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Department of Biomedical Engineering, Graduate School of Medicine, University of Tokyo, Tokyo 113-0033, Japan
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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To clarify the transport of O2 across the microvessels in skeletal muscle, we designed an intravital laser microscope that utilizes a phosphorescence quenching technique to determine both the microvascular and tissue PO2. After we injected the phosphorescent probe into systemic blood, phosphorescence excited by a N2-dye pulse laser was detected with a photomultiplier over a 10 µm in diameter area. In vitro and in vivo calibrations confirmed that the present method is accurate for PO2 measurements in the range of 7-90 Torr (r = 0.958) and has a rapid response time. This method was then used to measure the PO2 of microvessels with different diameters (40-130 µm) and of interstitial spaces in rat cremaster muscle. These measurements showed a significant drop in PO2 in the arterioles after branching (from 74.6 to 46.6 Torr) and the presence of a large PO2 gradient at the blood-tissue interface of arterioles (15-20 Torr). These findings suggest that capillaries are not the sole source of oxygen supply to surrounding tissue.
oxygen transport; intravital microscope; microcirculation; palladium-porphyrin; cremaster muscle
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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ALTHOUGH RESEARCHERS HAVE KNOWN for over 100 years that one of the principal functions of the microcirculation is O2 delivery to tissues (19, 20, 28), our understanding of the processes involved in the transport of O2 from blood to tissue is incomplete (6, 9, 14). A major problem is that we do not know how PO2 levels in microvessels and tissues vary, particularly in the vicinity of blood vessels and around individual cells. Several methods have been utilized in efforts to measure these parameters. Recent progress in O2 microelectrodes (17, 30), which are currently the most widely used and successful method, has produced many advantages in numerous physiological studies because of the rapid time response and wide range of PO2 measurements these microelectrodes make possible (1, 40, 41). However, the microelectrodes must be inserted into the tissue, disturbing the local environment. Optical methods using spectrophotometry and O2 indicators, such as hemoglobin or myoglobin, have also been utilized (3, 4, 7, 24, 37). These methods allow noninvasive and reliable measurements to be performed, but only when the signals of interest have a homogeneous distribution. In addition, these methods cannot simultaneously measure the PO2 of blood and tissue, and these parameters are probably necessary for complete analysis of O2 delivery to tissues surrounding the microvessels.
In the last decade, methods involving the O2-dependent quenching of fluorescence or phosphorescence (2, 23, 27, 38, 46) have undergone considerable improvement, and several successful measurements of microvascular and interstitial PO2 values in normal tissues (15, 16, 32, 44) and tumors (34, 43) have been made. In addition, this technique has been used to measure microvascular and interstitial PO2 gradients in rat mesentery (35, 45) and hamster skin (33) to clarify the distribution of O2 on the order of a micrometer. However, these measurements have only been performed in thin tissues, and only a few reports have been made of microvascular and interstitial PO2 measurements in thick tissues like skeletal muscle (46). The reason for this is that, with incident light using a conventional excitation like a xenon flash lamp, it is difficult to excite the phosphorescent probe in a limited volume. Thus the light cannot penetrate deeper tissues because it is absorbed and scattered.
In a previous study (29), we reported on the development of a fluorescence intravital microscope equipped with a laser illuminator. The use of the laser illuminator allows deeper tissues to be penetrated, enabling tomographic observations of the microcirculation in thicker tissues. Herein, we report the development of a new phosphorescence quenching microscope based on the laser illuminator technique that allows noninvasive and regional determination of intravascular and interstitial PO2 values in skeletal muscle.
