1 Cardiovascular Division and 2 Division of Endocrinology, University of Virginia School of Medicine, Charlottesville, Virginia 22908
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ABSTRACT |
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The purpose of this
study was to noninvasively quantify the effects of insulin on capillary
blood volume (capBV) and RBC velocity (VRBC) in
skeletal muscle in vivo with the use of contrast-enhanced ultrasound.
We performed contrast ultrasound of the rat hindlimb adductor muscles
at baseline and after 2-h infusions of either insulin (3 or 40 mU · kg1 · min
1) or saline.
Saline-treated animals were also studied during contractile exercise.
VRBC and capBV were calculated from the relation
between pulsing interval and video intensity. Femoral artery blood
flow, measured by a flow probe, increased with both contractile
exercise and insulin. Contractile exercise increased capBV more than
twofold and VRBC fivefold. Insulin also
increased capBV more than twofold in a dose-dependent fashion but did
not significantly alter VRBC. Saline infusion
did not significantly alter capBV, VRBC, or
femoral artery blood flow. We conclude that physiological changes in
skeletal muscle capillary perfusion can be assessed in vivo with the
use of contrast-enhanced ultrasound. Exercise increases both
VRBC and capBV, whereas hyperinsulinemia
selectively increases only capBV, which may enhance skeletal muscle
glucose uptake.
blood volume; capillaries; insulin
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INTRODUCTION |
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THE NUMBER OF PERFUSED CAPILLARIES (Ncap) in skeletal muscle can change in response to various physiological stimuli. Increases in Ncap during skeletal muscle exercise are thought to enhance capillary surface area for oxygen exchange and to decrease oxygen diffusion distance (4, 6, 7). Similarly, it has been proposed that insulin increases Ncap, thereby enhancing glucose delivery to skeletal muscle by augmenting surface area for diffusion. Experimental evidence for insulin-mediated changes in microvascular perfusion in humans has been based largely on increases in limb blood flow and skeletal muscle blood volume that occur in response to hyperinsulinemia (1, 3, 12, 14, 17). The extent of capillary recruitment in skeletal muscle remains uncertain because previous studies have used techniques that provide a measure of total blood volume, most of which resides in larger conduit and resistance vessels (16). Hence, capillary responses to various physiological stimuli have been difficult to assess in intact skeletal muscle due to a paucity of noninvasive methods capable of quantifying capillary blood volume (capBV).
Recently, changes in myocardial and renal capBV have been measured with the use of contrast-enhanced ultrasound imaging (2, 22, 23). This technique also provides information on microbubble velocity within capillaries by measuring their reappearance rate in tissue after their destruction with acoustic energy (2, 22). Because the microvascular rheology of microbubbles is similar to that of red blood cells (8), this method can be used to study microvascular red blood cell velocity (VRBC) (22). In this study, we used contrast-enhanced ultrasound to noninvasively assess changes in capBV and VRBC in skeletal muscle during contractile work and physiological hyperinsulinemia. Microvascular volume changes measured by contrast-enhanced ultrasound were compared with those made by endothelial xanthine oxidase activity, which reflects capillary surface area (18, 25). The primary purpose of the study was to assess insulin-mediated changes in the volume and velocity of blood in the small microvessels in skeletal muscle, since these changes have previously been evaluated using methods that largely reflect total blood volume. A second goal of these studies was to establish a noninvasive method that may potentially be used to rapidly assess skeletal muscle microvascular responses in patients.
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METHODS |
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Animal preparation. The study protocol was approved by the animal research committee at the University of Virginia. Twenty-two male Sprague-Dawley rats (230-280 g) were anesthetized with pentobarbital sodium (50 mg/kg), and body temperature was maintained with a heating lamp. Catheters were placed in a carotid artery for blood pressure monitoring and blood sampling and in both jugular veins for administration of insulin, glucose, and microbubbles. An ultrasonic flow probe connected to a flowmeter (T106, Transonics) was placed on the exposed femoral artery of the study hindlimb.
Contrast-enhanced ultrasound.
The adductor magnus and semimembranosus muscles of the hindlimb were
imaged in short axis with a linear-array transducer connected to an
ultrasound system (L7-4 transducer, HDI-5000, ATL Ultrasound). Pulse inversion imaging was performed at a centerline transmission frequency of 3.3 MHz. The mechanical index [(peak acoustic
pressure) × (frequency)1/2], a measure of acoustic
power, was set at 0.9 to destroy and image microbubbles with the same
pulse (22). The acoustic focus was placed at the midmuscle
level, and gain settings were optimized and held constant throughout
the experiment. Data were recorded on 1.25-cm videotape by use of a
S-VHS recorder (Panasonic MD830, Matsushita Electric).
