Departments of Medicine, and of Physiology and Cellular Biophysics, College of Physicians and Surgeons, Columbia University; and St. Luke's-Roosevelt Hospital Center, New York, New York 10019
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ABSTRACT |
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Endothelial second messenger responses may contribute to the pathology of high vascular pressure but remain poorly understood because of the lack of direct in situ quantification. In lung venular capillaries, we determined endothelial cytosolic Ca2+ concentration [Ca2+]i by the fura 2 ratioing method. Pressure elevation increased mean endothelial [Ca2+]i by Ca2+ influx through gadolinium-inhibitable channels and amplified [Ca2+]i oscillations by Ca2+ release from intracellular stores. Endothelial [Ca2+]i transients were induced by pressure elevations of as little as 5 cmH2O and increased linearly with higher pressures. Heptanol inhibition of [Ca2+]i oscillations in a subset of endothelial cells indicated that oscillations originated from pacemaker endothelial cells and were propagated to adjacent nonpacemaker cells by gap junctional communication. Our findings indicate the presence of a sensitive, active endothelial response to pressure challenge in lung venular capillaries that may be relevant in the pathogenesis of pressure-induced lung microvascular injury.
pulmonary; endothelium; calcium; hydrostatic pressure
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INTRODUCTION |
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ELEVATION OF LUNG microvascular pressures increases lung fluid leak and thereby predisposes the lung to pulmonary edema, a condition associated with high morbidity and mortality. Although this pathology has been traditionally attributed to the passive effects of high pressure (13, 33), growing evidence implicates inflammation as an active response of the pressure-challenged capillary. This is supported by the presence of inflammatory cells in the bronchoalveolar lavage in hydrostatic and high-altitude pulmonary edema (10, 17, 18, 26) and by our previous finding that pressure induces proinflammatory responses in the lung capillary, as reflected in the expression of leukocyte adhesion receptors (21). These considerations indicate that the lung capillary response to pressure challenge is more complex than previously believed and must be better understood.
Here we consider the question in the context of the endothelial cytosolic Ca2+ concentration ([Ca2+]i). We have shown that increases of the endothelial cell (EC) [Ca2+]i determine P-selectin expression in the lung capillary (21). However, since low-frequency [Ca2+]i oscillations are constitutive in lung capillaries (35), it is important to understand the extent to which the oscillations form a part of the lung response to pathologic stimuli. Pacemaker EC located at capillary branch points generate [Ca2+]i oscillations that propagate along the capillary wall as intercellular Ca2+ waves (35). Because [Ca2+]i oscillations have come under increased scrutiny as inducers of cell signaling pathways (1, 11, 12), we considered the possibility that enhancement of [Ca2+]i oscillations in the capillary wall may constitute a feature of the lung capillary response to pressure elevation.
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MATERIALS AND METHODS |
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Fluorescent probes and drugs. Fura 2-AM (5 µM; Molecular Probes, Eugene, OR), gadolinium (GdCl3, 10 µM) and heptanol (3 mM; Sigma, St. Louis, MO) were diluted in 2% dextran (70 kDa; Pharmacia Biotech, Piscataway, NJ)-1% fetal bovine serum (Gemini Bio-Products, Calabasas, CA) HEPES solution containing 150 mmol/l Na+, 5 mmol/l K+, 1.5 mmol/l Ca2+, and 20 mmol/l HEPES (Calbiochem-Novabiochem, San Diego, CA) at pH 7.4 and osmolarity of 295 mosM.
Lung preparation. Experimental procedures and setup have previously been described (21, 35). In brief, lungs excised from anesthetized Sprague-Dawley rats were continuously pump perfused with 14 ml/min autologous rat blood at 37°C. Lungs were constantly inflated with positive airway pressure of 5 cmH2O. At baseline, pulmonary artery pressure and left atrial pressure (PLA) were adjusted to 10 and 5 cmH2O, respectively. A microcatheter (PE-10; Baxter Diagnostics, McGaw Park, IL) was advanced through the left atrium and wedged in a pulmonary vein, allowing for local infusion of solutions (20, 35). Lungs were positioned on a vibration-free air table. To prevent drying, the surface was superfused with normal saline at 37°C.