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MATERIALS AND METHODS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Animal preparation. Adult male Wistar rats weighing between 150 and 180 g were anesthetized with urethane intramuscularly (1 g/kg body wt), and a tracheotomy was performed to facilitate spontaneous breathing. The carotid artery was cannulated so that the arterial blood pressure could be measured. The jugular vein was also cannulated, facilitating injection of the intravascular phosphorescence probes and supplementary doses of anesthetic. The cremaster muscle, having a thickness of 200-400 µm, was spread out in a special bath chamber with an optical port for transillumination, and the surface of the cremaster muscle was suffused with a 37°C Krebs solution with 5% CO2 in 95% N2, adjusted to pH 7.3-7.4. After a 30-min equilibration period, the suffusion was stopped and a coverslip was placed on the cremaster muscle to prevent dehydration and hyperoxia. Under these conditions, tissue PO2 levels might be less than those in the physiological range because the tissue PO2 falls to 10 Torr during suffusion with 0% solution (10, 22). All animals in which the mean arterial pressure fell to <70 mmHg during the experiment were excluded.
The PO2 measurements were performed at several locations in the rat cremaster muscle (Fig. 1). Arterioles and venules were classified according to their branching order in the microscopic field. Large arterioles with a diameter of ~80-120 µm branching from the central cremasteric artery were designated as first order (A1). Branches of first-order arterioles were designated as second order (A2, 50-80 µm in diameter). Third-order arterioles (A3) had a diameter of <60 µm and branched from second-order arterioles. Venules were also classified by their branching order. The large venules entering the central cremasteric vein were designated as first order (V1, 80-130 µm in diameter) and so on. The diameters of the second-order (V2) and third-order (V3) venules were ~60-100 µm and <60 µm, respectively. PO2 measurements in the interstitial spaces were performed in two places. The first position was closed within 20 µm from the arterial wall, but the illumination spot (10 µm in diameter) did not come in contact with the luminal surface of the vessel. The second position was more than 100 µm away from the arteriole.
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PO2 determination.
Microvascular and interstitial PO2 were
measured using the O2-dependent quenching of
phosphorescence decay technique (23, 38, 42).
Pd-meso-tetra(4-carboxyphenyl)porphyrin (Pd-porphyrin, Porphyrin
Products, Logan, UT) bound to bovine serum albumin was used as the
phosphorescent probe for the O2-dependent quenching. The
basis of this technique is a well-known reaction in which Pd-porphyrin
is excited to its triplet state by exposure to pulsed light, after
which phosphorescence intensity is reduced by emission and energy
transfer to O2. The quenching of the phosphorescence by the
O2 is diffusion limited. Thus, if the
PO2 distribution is homogeneous, it can be
described as
![I(<IT>t</IT>)<IT>/</IT>I<SUB>0</SUB><IT>=</IT>exp [−(1<IT>/&tgr;</IT><SUB>0</SUB><IT>+K</IT><SUB>q</SUB><IT>×</IT>P<SC>o</SC><SUB>2</SUB>)<IT>t</IT>]<IT>=</IT>exp (<IT>−t/&tgr;</IT>)](/content/vol91/issue1/fulltext/321/img001.gif)
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(1) |
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(2) |
0 and are the phosphorescence lifetimes
in the absence of O2 and in the area being measured,
respectively, and Kq is the quenching constant.
The PO2 values can be obtained from the
measurement of , because Kq and
0 are substance specific. However, Golub et al.
(11) pointed out that the rectangular distribution model
should be used to analyze the data when the PO2
distribution is heterogeneous in the measuring area. The fitting equation they proposed is
![I(<IT>t</IT>)<IT>/</IT>I<SUB>0</SUB><IT>=</IT>exp [−(1<IT>/&tgr;</IT><SUB>0</SUB><IT>+K</IT><SUB>q</SUB><IT>×</IT>P<SC>o</SC><SUB>2</SUB>)<IT>t</IT>]<IT>×</IT>[1<IT>+</IT>(<IT>K</IT><SUB>q</SUB><IT>&sfgr;t</IT>)<SUP>2</SUP><IT>/</IT>2]](/content/vol91/issue1/fulltext/321/img003.gif)
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(3) |
Phosphorescence quenching laser microscope.