In vitro characterization of the acoustic beam profile. In vitro experiments were designed to 1) confirm complete microbubble destruction with the ultrasound settings used in the in vivo experiments and 2) calculate the beam elevation at the acoustic focus. The latter information was used to determine the blood velocity of vessels eliminated from analysis by performing background subtraction with frames obtained at a PI of either 0.05 or 1 s. A segment of canine jugular vein was attached at either end to polyethylene tubing and immersed in a water bath. One section of tubing was placed in a calibrated roller pump (EP-1, Bio-Rad), and a reservoir was connected to the end of the tubing. The ultrasound transducer was placed in the water bath and oriented to image the vein in short axis with identical imaging parameters as in the in vivo experiments.
Initial images were recorded during infusion of 0.9% saline. A suspension of Optison (5×104 mlEndothelial xanthine oxidase activity.
Capillary xanthine oxidase activity, measured by single-pass metabolism
of 1-methylxanthine (1-MX) to 1-methylurate, was used to assess changes
in capillary surface area (18, 25). Allopurinol (10 µmol/kg) was administered intravenously to partially inhibit xanthine
oxidase 5 min before a continuous intravenous infusion of 1-MX (0.4 mg · kg1 · min
1) was begun
(18). Whole blood (300 µl) was obtained from the carotid
artery and femoral vein and immediately centrifuged. Plasma (100 µl)
was separated and added to 20 µl of 1 M perchloric acid and 12 µl
of 2.5 M K2CO3. Plasma concentrations of 1-MX
and oxypurinol (reflecting allopurinol concentration) were measured
using reverse-phase high-performance liquid chromatography (model
600E/486, Waters Technologies), as previously described, by use of a
linear gradient elution technique (18, 24). The rate of
1-MX metabolism was calculated by the product of femoral artery blood
flow and arteriovenous difference of 1-MX concentration.
In vivo protocol.
The experimental protocol is shown schematically in Fig.
1. One hour after surgical preparation,
baseline hemodynamics and femoral blood flow were recorded, and
contrast-enhanced ultrasound of the adductor muscles was performed.
These measurements were repeated just before completion of a 2-h
infusion of either normal saline (n = 6), low-dose
insulin (3 mU · kg1 · min
1;
n = 6), or high-dose insulin (40 mU · kg
1 · min
1;
n = 4) while systemic euglycemia was maintained
(18). Arterial and femoral venous blood samples were
collected for measurement of glucose uptake. In the six saline-treated
animals, electrodes were placed into the adductor tendons and connected
to a pulse generator (5345, Medtronic). Muscles were stimulated at 2 Hz
using 5- to 7-mA monophasic square-wave pulses 1 ms in duration.
Hemodynamics and femoral blood flow were recorded, and contrast
ultrasound was performed 2-3 min after initiation of
electrostimulated contraction. In six separate animals, measurement of
capillary endothelial surface area by 1-MX metabolism was performed
after a 2-h infusion of saline and repeated 2-3 min after
initiation of stimulated contractile exercise.
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Statistical analysis. Data are expressed as means ± SD. Comparisons were made by using Student's t-test (paired and unpaired) and repeated-measures ANOVA. Data were considered significant at P < 0.05 (two sided).
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RESULTS |
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Characterization of the acoustic beam.
Contrast-enhanced ultrasound images and video intensity data from the
vessel lumen in the in vitro experiment are illustrated in Fig.
2. The mean video intensity measured
during infusion of microbubbles while imaging at PI of 50 ms (20 Hz)
was similar to that measured before contrast infusion (14 ± 4 vs.
14 ± 3), confirming complete microbubble destruction with the
ultrasound settings used in this study. During infusion of
microbubbles, video intensity increased progressively with prolongation
of the PI until an interval of ~1.5 s was reached. The relation
between PI and video intensity was slightly curvilinear due to laminar rather than plug flow (Fig. 2). The beam elevation at the acoustic focus was estimated to be 2.4 mm by the product of flow velocity in the
vein (1.6 mm/s) and the estimated time required to completely refill
the ultrasound elevation (1.5 s). On the basis of these measurements,
we assumed that background subtracting-averaged frames acquired during
continuous imaging at a frame rate of 20 Hz in the in vivo protocols
would completely exclude from analysis vessels with a mean velocity
greater than ~4.8 × 102 m/s (calculated by
dividing the elevation by 0.05 s). These velocities are
characteristic for arterioles that are greater than ~100 µm in
diameter, although there is significant heterogeneity in the velocity-diameter relation (5). Similarly, use of images
acquired at a PI of 1 s as background would exclude vessels with a
mean velocity greater than ~2.4 × 10
3 m/s, which
eliminates signal from almost all noncapillary microvessels, as well as
a fraction of the capillary signal (4, 5, 7).
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Effect of exercise and insulin on capillary perfusion.
