization of DVR.
To achieve pericyte membrane depolarization exceeding that resulting
from BaCl2- or TEACl-induced K+ channel
blockade (Fig. 1), we tested the effect of raising extracellular KCl
concentration to 100 mM. As expected, this maneuver strongly depolarized the pericytes from 58.2 ± 2.5 to 12.5 ± 0.2 mV (Fig. 3, A and
B). We previously showed that
ANG II depolarizes DVR pericytes toward the expected equilibrium
potential for Cl ion, about 33 mV (see below)
(23). Despite the fact that KCl depolarized pericytes to a
greater extent than ANG II, it was less effective in constricting in
vitro-perfused DVR (Fig. 3C). In separate experiments we
tested the hypothesis that depolarization by 100 mM KCl would increase
pericyte [Ca2+]i. Again, KCl depolarization
increased pericyte [Ca2+]i, but did so less
effectively than ANG II (Fig. 3D). The effect of KCl to
depolarize m occurs more rapidly in Fig. 3A than the effect to vasoconstrict or increase calcium (Fig. 3, C and
D). This is likely to be related to differences in the rate
of bath exchange that, with our apparatus, is faster for patch clamp
studies than for videomicroscopy or fluorescent microscopy.
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Vasodilation and membrane repolarization by pinacidil and BK.
If voltage-gated Ca2+ entry pathways exist in DVR
pericytes, agents that hyperpolarize the cells should be vasodilators.
To test this hypothesis, we examined the effects of the
KATP channel opener pinacidil. When this agent was applied
to the bath of DVR pericytes in log molar increasing concentrations,
m progressively declined from resting levels toward the equilibrium
potential of K+ ion (Fig. 4),
a finding that supports the expression of KATP channels in
these cells. We tested whether this agent would both repolarize DVR
pericytes and vasodilate in vitro-perfused vessels constricted by ANG
II. ANG II (108 M) depolarized pericytes from a resting
level of 63.5 ± 3.5 to 32.0 ± 1.0 mV (n = 9, P < 0.01). Addition of pinacidil
(105 M) to the bath induced m oscillations in all but
one cell, examples of which are shown in Fig. 5, A and
B. On average, the effect of
pinacidil was to repolarize the pericytes to 53.7 ± 4.3 mV (P < 0.01, Fig. 5C), an effect that was
reversible after washout. As anticipated, pinacidil effectively
vasodilated ANG II (108 M)-preconstricted DVR
(n = 8, Fig. 5D).
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7 M) vasodilates ANG
II-preconstricted in vitro-perfused DVR (24). We tested
the hypothesis that BK would hyperpolarize the pericyte cell membrane.
BK exhibited a complex biphasic effect on m and repolarized ANG II
(108 M)-treated pericytes (Fig. 6, A and
B). On average, ANG II
depolarized pericytes from 52.6 ± 2.9 to 33.4 ± 1.5 mV.
BK repolarized pericyte m to 60.4 ± 4.4 mV (Fig.
6C, n = 7, P < 0.01).
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Evidence for voltage-gated Ca2+ entry
into DVR pericytes.
Having established that DVR vasoreactivity parallels the expected
changes in m, we next tested whether the L-type channel blocker
diltiazem would induce vasodilation and whether the L-type agonist BayK
8644 would induce constriction. Diltiazem reversibly vasodilated in
vitro-perfused DVR that had been preconstricted with 100 mM KCl (Fig.
7A) or 108 M ANG
II (Fig. 7B). Also, as expected for functional expression of
L-type calcium channels, BayK 8644 constricted DVR, however, compared
with ANG II (108 M), the constriction by BayK
8644 (106 M) was mild (Fig.
8).
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8 M). In the protocol illustrated
by Fig. 9A, pericytes isolated by stripping from the abluminal surface of isolated DVR exhibited a
classical ANG II-induced peak and plateau increase in
[Ca2+]i. Diltiazem had little effect on the
peak but reduced the plateau phase of the ANG II response. For
additional confidence, diltiazem was added to the bath of six of the
seven pericyte preparations that constitute the control group in Fig.