Figure 2 shows a schematic diagram of the
system used in this study. The bath chamber containing the cremaster
muscle was placed on a three-way movable stage equipped with a 20-W
halogen lamp for transillumination. A general observation of the
microcirculation was performed using a modified Nikon microscope with a
×20 long-working-distance dry objective (CF Plan 20×/0.40 EPI ELWD,
Nikon, Tokyo). The microcirculation was filmed using a charge-coupled
device (CCD) camera (DXC-107A, Sony, Tokyo) connected to a videotimer
(VTG-33, For-A, Tokyo, Japan) and videocassette recorder (SLV-RS1,
Sony), and the image was displayed on a 14-in. high-resolution
television monitor (PVM-1442Q, Sony) at a final magnification of
approximately ×800. The Pd-porphyrin phosphorescent probe was excited
by epi-illumination using a N2-dye pulse laser (LN120C,
Laser Photonics) with a 535-nm line at 20 Hz via the objective lens.
The average optical power and pulsewidth of the laser were 1.2 mW and
300 ps, respectively. The area of the epi-illuminated tissue was 10 µm in diameter on the surface. The phosphorescent emissions from the
tissue were captured by a photomultiplier (C6700, Hamamatsu Photonics,
Hamamatsu, Japan) through a long-pass filter at 610 nm. Signals from
the photomultiplier were converted to 10-bit digital signals at
intervals of 3 µs. The averaged 20-40 data were calculated by
mathematically fitting the decay of the phosphorescence to the
rectangular model equation (11) using online computer
analysis. Intravascular PO2 measurements were
carried out immediately, whereas interstitial
PO2 measurements were started 30 min after
injection of the Pd-porphyrin solution (~25 mg/kg body wt) into the
cannulated jugular vein. In the measurements of interstitial
PO2, Pd-porphyrin solution injection was
adjusted to the magnitude of the photomultiplier signal and equivalent in changing the sensitivity of the photomultiplier at three to four
times.
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In vitro and in vivo calibration.
The values of the phosphorescent probe at various
PO2 levels were measured in vitro to obtain
0 and Kq for the present system
because these values depend on pH and temperature. In vitro calibration
was carried out to keep the temperature of the phosphorescent probe at
37°C and the pH at 7.3-7.4, at which the probe solution was
stationary during measurement. The in vitro value of the phosphorescent probe as a function of PO2 is
shown in Fig. 3. The values of
0 and Kq calculated from
this result were 545 µs and 362 Torr
1 · s1, respectively. These
values were used for all PO2 calculations in
this study.
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Statistics. All data are means ± SD. Order-related differences were analyzed using a one-way ANOVA and multiple comparisons test. For all statistical tests, a P value of <0.05 was considered significant.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Systemic arterial PO2, PCO2, and pH were measured using a blood analysis system (Series 2000, Diametrics Medical, St. Paul, MN) in samples from the carotid arteries of four rats. Arterial PO2 averaged 98.1 ± 12.9 Torr, whereas arterial PCO2 and pH averaged 48.7 ± 9.2 Torr and 7.32 ± 0.05, respectively.
A typical example of a digitized phosphorescence decay curve measured
in the interstitial space of the rat cremaster muscle is shown in Fig.
5. The symbols indicate the original
data, whereas the solid line represents the theoretical curve fitted to
the original data. This curve was obtained from the average of 20 curves. These results show clearly that the phosphorescence decay curve
is virtually equal to the theoretical curve. In addition, the
application of the pulse laser illuminator enables the phosphorescence quenching curve to be quickly detected in the initial segment by
excluding the afterglow produced by incidental light. In this example,
the calculated values of and PO2 were 87 µs and 26.7 Torr, respectively.