In the in vivo studies, mean heart rate and arterial blood pressure did
not vary significantly in the different treatment groups. Compared with
baseline measurements, saline infusion did not alter skeletal muscle
microvascular blood volume (measured using 20 Hz imaging as
background), VRBC, or femoral artery blood flow
(Fig. 3). In these same animals,
stimulated contractile exercise produced an approximately twofold
increase in microvascular blood volume and a fivefold increase in mean
VRBC, accounting for a marked increase in
femoral artery blood flow (Fig. 3). Examples of contrast-enhanced
ultrasound images from the hindlimb adductor muscles and corresponding
PI vs. video intensity curves from a rat at baseline and during
contractile exercise are illustrated in Fig.
4. Compared with baseline, contractile
exercise resulted in a more rapid rate constant ( values of 0.10 vs.
0.45) and a higher plateau video intensity (A values of 6.1 vs. 14.1), indicating greater VRBC and
microvascular blood volume, respectively.
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Effect of exercise on 1-MX metabolism.
Changes in microvascular blood volume measured by contrast-enhanced
ultrasound were compared with changes in microvascular endothelial
surface area, measured by activity of xanthine oxidase present in
capillary endothelial cells. These comparisons were made in animals
undergoing contractile exercise. Arterial oxypurinol concentrations at
baseline and after initiation of contractile exercise were not
significantly different (8.6 ± 2.2 vs. 10.0 ± 1.6).
Increases in capillary surface area, measured by 1-MX metabolism, in
animals undergoing exercise were similar to increases in microvascular
blood volume determined by contrast-enhanced ultrasound (Fig.
8).
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DISCUSSION |
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Contrast-enhanced ultrasound imaging performed during a steady-state blood pool concentration of microbubbles provides information on the two primary components of microvascular perfusion, VRBC and microvascular blood volume (22). Assessment of these parameters as a means to quantify myocardial and renal perfusion has been explored with contrast-enhanced ultrasound in animal models (2, 22, 23) and in humans (13, 15). In the present study, we have demonstrated for the first time that physiological changes in skeletal muscle VRBC and capBV can be assessed in vivo with the use of contrast-enhanced ultrasound imaging.
During skeletal muscle work, large increases in oxygen consumption must at least partially be met by increased red cell flux through tissue because enhancement of oxygen extraction is limited (4, 6, 7, 10, 19). Increased red cell flux can be achieved by increasing capillary VRBC. Electrically stimulated muscle contraction has been shown in animal models to increase VRBC in skeletal muscle by >300% (4, 6, 20). However, the methods used to measure these changes are complex and too invasive to be applied in human studies. In the current study, we noninvasively assessed skeletal muscle VRBC during contractile exercise with the use of contrast-enhanced ultrasound and found changes comparable to those found previously (4, 20). Increases in flow can also occur by increasing Ncap, which may also serve to decrease oxygen diffusion distance. Muscle stimulation similar to that used in our study has been shown to increase Ncap by 35-100% depending on whether intravital microscopy or freeze-clamp histology techniques were used (4, 6, 7, 20). In the present study, changes in capBV measured with contrast-enhanced ultrasound suggest that the extent of capillary recruitment in response to exercise may even exceed 100%.
Increases in skeletal muscle blood flow may also occur in response to
hormonal stimuli such as hyperinsulinemia (1, 3, 12, 14, 17,
18). The vasoactive properties of insulin may facilitate glucose
delivery to skeletal muscle, which is responsible for >80% of glucose
disposal. On the basis of Renkin models of homogeneous capillary flow
and limited endothelial glucose permeability, increases in
VRBC would be expected to have a minimal effect
on glucose disposal, since the glucose diffusion capacity of individual capillaries can be enhanced only to a small degree (3,
11). Alternatively, changes in capillary density would have a
much greater impact on skeletal muscle glucose disposal, because uptake is governed more by capillary surface area than by capillary
permeability (3). In accord with these concepts, we
observed that physiological hyperinsulinemia (low-dose infusion of 3 mU · kg1 ·min
1 in the rat)
(21) did not alter VRBC but did
increase capBV to a similar extent as did exercise. Moreover, greater
increases in capBV in response to high-dose supraphysiological compared with physiological insulin were associated with an augmentation in
skeletal muscle glucose uptake.
The insulin-mediated increases in capBV measured in the current study exceed muscle blood volume changes estimated by multicompartment indicator-dilution models (3) or by positron emission tomography (12, 17). Although these techniques have provided valuable insight into the vascular actions of insulin, they are somewhat limited by their inability to resolve microvascular blood volume alone. Indicator-dilution models estimate total extracellular volume, whereas positron emission tomography measures changes in total vascular rather than microvascular blood volume. Accordingly, the extent of capillary recruitment may be underestimated by these techniques, because only one-half of the blood volume in resting skeletal muscle resides in microvessels, of which only approximately one-half of vessels <200 µm is in capillaries (16).