Fluorescence microscopy. Our methods for intravital microscopy have been reported (21, 35). Fluorophores were excited by mercury lamp illumination directed through a filter wheel and shutter (Lambda-10; Sutter Instrument, Novato, CA) equipped with filters appropriate for excitation at 340 and 380 nm (340HT15 and 380HT15; Omega Optical, Brattleboro, VT). Fluorescence emission was collected through an ultraviolet-compatible objective (Wplan FL ×40 UV; Olympus America, Melville, NY), dichroic and emission filters (400 DCLPO2 and 510WB40; Omega Optical) by image intensifier (KS1381; Video Scope International, Sterling, VA), and video camera (CCD-72; Dage-MIT, Michigan City, IN), then subjected to digital image analysis (MCID-M4; Imaging Research, St. Catharine's, ON, Canada). Single venular capillaries were viewed at a focal plane corresponding to maximum diameter (12-20 µm).
[Ca2+]i imaging and analysis. EC [Ca2+]i in lung venular capillaries was quantified using our previously described fura 2 ratiometric imaging technique (35). Membrane-permeant fura 2-AM, which deesterifies intracellularly to impermeant fura 2, was infused continuously for 20 min into pulmonary venular capillaries using the venous microcatheter. Fluorescence images were obtained at 10-s intervals. For each image, four sets of frame-averaged exposures were obtained that alternated every 132 ms between excitations of 340 and 380 nm. EC [Ca2+]i was determined from the computer-generated 340/380 ratio based on a Kd of 224 nmol/l and appropriate calibration parameters (14, 35). EC [Ca2+]i oscillations were analyzed for amplitude and frequency using fast Fourier transformation (FFT; Origin 3.54, Microcal Software, Northampton, MA) (7). Data presented refer to the dominant wave component, i.e., the wave with highest amplitude, which we had previously identified to occur at the low-frequency end of the amplitude frequency spectrum (35). FFT analyses of imaging noise in our recording system, determined by recording fura 2 fluorescence 1) in unstimulated cultured bovine pulmonary artery EC (35), 2) in alveolar epithelial cells in situ, which do not exhibit spontaneous [Ca2+]i oscillations (1), or 3) in EC pretreated with the intracellular Ca2+ chelator 1,2-bis(2-aminophenoxy)ethane-N,N,N',N'-tetraacetic acid-AM, revealed wave components with amplitudes of <10 nmol/l. Hence, to exclude contamination from noise data, in the experimental FFT analyses, we rejected all wave components with an amplitude of <15 nmol/l. Capillary diameters were determined in triplicate from the 380-nm images as the perpendicular distance between longitudinal lines drawn through the endothelial midaxis.
Experimental protocols. 1) Pressure elevation: baseline recordings were obtained at PLA of 5 cmH2O. PLA was raised to 10, 15, or 20 cmH2O, respectively, for 30 min by adjusting the height of the venous outflow. 2) Inhibition of external Ca2+ entry: the trivalent lanthanide gadolinium (10 µM), which effectively blocks stretch-activated Ca2+ influx (16), was added to the perfusing blood 10 min before PLA elevation. 3) Gap junction uncoupling: heptanol (3 mM), the gap junctional uncoupler (9), was added to the perfusing blood 10 min before PLA elevation. 4) Combined inhibition of external Ca2+ entry and gap junction uncoupling: both gadolinium (10 µM) and heptanol (3 mM) were added to the perfusing blood 10 min before PLA elevation. 5) Ca2+-free conditions: infusion of nominally Ca2+-free HEPES solution containing 2% dextran and EGTA (0.5 mmol/l) through the venous microcatheter was started 10 min before PLA elevation.
Statistics. All data are means ± SE. Values of several groups were compared by Wilcoxon and Friedman tests for dependent groups and by Kruskal-Wallis and Mann-Whitney U-tests for independent groups. Spearman's coefficient of correlation, rs, was calculated to test correlation between parameters, and linear regression analysis was performed (SigmaPlot; Jandel Scientific, San Rafael, CA). Statistical significance was assumed at P < 0.05.
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RESULTS |
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We quantified EC [Ca2+]i in digitally imaged, single venular capillaries of the isolated blood-perfused rat lung. Baseline [Ca2+]i was determined at PLA of 5 cmH2O, which approximates physiological pressure in lung venular capillaries (5).
Increasing PLA from 5 to 20 cmH2O increased
mean EC [Ca2+]i and the amplitude of EC
[Ca2+]i oscillations. Both increases were
initiated after a lag of 3-5 min and continued progressively for
the 30-min pressure elevation period (Fig.
1). The oscillation frequency did not
change from baseline. Returning PLA to 5 cmH2O
reestablished baseline [Ca2+]i values in <2
min.