9A. Those cells had been exposed to ANG II for 10 min before
diltiazem treatment and had reached the plateau phase of the
Ca2+ transient. Diltiazem reversibly reduced the plateau
pericyte [Ca2+]i (Fig. 9, B and
C).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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It is generally accepted that m plays an important role in the
excitation-contraction coupling of vascular smooth muscle. Depolarization of the plasma membrane reduces the electrochemical driving force for calcium entry into the cytoplasm but activates voltage-gated calcium entry pathways to enhance transmembrane conductance. A diverse array of voltage-gated calcium channels has been
identified; however, in the cardiovascular system, L type and T type
predominate (11, 29). In past studies, investigators have
examined the effect of L-type voltage-gated channel blockers on
regional blood flow in the kidney. Greater enhancement of medullary than cortical blood flow was frequently observed (3, 6, 8, 18,
34). Whether this is due to effects at the juxtamedullary afferent arteriole, efferent arteriole, or DVR is uncertain.
The high degree of specificity of L-type calcium channel blockers has been exploited in several studies to establish the role of L channels in the modulation of vasomotor tone of resistance vessels in the kidney. In the isolated perfused kidney, diltiazem and amlodipine inhibited pressure-dependent and ANG II-induced vasoconstriction, respectively (15, 16). In the hydronephrotic kidney preparation, nitrendipine was found to preferentially vasodilate preglomerular vessels (arcuate, interlobular, and afferent arterioles) (7). L-type calcium channel blockers also effectively dilate ANG II-preconstricted afferent arterioles in the in vitro-perfused juxtamedullary nephron preparation (2, 10). The demonstration that ANG II depolarizes afferent arteriolar smooth muscle implies that this constrictor could activate L channels in the afferent circulation (14).
In addition to voltage-gated calcium entry pathways, vasoconstrictors can increase [Ca2+]i via other pathways such as store-operated or receptor-operated channels. To examine functional expression of voltage-gated calcium channels, the effect of KCl-induced depolarization on vasoreactivity and [Ca2+]i has been tested. In the hydronephrotic kidney preparation, 30 mM KCl constricted afferent arterioles to a much greater degree than efferent arterioles, an effect that was blocked by nifedipine (17). Similarly, diltiazem has been found to block KCl-induced vasoconstriction in isolated perfused afferent arterioles (4). Carmines and colleagues (1) showed that KCl depolarization increased [Ca2+]i of afferent but not efferent arteriolar smooth muscle. Recently, the pathways through which ANG II stimulates Ca2+ entry into afferent and efferent arteriolar smooth muscle were examined using ratiometric detection of fura-2. ANG II increased [Ca2+]i in both arteriolar segments, but nifedipine inhibited only the afferent response, whereas the receptor-operated Ca2+ channel blocker SKF96365 blocked the increase in efferent [Ca2+]i (13). These and other studies established that L-type voltage-gated channels provide a functionally important route for calcium entry into smooth muscle of the afferent arteriole.
The recent study of Hansen and colleagues (9) provides an
important new perspective on the channel architecture of juxtamedullary renal resistance vessels. Coexpression of the 
1-subunit
for both L- and T-type calcium channels was identified in afferent
arterioles and both efferent arterioles and DVR of the juxtamedullary
circulation. In contrast, efferent arterioles arising from superficial
glomeruli did not express those channel subunits. The authors found
that depolarization by KCl could increase
[Ca2+]i of both juxtamedullary afferent and
efferent smooth muscle. The data in Figs. 7-9 provide similar
corroborating evidence for the functional presence of such pathways in
DVR pericytes. The incomplete inhibition of ANG II-induced
vasoconstriction by diltiazem in Fig. 7 raises the possibility that
pathways other than L-type channels, such as T-type or
receptor-operated channels, might be present in DVR pericytes.