In this study, we were able to eliminate signal from larger vessels by exploiting the blood velocity gradient from large to small vessels. Elimination of signal from larger vessels was not necessary in previous studies using myocardial contrast echocardiography because the vast majority of the myocardial microvascular volume at rest resides in the capillaries (9). Results from the in vitro protocol indicated that digitally subtracting frames obtained at a PI of 0.05 s eliminated signal from vessels with a velocity greater than ~48 mm/s, characteristic of vessels that are larger than ~100 µm (5, 26). Analysis was also performed by background-subtracting images obtained at a PI of 1 s, which completely eliminated vessels with a velocity >2.4 mm/s, thus eliminating signal from most noncapillary vessels. In insulin-treated animals, background-subtracting frames at the longer PI resulted in only small changes in the blood volume, represented by the mean A value, which is expected since the majority of blood volume in <100-µm microvessels resides within the capillary compartment (16). Accordingly, changes in blood volume during insulin infusion, regardless of dose, were similar in extent when capBV and total microvascular blood volume was observed. In saline-treated animals, background-subtracting frames obtained at a PI of 1 rather than 0.05 s significantly decreased the mean A value only during exercise, resulting in a lower calculated percent change in capBV compared with total microvascular blood volume. This difference was most likely due to a marked increase in VRBC during exercise, which would increase capillary signal at a PI of 1 s and, hence, would eliminate a greater proportion of the capillary signal. Therefore, the 1.5-fold increase in capBV with exercise calculated using a PI of 1 s as background probably slightly underestimated the true increase in Ncap.
To determine whether changes in the A value reflected changes in microvascular blood volume, we compared data obtained by contrast-enhanced ultrasound with measurements of capillary endothelial xanthine oxidase activity, an independent measure of microvascular surface area. Contrast ultrasound data on microvascular blood volume were used because we had reason to believe that capBV data might have slightly underestimated changes in Ncap. The extent of microvascular blood volume changes by the two techniques was similar, although these comparisons were limited by the technical inability to make both measurements simultaneously in the same animals.
Contrast-enhanced ultrasound can also provide a quantitative measure of
microvascular blood flow by the product of capBV and VRBC (or A · )
(22). In this study, we determined that exercise- or
insulin-mediated increases in microvascular blood flow calculated in
this manner were greater than changes in femoral artery blood flow. One
likely explanation for this discrepancy is that the femoral artery
supplies other hindlimb tissues not affected by adductor exercise or
hyperinsulinemia. In insulin-treated animals, this finding is also
congruent with the previously proposed notion that insulin-mediated
increases in capillary perfusion can result from a redistribution of
blood flow from "nonnutritive" to "nutritive" vascular pathways
within muscle (18). The concept of flow redistribution within the muscle or different tissue components of the hindlimb is
further supported by the lack of further increases in femoral artery
blood flow for high- compared with low-dose insulin, despite further
increases in CapBV and microvascular blood flow.
We believe that the results of the current study offer important insight into the controversial topic of the relation between the vascular and metabolic actions of insulin. The microvascular effect of insulin to recruit capillaries in skeletal muscle, which may have been underestimated in previous studies, may be more critical to substrate exchange and glucose disposal than changes in total blood flow. This issue will likely be solved only by detailed analysis of the relationship between capillary perfusion and substrate exchange in muscle in response to insulin.
In summary, this is the first study to quantify changes in skeletal muscle perfusion with contrast-enhanced ultrasound. This noninvasive imaging technique may potentially be applied to assess metabolic regulation of skeletal muscle perfusion and responses to physiological stimuli in humans. Moreover, it may prove valuable for studying abnormal skeletal capillary responses in metabolic disorders, such as glucose intolerance and diabetes, and muscle-wasting diseases in humans.
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ACKNOWLEDGEMENTS |
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This study was supported by Grants HL-03810 (to J. R. Lindner) and HL-48890 (to S. Kaul) from the National Institutes of Health, Bethesda, Maryland; a Beginning Grant-in-Aid (J. R. Lindner) from the American Heart Association, Mid-Atlantic Affiliate, Baltimore, Maryland; a grant from the American Diabetes Association (to E. J. Barrett, M. A. Vincent, and A. Clarke), Alexandria, VA; a grant from the Soros Foundation (to D. Dawson); and an equipment grant from ATL Ultrasound, Bothell, WA.
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FOOTNOTES |
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Address for reprint requests and other correspondence: J. R. Lindner, Box 800158, Cardiovascular Division, Univ. of Virginia Medical Center, Charlottesville, VA 22908 (E-mail: jlindner{at}virginia.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.
10.1152/ajpendo.00373.2001
Received 16 August 2001; accepted in final form 7 November 2001.
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