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To determine the effects of different levels of pressure increase, we
instituted PLA elevations to 10, 15, or 20 cmH2O in random order in each of which we held baseline
conditions for 15 min before pressure elevation. The resulting EC
[Ca2+]i increases at the end of each 30-min
pressure elevation period occurred in proportion to the imposed
pressure increase (Fig. 2).
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To determine the effect of external Ca2+ entry on these
responses, we instituted PLA elevations to 20 cmH2O while infusing capillaries with either gadolinium,
the inhibitor of cell membrane calcium channels, or
Ca2+-free HEPES. Both treatments inhibited the increase in
mean [Ca2+]i but not the increase in
[Ca2+]i oscillations (Fig.
3), indicating that amplitude increases were independent of external Ca2+ entry.
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Intercellularly propagating EC [Ca2+]i waves
were evident in these capillaries both during baseline and pressure
elevation (Fig. 4A). These
[Ca2+]i waves emanated from a specific subset
of EC located at the microvascular branch points, the "pacemakers,"
and were propagated to adjacent EC. As previously reported
(35), [Ca2+]i was 30% higher in
pacemaker, compared with nonpacemaker, EC (Fig. 4B). This
difference was also preserved when lungs were perfused with
Ca2+-free HEPES (data not shown, n = 6).
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To compare pressure responses of pacemaker vs. nonpacemaker EC, we determined the diameter increases at capillary branch-point and midsegmental locations. Pressure elevation from 5 to 20 cmH2O increased these diameters by 10 ± 2 and 38 ± 5%, respectively (Fig. 4B). This difference was statistically significant (P < 0.05), indicating that despite the equal pressure increase the increase of diameter was considerably less at branch points. Despite this difference, both [Ca2+]i oscillations and mean [Ca2+]i increased to the same extent at branch-point and midsegmental EC.
To determine the role of intercellular communication in these responses, we infused capillaries with the cell communication inhibitor heptanol. In the presence of heptanol, pressure-induced [Ca2+]i oscillations were blocked in midsegmental, but not in branch-point, EC (Fig. 4C), indicating that the oscillations originated in pacemaker EC and propagated to midsegmental EC through gap junctions. However, heptanol did not block the pressure-induced increase of mean [Ca2+]i in midsegmental or branch-point EC. When capillaries were infused with both heptanol and gadolinium, the [Ca2+]i response in midsegmental EC was completely abrogated (Fig. 4D).
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DISCUSSION |
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We show here that increasing lung vascular pressure enhanced the amplitude, but not frequency, of EC [Ca2+]i oscillations, while also increasing the mean EC [Ca2+]i. The enhanced oscillations were inhibited by heptanol in midsegmental but not in branch-point EC, indicating that the oscillations arose in branch-point pacemaker EC then propagated to adjacent EC by gap junctional communication. Importantly, neither gadolinium nor external Ca2+-free conditions blocked the enhanced oscillations in branch-point EC, indicating that the oscillations were driven by intracellular Ca2+ release and not by influx of external Ca2+. These findings indicate that, in EC in situ, pressure-induced cell stretch enhances Ca2+ oscillations.
Temporal profile. The ~5-min lag in the onset of these [Ca2+]i responses contrasts with the response in cultured EC in which mechanical stretch mobilizes Ca2+ within seconds (27, 30, 34). Although mechanisms are unclear, this lag was not due to delayed EC distortion since pressure-induced changes of capillary diameter are complete in <15 s (32). The lag may be protective since lung capillary EC are normally exposed to pressure pulsations transmitted from the arterial segment (3) and cyclic distortional stress during the breathing cycle (23). The lag exceeds the time course of these distortional fluctuations, thereby ensuring the absence of potentially deleterious EC [Ca2+]i increases during these physiological cycles. Processes that quickly restore baseline [Ca2+]i after relief of pressure stress may also be protective for similar reasons.
Sensitivity. Previous studies of lung hydrostatic stress indicate that pressure elevations of >50 cmH2O deteriorate the microvascular barrier (2, 28, 33), whereas more intermediate elevations to 20-50 cmH2O increase the capillary filtration coefficient (13, 29) and the transvascular protein flow (25). Here, we demonstrate that PLA increases of as little as 5 cmH2O are capable of generating second messenger responses in lung capillary EC. PLA elevation from 5 to 10 cmH2O dilates and, thereby, circumferentially stretches lung venular capillaries by ~10% (32). Our findings indicate that, in the lung, microvascular pressure elevations that were previously considered nonpathogenic (22, 29) activate an important endothelial signaling mechanism that is potentially proinflammatory.