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Table 1 summarizes the results of the
statistical analysis on data from four animal experiments. The mean
arteriolar PO2 values of the different
arteriole orders decreased significantly after branching, but the
venular PO2 showed no dependency on vessel order. Mean PO2 values in the interstitial
spaces adjacent to the arterioles of different orders were
significantly lower than intravascular PO2
values. In addition, PO2 values measured in the
interstitial spaces at a distance of more than 100 µm from the
arterioles showed no significant differences with respect to vessel
order, although their values were significantly lower than the
PO2 values at locations adjacent to the
arterioles. Figure 6 shows the
PO2 profile for the data in Table 1. The
systemic arterial PO2 value, which is
significantly higher than that of the A1 arteriole, is also indicated
in Fig. 6. A large drop in PO2 across the
blood-tissue interface followed by a gentle decrease is clearly
demonstrated for every order of arteriole.
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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O2-dependent quenching of phosphorescence has proven to be a powerful method for measuring the PO2 of tissues in living animals because it allows rapid and noninvasive measurements to be performed. However, to determine PO2 values using in vivo measurements obtained by the phosphorescence quenching technique, the heterogeneous distribution of PO2 in the measuring area always becomes a large problem (8, 21). In an effort to resolve this problem, many researchers have proposed an effective algorithm for analyzing a heterogeneous system (39, 46). These investigations generally encourage the use of multiexponential analysis because the phosphorescence decay curve in a heterogeneous system consists of several exponents. On the other hand, Golub et al. (11) proposed the continuous distribution model, in which the fitting procedure based on this model can result in more accurate values than other methods, for determining PO2 values in a heterogeneous system. However, both investigations suggested that measurement accuracy depends on the volume of the detection area. In this study, a 535-nm N2-dye pulse laser was used to excite the phosphorescent probe through a long-working-distance objective lens. This optical arrangement enabled the phosphor in a limited volume to be excited for short time (1-2 s).
Buerk et al. (2) reported direct comparison of tissue PO2 measurement in hamster skinfold preparations using the phosphorescence quenching technique with microelectrodes. The major difference in the optical arrangement between their system and ours is the lighting source. They used a xenon strobe lamp with an optical window for detecting the phosphorescence emission in a limited area (10 × 10 µm), whereas our system was equipped with a N2-dye pulse laser. They found that there was no significant difference between the optical and microelectrode tissue PO2 measurements and that there was no significant depletion of O2 during excitation of the phosphor (3 s). Consequently, our measurements, made under similar conditions, suggest that, even though the fluid movement in the interstitial space was slow, the photoactivated consumption of O2 might have had a minimal effect on our data.
In the last decade, the phosphorescence quenching technique has been substantially improved and applied to in vivo measurements by several investigators (38, 44). Torres Filho et al. (33) reported on the intravascular PO2 gradients in arterioles and venules of different orders in a hamster skin preparation. In addition, Tsai et al. (35) reported on the distribution of PO2 in the microvessels and interstitial spaces of a rat mesentery preparation. However, both of these investigations used thin preparations. Only a few reports have been made of intravascular and interstitial PO2 measurements in skeletal muscle using the phosphorescence technique (46) because skeletal muscle is generally too thick for the phosphorescent probe to be excited by the xenon flash lamp that is usually used in this method. In this study, a 535-nm N2-dye pulse laser was used to excite the phosphorescent probe through a long-working-distance objective lens. This optical arrangement might anticipate the application of the PO2 measurement in the deeper tissue.
In a previous study from our laboratory (29), we evaluated the divergence of the incident light in tissue as a result of light scattering and absorption when a laser illuminator was used to excite a fluorescent probe in rabbit tenuissimus muscle. Our results indicated that, at tissue depths of 100 and 200 µm below the surface, the intensity of the incident light was at least 50 and 30%, respectively. Moreover, each augmentation was no more than 1.7-2.5 times wider. Pulse laser can also be used to excite the phosphorescent probe in regions where the PO2 is higher than 100 Torr and the lifetime of Pd-porphyrin is shorter than 30 µs. With a xenon flash lamp, the decay in the light from the xenon flash remains for the first 30 µs of the phosphorescence decay curve (32). Thus high PO2 values cannot be measured.