Despite the small size of DVR pericytes, it has been possible to
measure ms and cellular currents in those cells (23). It is also possible to examine [Ca2+]i
transients in DVR pericytes after they have been isolated from endothelial cells by stripping. Without prior isolation of the pericytes from the DVR wall, pericyte [Ca2+]i
cannot be measured because the adjacent endothelia strongly load fura-2
and obscure the small fluorescent emission that originates from the
pericytes (32). In this study we exploited those methods to test the hypothesis that depolarization and voltage-gated
[Ca2+]i entry into DVR pericytes accompany
vasoreactivity. The nonspecific K+ channel blockers
BaCl2 and TEACl depolarize the pericytes and constrict
isolated DVR (Figs. 1 and 2). Similarly, elevation of extracellular
K+ markedly depolarizes pericytes (Fig. 3, A and
B) and induces DVR vasoconstriction that is reversed by
L-type Ca2+ channel blockade (Fig. 7). In this and a prior
study, we showed that ANG II depolarizes pericytes from resting levels
that lie between 50 and 65 mV toward the equilibrium potential for
Cl ion (Figs. 5 and 6; Ref. 23). Despite the
ability of K+ channel blockade and 100 mM extracellular KCl
to depolarize pericytes to a similar degree, they are less effective
than ANG II to stimulate DVR vasoconstriction. This finding contrasts
with observations in afferent arteriolar smooth muscle, where KCl is
highly effective to induce vasoconstriction (1, 4). On the
basis of the comparison among ANG II, Ba2+,
TEA+, and KCl (Figs. 1-3), it seems likely that ANG II
activates signaling events that are not mimicked by nonspecific
depolarization. Downstream effects of ANG II receptor occupancy, such
as tyrosine kinase activation and receptor transactivation, may be
needed to fully activate the pericyte contractile response (19,
30).
In addition to verifying that depolarization induces vasoconstriction,
we tested whether ANG II-induced vasoconstriction could be reversed by
agents that repolarize the pericyte cell membrane. Pinacidil
hyperpolarized resting pericytes and repolarized ANG II depolarized
pericytes to a remarkable degree (Figs. 4 and 5). In resting cells,
pinacidil (
105 M) reduced m to values that
approached the equilibrium potential of K+ ion (Fig. 4).
After ANG II pretreatment, the average effect of this agent was to
repolarize the pericyte to a level that lies below the threshold for
activation of either T- or L-type calcium channel activation (Fig.
5C). Pinacidil strongly reversed ANG II-induced
vasoconstriction, a finding that is consistent with functional
importance of depolarization for ANG II to constrict DVR (Fig.
5D). Given the origin of DVR in the relatively hypoxic renal
outer medulla, it is not surprising to have identified a robust effect
of KATP channel activation in these vessels. Glybenclamide is a blocker of KATP channels that is widely used as a
hypoglycemic agent in the treatment of diabetes. Two prior studies
demonstrated that glybenclamide reduces blood flow to the renal medulla
(28, 33), suggesting that KATP channel
activity exerts tonic vasodilatory effects to preserve medullary blood
flow. We previously demonstrated that BK relaxes ANG II-constricted
DVR, increases NO production, and increases DVR endothelial
[Ca2+]i (24, 27, 31). In this
study, we verified that this is accompanied by pericyte repolarization
to a degree that could inhibit voltage-gated calcium entry pathways
(Fig. 6).
A number of investigators has examined the ability of L-type calcium channel blockers to affect renal medullary blood flow. Infusion of diltiazem into the renal interstitium resulted in enhancement of papillary blood flow (18). Similarly, intravenous infusion of verapamil selectively enhanced medullary blood flow (8). Using single vessel videomicroscopy, Yagil and colleagues (34) found an increase in vasa recta blood flow with low rates of infusion of the dihydropyridine blocker CS-905. The effects of calcium channel blockade on medullary blood flow have also been examined in pathological models. Papillary plasma flow increased when verapamil was infused into the renal artery of dogs subjected to caval constriction (3). Treatment of the spontaneously hypertensive rat with nisoldipine enhanced medullary blood flow and sodium excretion (6). Taken together, an ability of calcium channel blockade to increase renal medullary blood flow seems well established. The present findings, coupled with the recent work of Hanssen and colleagues (9), imply that DVR are a likely a site of action for L-type calcium channel blockers to induce vasodilation.
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ACKNOWLEDGEMENTS |
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Studies in our laboratory are supported by National Institutes of Health Grants DK-42495, HL-62220, and HL-68686.
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FOOTNOTES |
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Address for reprint requests and other correspondence: T. L. Pallone, Division of Nephrology, N3W143, Univ. of Maryland at Baltimore, Baltimore, MD 21201-1595 (E-mail: tpallone{at}medicine.umaryland.edu).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
June 27, 2002;10.1152/ajpregu.00251.2002
Received 6 May 2002; accepted in final form 24 June 2002.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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