Mechanotransduction. Because pressure-induced [Ca2+]i oscillations occurred both under external Ca2+-free conditions and in the presence of gadolinium, a nonspecific inhibitor of Ca2+ entry, we interpret the results to mean that the [Ca2+]i oscillations result from mobilization of intracellular Ca2+ stores, not entry of external Ca2+. Ca2+ release from intracellular stores is mediated via two different receptor families, the inositol 1,4,5-trisphosphate (IP3) receptors and the ryanodine receptors. In addition, depletion of intracellular Ca2+ stores causes capacitative entry of extracellular Ca2+ through store-operated channels in the plasma membrane (4). Pacemaker-generated [Ca2+]i oscillations in lung capillaries are propagated as intercellular endothelial waves through gap junctions (35), a mechanism previously attributed to the generation and intercellular communication of IP3 (6). Cultured EC subjected to cyclic stretch show increased phospholipase C activation leading to IP3 generation (8, 31) and IP3-mediated Ca2+ release from intracellular pools, which is not dependent on influx of extracellular Ca2+ (30). Hence, IP3-mediated Ca2+ release may account for the pressure-induced generation of EC Ca2+ oscillations.
In heptanol-treated midsegmental EC, in which [Ca2+]i oscillations are absent, the pressure-induced increase of mean EC [Ca2+]i was not impaired. Hence, it may be independent from store-operated, capacitative Ca2+ influx. Because the increase of mean [Ca2+]i was inhibited by both gadolinium and external Ca2+-free conditions, it resulted from entry of extracellular Ca2+.Pacemaker cells. Unexpectedly, diameter increases to pressure elevation varied regionally within the same capillary. Thus, for a pressure elevation from 5 to 20 cmH2O, the diameter increase at capillary branch points was markedly less than that at midsegments, yet pressure-induced [Ca2+]i transients were not different between these locations. These differential diameter responses suggest that pacemaker EC at branch points were stretched less than midsegmental EC. Nevertheless, they generated [Ca2+]i transients that were similar, suggesting that pacemaker EC may be more mechanosensitive to stretch.
Mechanotransduction in the capillaries was heterogeneous in that, although gadolinium-inhibitable channels were present in all EC, pressure-induced [Ca2+]i oscillations were exclusively generated in pacemaker EC and propagated to adjacent nonpacemaker EC by intercellular communication. This pressure-induced response pattern is essentially similar to that induced pharmacologically in lung capillaries. Thus histamine induces Ca2+ entry in both pacemaker and nonpacemaker EC but generates [Ca2+]i oscillations only in pacemaker EC (35). The oscillations are then propagated to adjoining EC through gap-junctional communication. The unique ability of pacemaker EC to generate [Ca2+]i oscillations is not explained. A rheological explanation may be considered, in that shear forces acting on the vascular wall may differ between branch points and midsegments. However, baseline diameters do not differ between these locations, and low Reynolds number flows in lung capillaries make turbulence at branch points unlikely (19). The issue may be addressed by direct study of pacemaker EC. However, methods for isolating this specific subset of EC have not been established. In conclusion, the present results indicate that increases of hydrostatic pressure evoke complex [Ca2+]i responses in lung capillary endothelium. Mean EC [Ca2+]i increases because of Ca2+ influx through membrane channels, whereas pacemaker-generated [Ca2+]i oscillations are induced presumably through store-release. Although the significance of this dual response remains unclear at present, we suggest that the rise of mean [Ca2+]i may provide the critical step that initiates secretion, for example, of P-selectin (21), or induces formation of nitric oxide by activating endothelial nitric oxide synthase (24). [Ca2+]i oscillations may activate mechanisms responsive to oscillation amplitude or frequency, as, for example, mitochondrial dehydrogenases (15), calmodulin-dependent protein kinases (11), or nuclear factor- ![]() |
ACKNOWLEDGEMENTS |
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This study was supported by National Heart, Lung, and Blood Institute Grants HL-57556, HL-36024, and HL-64896. W. M. Kuebler was a research fellow of the Deutsche Forschungsgemeinschaft.
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FOOTNOTES |
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Present address for W. M. Kuebler: Dept. of Physiology, Free University of Berlin, Arnimallee 22, 14195 Berlin, Germany.
Address for reprint requests and other correspondence: J. Bhattacharya, College of Physicians & Surgeons, St. Luke's-Roosevelt Hospital Center, 1000 10th Ave., New York, NY 10019 (E-mail jb39{at}columbia.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/ajplung.00275.2001
Received 24 July 2001; accepted in final form 19 December 2001.
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