A significant drop in the PO2 levels of different order arterioles was found (see Table 1). Similar levels of decrease in PO2, including the longitudinal PO2 gradient in arterioles, were also found by many investigators (6, 9, 21, 31). For instance, in hamster skin arterioles, a similar tendency was reported by Torres Filho et al. (33), although the arterioles in their study were smaller than those in the present study. The PO2 values of A1, A2, and A3 in our results were 74.6, 54.4, and 46.6 Torr, respectively. These values are higher than the data for skin (A1, 51.8; A2, 44.1; A3, 39.9 Torr). However, the systemic arterial PO2 value in our preparation (98.1 Torr) was also much higher than that of the skin preparation (71.1 Torr). These differences may be due to the poorer respiratory gas exchange of hamsters relative to that of rats and/or the organ specificity. When arteriolar PO2 values for vessels with a similar diameter were compared, our A2 and A3 PO2 values were consistent with the A1 and A2 PO2 values in the skin. In addition, the PO2 value of the venules (31.3 Torr) was consistent with the venular PO2 value in the skin (30.8 Torr).
In this study, a significant reduction in the PO2 level was found at the interface between the blood vessels and the tissue as shown in Fig. 6. A similar PO2 gradient has been reported for rat mesenteric arterioles (35). The interstitial PO2 values adjacent to the A1, A2, and A3 arterioles were 50.7, 39.4, and 28.8 Torr, respectively. These values are 15-20 Torr lower than the PO2 values in each arteriole. These findings, and a significant drop in the PO2 levels of different order arterioles as was stated previously, strongly support the view that capillaries are not the sole source of O2 supply to surrounding tissue. These phenomena are with the hypothesis that the intravascular O2 flux is facilitated by a high diffusion constant (26) and/or they are due to high O2 solubility in tissue (25). In contrast, a possibility remains that there is a high rate of O2 consumption in the vessel walls (14) because O2 consumption decreased by 34% when the endothelium was removed from the hindlimb of a dog (5). More recently, Vadapalli et al. (36) predicted that some other extramitochondrial pathways are associated with O2 utilization. Further study is necessary to clarify these phenomena.
PO2 levels in the interstitial spaces at points near and far from the arterioles were significantly different (see Table 1). The interstitial PO2 values adjacent to the A1, A2, and A3 arterioles were significantly higher than the interstitial PO2 values located farther away (10-13 Torr). It is difficult to compare these values with those of other reports using different preparations and measurement techniques because the area of measurement depends on the microvascular arrangement. For instance, in the hamster skin preparation in which the photoquenching technique was used to obtain measurements, interstitial PO2 values were between 11 and 36 Torr (33). However, in the hamster cremaster muscle measurement using microelectrodes, the tissue PO2 values were between 14 and 17 Torr (12). In addition, using the same preparation and the same technique, the mean tissue PO2 value was lowered still further (11-15 Torr) under superfusion with a low PO2 solution (18). In our experiment, the muscle surface was suffused with 0% O2 solution before PO2 measurement, and then the suffusion was stopped and a coverslip was placed on the muscle surface during PO2 measurement. Consequently, no O2 supply from room air through the coverslip may be one of the causes of low interstitial PO2 values. In addition, the relatively high temperature of suffusate (37°C) in our experiment may have induced high metabolic activity in the tissue. Otherwise, the differences between our values and those reported before are likely due to the differences in tissue metabolism between rats and hamsters.
This study has shown that the phosphorescence quenching laser microscope can be used to clarify the transport of O2 across microvessels and the distribution of O2 in tissues, although more regional data on PO2 values in tissues are required at the present. The use of lasers to excite phosphorescent probes enables a smaller area of tissue to be illuminated (<10 µm) if the potential for tissue damage is clarified in detail. In addition, intracellular measurements of PO2 will require the phosphorescent probe to penetrate the cell membrane.
In conclusion, a new intravital microscope has been designed that utilizes O2-dependent phosphorescence quenching. This microscope may feasibly be applied to studies for O2 transport across microvessels and the distribution of O2 in skeletal muscle. In addition, we found a large reduction in PO2 levels of different order arterioles as well as a large PO2 gradient at the interface between blood and tissue. These findings suggest that capillaries are not the sole source of oxygen supply to surrounding tissue.
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ACKNOWLEDGEMENTS |
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The authors thank M. Yamada for kind assistance.
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FOOTNOTES |
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This work was supported by a Grant-in-Aid for Scientific Research (11558103) from the Ministry of Education, Science, and Culture, Japan, and a grant from the Research for the Future Program (97100401) of the Japan Society for the Promotion of Science.
Address for reprint requests and other correspondence: M. Shibata, Dept. of Biomedical Engineering, Graduate School of Medicine, The Univ. of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-0033, Japan (E-mail: shibatam{at}m.u-tokyo.ac.jp).
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.
Received 1 September 1999; accepted in final form 22 February 2001.
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REFERENCES |
|---|
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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1.
Buerk, DG,
and
Nair P.
PtiO2 and CMRO2 changes in cortex and hippocampus of aging gerbil brain.
J Appl Physiol
74:
1723-1728,
1993
2.
Buerk, DG,
Tsai AM,
Intaglietta M,
and
Johnson PC.
Comparing tissue PO2 measurements by recessed microelectrode and phosphorescence quenching.
Adv Exp Med Biol
454:
367-374,
1998[ISI][Medline].
3.
Chance, B,
Dait MT,
Zhang C,
Hamaoka T,
and
Hagerman F.
Recovery from exercise-induced desaturation in the quadriceps muscles of competitive rowers.
Am J Physiol Cell Physiol
262:
C766-C775,
1992
4.
Chance, B,
and
Quistorff B.
Study of tissue oxygen gradients by single and multiple indicators.
Adv Exp Med Biol
94:
331-338,
1977[Medline].
5.
Curtis, SE,
Vallet B,
Winn MJ,
Caufield JB,
King CZ,
Chapler CK,
and
Cain SM.
Role of the vascular endothelium in O2 extraction during progressive ischemia in canine skeletal muscle.
J Appl Physiol
79:
1351-1360,
1995
6.
Duling, BR,
and
Berne RM.
Longitudinal gradients in periarteriolar oxygen tension. A possible mechanism for the participation of oxygen in the local regulation of blood flow.
Circ Res
27:
669-678,
1970
7.
Ellis, CG,
Ellsworth ML,
and
Pittman RN.
Determination of red blood cell oxygenation in vivo by dual video densitometric image analysis.
Am J Physiol Heart Circ Physiol
258:
H1216-H1223,
1990
8.
Ellsworth, ML,
and
Pittman RN.
Evaluation of photometric methods for quantifying convective mass transport in microvessels.
Am J Physiol Heart Circ Physiol
251:
H869-H879,
1986
9.
Ellsworth, ML,
and
Pittman RN.
Arterioles supply oxygen to capillaries by diffusion as well as by convection.
Am J Physiol Heart Circ Physiol
258:
H1240-H1243,
1990
10.
Frisbee, JC,
and
Lombard H.
Elevated oxygen tension inhibits flow-induced dilation of skeletal muscle arterioles.
Microvasc Res
58:
99-107,
1999[ISI][Medline].
11.
Golub, AS,
Popel AS,
Zheng L,
and
Pittman RN.
Analysis of phosphorescence in heterogeneous systems using distributions of quencher concentration.
Biophys J
73:
452-465,
1997
12.
Gorczynski, RJ,
and
Duling BR.
Role of oxygen in arteriolar functional vasodilation in hamster striated muscle.
Am J Physiol Heart Circ Physiol
235:
H505-H515,
1978
13.
Greenbaum, AR,
Etherington PJ,
Manek S,
O'Hare D,
Parker KH,
Green CJ,
Pepper JR,
and
Winlove CP.
Measurements of oxygenation and perfusion in skeletal muscle using multiple microelectrodes.
J Muscle Res Cell Motil
18:
149-159,
1997[ISI][Medline].
14.
Intaglietta, M,
Johnson PC,
and
Winslow RM.
Microvascular and tissue oxygen distribution.
Cardiovasc Res
32:
632-643,
1996[ISI][Medline].
15.
Kerger, H,
Saltzman DJ,
Menger MD,
Messmer K,
and
Intaglietta M.
Systemic and subcutaneous microvascular PO2 dissociation during 4-h hemorrhagic shock in conscious hamsters.
Am J Physiol Heart Circ Physiol
270:
H827-H836,
1996
16.
Kerger, H,
Torres Filho IP,
Rivas M,
Winslow RM,
and
Intaglietta M.
Systemic and subcutaneous microvascular oxygen tension in conscious Syrian golden hamsters.
Am J Physiol Heart Circ Physiol
268:
H802-H810,
1995
17.
Kessler, M,
Harrison DK,
and
Hoper J.
Tissue oxygen measurement techniques.
In: Microcirculatory Technology, edited by Baker CH,
and Nastuk WL.. Orlando, FL: Academic, 1986, p. 391-425.
18.
Klitzman, BK,
Popel AS,
and
Duling BR.
Oxygen transport in resting and contracting hamster cremaster muscle: experimental and theoretical microvascular studies.
Microvasc Res
25:
108-131,
1983[ISI][Medline].
19.
Krogh, A.
The number and distribution of capillaries in muscle with the calculation of the oxygen pressure necessary for supplying the tissue.
J Physiol
52:
409-515,
1919.
20.
Krogh, A.
The Anatomy and Physiology of Capillaries. New York: Hafner, 1959.
21.
Kuo, L,
and
Pittman RN.
Effect of hemodilution on oxygen transport in arteriolar networks of hamster striated muscle.
Am J Physiol Heart Circ Physiol
254:
H331-H339,
1988
22.
Lombard, JH,
and
Duling BR.
Relative importance of tissue oxygenation and vascular smooth muscle hypoxia in determining arteriolar responses to occlusion in the hamster cheek pouch.
Circ Res
41:
546-551,
1977
23.
Longmuir, IS,
and
Knopp JA.
Measurement of tissue oxygen with a fluorescent probe.
J Appl Physiol
41:
598-602,
1976
24.
Pittman, RN.
Microvessel blood oxygen measurement technique.
In: Microcirculatory Technology, edited by Baker CH,
and Nastuk WL.. Orlando, FL: Academic, 1986, p. 367-389.
25.
Pittman, RN.
Influence of microvascular architecture on oxygen exchange in skeletal muscle.
Microcirculation
2:
1-18,
1995[Medline].
26.
Popel, AS,
Pittman RN,
and
Ellsworth ML.
Rate of oxygen loss from arterioles is an order of magnitude higher than expected.
Am J Physiol Heart Circ Physiol
256:
H921-H924,
1989
27.
Rumsey, WL,
Vanderkooi JM,
and
Wilson DF.
Imaging of phosphorescence: a novel method for measuring oxygen distribution in perfused tissue.
Science
241:
1649-1651,
1988
28.
Shibata, M,
and
Kamiya A.
Microcirculatory responses to carotid sinus nerve stimulation at various ambient O2 tension in the rabbit tenuissimus muscle.
Microvasc Res
30:
333-345,
1985[ISI][Medline].
29.
Shibata, M,
Kawamura T,
Sohirad M,
and
Kamiya A.
A new fluorescence microscopy for tomographic observation of microcirculation by using dual-beam slit laser illumination.
Microvasc Res
49:
300-314,
1995[ISI][Medline].
30.
Silver, IA.
Some observations on the cerebral cortex with an ultramicro, membrane-covered, oxygen electrode.
Med Biol Eng
3:
377-387,
1965.
31.
Swain, DP,
and
Pittman RN.
Oxygen exchange in the microcirculation of hamster retractor muscle.
Am J Physiol Heart Circ Physiol
256:
H247-H255,
1989
32.
Torres Filho, IP,
and
Intaglietta M.
Microvessel PO2 measurements by phosphorescence decay method.
Am J Physiol Heart Circ Physiol
265:
H1434-H1438,
1993
33.
Torres Filho, IP,
Kerger H,
and
Intaglietta M.
PO2 measurements in arteriolar networks.
Microvasc Res
51:
202-212,
1996[ISI][Medline].
34.
Torres Filho, IP,
Leunig M,
Yuan F,
Intaglietta M,
and
Jain RK.
Noninvasive measurement of microvascular and interstitial oxygen profiles in a human tumor in SCID mice.
Proc Natl Acad Sci USA
91:
2081-2085,
1994
35.
Tsai, AG,
Friesenecker B,
Mazzoni MC,
Kerger H,
Buerk DG,
Johnson PC,
and
Intaglietta M.
Microvascular and tissue oxygen gradients in the rat mesentery.
Proc Natl Acad Sci USA
95:
6590-6595,
1998
36.
Vadapalli, A,
Pittman RN,
and
Popel AS.
Estimating oxygen transport resistance of microvascular wall.
Am J Physiol Heart Circ Physiol
279:
H657-H671,
2000
37.
Van Beek, JH,
Osbakken MD,
and
Chance B.
Measurement of the oxygenation status of the isolated perfused rat heart using near infrared detection.
Adv Exp Med Biol
388:
147-154,
1996[Medline].
38.
Vanderkooi, JM,
Maniara G,
Green TJ,
and
Wilson DF.
An optical method for measurement of dioxygen concentration based on quenching of phosphorescence.
J Biol Chem
262:
5476-5482,
1987
39.
Vinogradov, SA,
and
Wilson DF.
Phosphorescence lifetime analysis with a quadratic programming algorithm for determining quencher distribution in heterogeneous system.
Biophys J
67:
2048-2059,
1994
40.
Whalen, WJ,
Riley J,
and
Nair P.
A microelectrode for measuring intracellular PO2.
J Appl Physiol
23:
798-801,
1967
41.
Whalen Savoca, J,
and
Nair P.
Oxygen tension measurements in carotid body of the cat.
Am J Physiol
225:
986-991,
1973.
42.
Wilson, DF.
Measuring oxygen using oxygen dependent quenching of phosphorescence: a status report.
Adv Exp Med Biol
333:
225-232,
1993[Medline].
43.
Wilson, DF,
and
Cerniglia GJ.
Localization of tumors and evaluation of their state of oxygenation by phosphorescence imaging.
Cancer Res
52:
3988-3993,
1992
44.
Wilson, DF,
Pastuszko A,
Digiacomo JE,
Pawlowski M,
Schneiderman R,
and
Delivoria-Papadopoulos M.
Effect of hyperventilation on oxygenation of the brain cortex of newborn piglets.
J Appl Physiol
70:
2691-2696,
1991
45.
Yaegashi, K,
Itoh T,
Kosaka T,
Fukushima H,
and
Morimoto T.
Diffusivity of oxygen in microvascular beds as determined from PO2 distribution maps.
Am J Physiol Heart Circ Physiol
270:
H1390-H1397,
1996
46.
Zheng, L,
Golub AS,
and
Pittman RN.
Determination of PO2 and its heterogeneity in single capillaries.
Am J Physiol Heart Circ Physiol
271:
H365-H372,
1996
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